CA1123437A - 3,4,5-trihydroxypiperidine compound, their production and their medicinal use - Google Patents
3,4,5-trihydroxypiperidine compound, their production and their medicinal useInfo
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- CA1123437A CA1123437A CA310,084A CA310084A CA1123437A CA 1123437 A CA1123437 A CA 1123437A CA 310084 A CA310084 A CA 310084A CA 1123437 A CA1123437 A CA 1123437A
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- desoxynojirimycin
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- C07—ORGANIC CHEMISTRY
- C07H—SUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
- C07H9/00—Compounds containing a hetero ring sharing at least two hetero atoms with a saccharide radical
- C07H9/02—Compounds containing a hetero ring sharing at least two hetero atoms with a saccharide radical the hetero ring containing only oxygen as ring hetero atoms
- C07H9/04—Cyclic acetals
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23K—FODDER
- A23K20/00—Accessory food factors for animal feeding-stuffs
- A23K20/10—Organic substances
- A23K20/116—Heterocyclic compounds
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23K—FODDER
- A23K20/00—Accessory food factors for animal feeding-stuffs
- A23K20/10—Organic substances
- A23K20/116—Heterocyclic compounds
- A23K20/132—Heterocyclic compounds containing only one nitrogen as hetero atom
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23K—FODDER
- A23K20/00—Accessory food factors for animal feeding-stuffs
- A23K20/10—Organic substances
- A23K20/116—Heterocyclic compounds
- A23K20/137—Heterocyclic compounds containing two hetero atoms, of which at least one is nitrogen
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- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23K—FODDER
- A23K50/00—Feeding-stuffs specially adapted for particular animals
- A23K50/30—Feeding-stuffs specially adapted for particular animals for swines
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P3/00—Drugs for disorders of the metabolism
- A61P3/08—Drugs for disorders of the metabolism for glucose homeostasis
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P3/00—Drugs for disorders of the metabolism
- A61P3/08—Drugs for disorders of the metabolism for glucose homeostasis
- A61P3/10—Drugs for disorders of the metabolism for glucose homeostasis for hyperglycaemia, e.g. antidiabetics
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P43/00—Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07D—HETEROCYCLIC COMPOUNDS
- C07D211/00—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings
- C07D211/04—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings with only hydrogen or carbon atoms directly attached to the ring nitrogen atom
- C07D211/06—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings with only hydrogen or carbon atoms directly attached to the ring nitrogen atom having no double bonds between ring members or between ring members and non-ring members
- C07D211/36—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings with only hydrogen or carbon atoms directly attached to the ring nitrogen atom having no double bonds between ring members or between ring members and non-ring members with hetero atoms or with carbon atoms having three bonds to hetero atoms with at the most one bond to halogen, e.g. ester or nitrile radicals, directly attached to ring carbon atoms
- C07D211/40—Oxygen atoms
- C07D211/44—Oxygen atoms attached in position 4
- C07D211/46—Oxygen atoms attached in position 4 having a hydrogen atom as the second substituent in position 4
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07D—HETEROCYCLIC COMPOUNDS
- C07D211/00—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings
- C07D211/04—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings with only hydrogen or carbon atoms directly attached to the ring nitrogen atom
- C07D211/06—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings with only hydrogen or carbon atoms directly attached to the ring nitrogen atom having no double bonds between ring members or between ring members and non-ring members
- C07D211/36—Heterocyclic compounds containing hydrogenated pyridine rings, not condensed with other rings with only hydrogen or carbon atoms directly attached to the ring nitrogen atom having no double bonds between ring members or between ring members and non-ring members with hetero atoms or with carbon atoms having three bonds to hetero atoms with at the most one bond to halogen, e.g. ester or nitrile radicals, directly attached to ring carbon atoms
- C07D211/60—Carbon atoms having three bonds to hetero atoms with at the most one bond to halogen, e.g. ester or nitrile radicals
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07H—SUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
- C07H15/00—Compounds containing hydrocarbon or substituted hydrocarbon radicals directly attached to hetero atoms of saccharide radicals
- C07H15/02—Acyclic radicals, not substituted by cyclic structures
- C07H15/12—Acyclic radicals, not substituted by cyclic structures attached to a nitrogen atom of the saccharide radical
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07H—SUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
- C07H15/00—Compounds containing hydrocarbon or substituted hydrocarbon radicals directly attached to hetero atoms of saccharide radicals
- C07H15/02—Acyclic radicals, not substituted by cyclic structures
- C07H15/14—Acyclic radicals, not substituted by cyclic structures attached to a sulfur, selenium or tellurium atom of a saccharide radical
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07H—SUGARS; DERIVATIVES THEREOF; NUCLEOSIDES; NUCLEOTIDES; NUCLEIC ACIDS
- C07H15/00—Compounds containing hydrocarbon or substituted hydrocarbon radicals directly attached to hetero atoms of saccharide radicals
- C07H15/18—Acyclic radicals, substituted by carbocyclic rings
Abstract
Abstract of the Disclosure The invention includes certain 3,4,5-trihydroxy-piperidine compounds, methods for their preparation, compositions containing said 3,4,5-trihydroxypiperidine compounds and methods for the use of said compounds and compositions.
The subject matter of the invention is useful against diabetes, hyperlipaemia and adiposity as well as in animal nutrition.
The subject matter of the invention is useful against diabetes, hyperlipaemia and adiposity as well as in animal nutrition.
Description
Z3'~3~
The present invention relates to certain new 3,4,5-trihydroxypiperidine compounds, to several processes for their production and to their use as medicaments, in particular as agents against diabetes, hyperlipaemia and adiposity, and in animal nutrition, for influencing the lean meat/fat ratio in favour of the proportion of lean meat.
The present invention provides compounds which are 3,4,5-trihydroxypiperidines of the following general formula or their pharmaceutically acceptable salts and bioprecursors:
3 \
~ N
HO \ r 2 HO OH
in which Rl and R3 are the same or different and each is H or alkyl having from l to 30 C atoms, alkenyl or alkinyl having from 2 to 18 C atoms, a monocyclic, bicyclic or tricyclic radical having from 3 to 10 C atoms, which is saturated, mono-unsaturated or di-unsaturated, aryl having 6 or 10 C atoms, or a heterocyclic radical having from 3 to 8 ring members which contains 1, 2, 3 or 4 heteroatoms and to which a benzene ring or a further said heterocyclic radical can be fused, each of the above groups being optionally substituted by from 1 to 5 substituents selected from the group consisting of hydroxyl;
alkoxy having from 1 to 4 carbon atoms; acyloxy, the acyl radical being derived from i) an aliphatic carboxylic acid having from 1 to 7 atoms or ~
ii) an aromatic carboxylic acid which optionally may be ;
substituted in the aromatic moiety by OH, halogen, nitro and/or amino or iii) a heterocyclic carboxylic acid whose heterocyclic B
~ -2- ~ :
343~
radical is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally being substituted in the heterocyclic moiety by Cl to C4-alkyl, chlorine, bromine or amino;
amino, mono- or dialkyl amino with 1 to 4 C-atoms in the alkyl radicals, monoacylamino, the acyl moiety being derived from i) an aliphatic Cl to C7-carboxylic acid or ii) an aromatic carboxylic acid optionally being substituted by OH, halogen, Cl to C4-alkyl, Cl to C4-alkoxy, nitro and/or amino or iii) a heterocyclic :
carboxylic acid optionally being substituted by Cl to C4-alkyl, chlorine, bromine or amino; mercapto or alkylthio having from 1 to 4 carbon atoms; halogen; alkylcarbonyl having from 1 to 4 carbon atoms in the alkyl moiety; carboxyl; nitro; cyano; an aldehyde group or a sulphonic acid group; a heterocyclic radical which is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally substituted in the heterocyclic moiety by Cl to C4 alkyl, chlorine, bromine or amino; a heterocyclic radical which is derived from a hexose or pentose, which is bonded to the alkyl moiety directly via a ring atom or via an -O-, -S- or -NH-bridge; naphthyl or phenyl, optionally having from 1 to 3, identical or different substituents each of which is -OH, ~NH2, Cl to C4-alkyl-NH-, Cl to C4-dialkyl-N-, Cl to C4-alkoxy, -NO2, -CN, -COOH, -COO-alkyl (Cl to C4), Cl to C6-alkyl, halogen, Cl to C4-alkylthio, -SH, Cl to C4-alkylsulphonyl, -SO3H, -SO2-NH2 and -SO2-NH-alkyl (Cl to C4); a monocyclic, bicyclic or tricyclic aliphatic substituent having from 3 to 10 carbon atoms, which in turn can be substituted by hydroxyl, amino, halogen or -COOH, and R2 is -H, -OH, -OR', -SH, -SR', -NH2, -NHR', -N ~
NH2CH2-, NHR'-CH2-, NRIR''-CH2-, -COOH, -COOR', HO-CH2-, R'CO-NHCH2-, R'CO-NR"CH2-, R'SO2NHCH2-, R'SO2-NR"CH2-~
~1 ~
i - ..
1~23~37 R~-NH-C-NH-CH2-, R'-NH-C-NH-CH- R'O-C-NH-CH - -SO H CN
-CONH2, -CONHR' or -CONR'R", wherein R'- and R" are the same or different and each has any of the meanings given above for Rl, provided that when R3 is -CH20H and R2 is H or OH; R3 is H and R2 is H, OH, SO3H, -CN or CH2-NH2; or R3 is -CH2-NH2 and R2 is OH, then R1 is other than hydrogen.
For the purpose of this specification the term 'pharmaceutically acceptable bioprecursor' of an active compound of the invention means a compound having a structural formula different from the active compound but which nonetheless, upon administration to a warm-blooded animal is converted in the patient's body to the active compound.
Suitable pharmaceutically acceptable salts are e.g.
chlorides, sulfates, acetates, carbonates and oxalates.
Rl, R' and R" are the same or different and preferably each is alkyl having from 1 to 30, desirably from 1 to 18, and more desirably from 1 to 10 C atoms, alkenyl or alkinyl having from 2 to 18, desirably from 3 to 10, C atoms, a monocyclic, bicyclic or tricyclic aliphatic radical having from 3 to 10 C
atoms, which can be saturated, mono-unsaturated or di-unsaturated, carbocyclic particularly cycloalkyl, cycloalkenyl or cycloalkinyl having 3 to 8 carbon atoms, such as cyclopentyl, cyclohexyl, -3a-B~ ~
~123437 cyclopentenyl, cyclohexenyl, cyclopentadienyl or cyclohexadienyl a~yl having 6 or 10 C atoms, such as phenyl or naphthyl, or a heterocyclic radical having from 3 to 8, in particular from 3 to 6, ring me~bers which can contain 1, 2, 3 or 4 hetero-atoms, each of which is preferably N, O or S, and to which a benzene ring or a further said heterocyclic radical can be fused, each of the akove groups being optionally substituted by from 1 to 5, most preferably by 1, 2 or 3, substituents.
Examples which may be mentioned of substituents for aIkyl are: hydroxyl, and aIkoxy having preferably from 1 to 4 carbon atoms, in p æ ticul æ methoxy and ethoxy; acyloxy, the acyl radical being derived from an aliphatic (particul æ ly alkane) carboxylic acid having from 1 to 7 C atoms, an aromatic carboxylic acid, most preferably a phenyl-carboxylic acid, such as benzoic acid, phthalic acid, etc, optionally substituted in the phenyl moiety by one, two or more of -OH, -halogen, preferably F, Cl or Br, Cl to C4-aIkyl, Cl to C4-alkoxy, nitro and/or amino, or a heterocyclic carboxylic acid which is derived from a 5-m~mkered or 6-~embered heterocyclic compound containing from 1 to 3 hetero-atoms each of which is N, O ~;
or S and optionally substituted in the heterocyclic ring moiety by Cl to C4-alkyl, chlorine, bromine or amino; amino, monoaIkylamino and dialkylamino having preferably from 1 to 4 carbon atoms in each alkyl moiety, m3st preferably mono~ethylamino, mon oe thylamino, di-methylamino and diethylamino, and monoacylamino, the acyl iety being derived from an aliphatic (particularly aIkane) carboxylic acid having f m m 1 to 7 C atoms, an aromatic carboxylic acid, most '., ' .~
1~39~37 preferably a phenyl-carboxylic acid, such as benzoic acid, phthalic acid, etc., optionally substituted in the phenyl moiety by -OH, -halogen, most preferably F, Cl or Br, Cl to C4-aIkyl, Cl to C4-alkoxy, nitro and/or am m o, or a heterocyclic carboxylic acid which is derived from a 5-m~mkered or 6-membered heterocyclic compound containing from 1 to 3 hetero-atoms each of which is N, O or S and optionally substituted in the heterocyclic ring moiety by Cl to C4-alkyl, chlorine, bromine or amino; me.rcapto, or alkylthio having preferably from 1 to 4 carbon atoms, in particular methylthio or ethylthio; halogen, preferably fluorine, chlorine or bromine; aIkyl-carbonyl having preferably from 1 to 4 carbon atoms in the alkyl moiety; carboxyl, nitro, cyano, an aldehyde group or a sulphonic acid group; or a heterocyclic radical of the above mentioned type, or m~st preferably, a heterocyclic radical which is derived from a sugar, preferentially from a hexose or pentose, which can be bonded to the aIkyl moiety directly via a ring atom or via an -C-, -S- or -NH- bridge.
Examples of heterocyclic substituents of the alkyl are:
phthalimido, pyridyl, thienyl, furyl, isoxazolyl, thiazolyl, glucopyranosyl, ribofuranosyl, oxiranyl and the like. Further suit- :
able substituents of the alkyl are aromatic radicals, such as naphthyl and in partic~Lar phenyl, optionally having one or more, preferably from 1 to 3, identical or different substituents each of
The present invention relates to certain new 3,4,5-trihydroxypiperidine compounds, to several processes for their production and to their use as medicaments, in particular as agents against diabetes, hyperlipaemia and adiposity, and in animal nutrition, for influencing the lean meat/fat ratio in favour of the proportion of lean meat.
The present invention provides compounds which are 3,4,5-trihydroxypiperidines of the following general formula or their pharmaceutically acceptable salts and bioprecursors:
3 \
~ N
HO \ r 2 HO OH
in which Rl and R3 are the same or different and each is H or alkyl having from l to 30 C atoms, alkenyl or alkinyl having from 2 to 18 C atoms, a monocyclic, bicyclic or tricyclic radical having from 3 to 10 C atoms, which is saturated, mono-unsaturated or di-unsaturated, aryl having 6 or 10 C atoms, or a heterocyclic radical having from 3 to 8 ring members which contains 1, 2, 3 or 4 heteroatoms and to which a benzene ring or a further said heterocyclic radical can be fused, each of the above groups being optionally substituted by from 1 to 5 substituents selected from the group consisting of hydroxyl;
alkoxy having from 1 to 4 carbon atoms; acyloxy, the acyl radical being derived from i) an aliphatic carboxylic acid having from 1 to 7 atoms or ~
ii) an aromatic carboxylic acid which optionally may be ;
substituted in the aromatic moiety by OH, halogen, nitro and/or amino or iii) a heterocyclic carboxylic acid whose heterocyclic B
~ -2- ~ :
343~
radical is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally being substituted in the heterocyclic moiety by Cl to C4-alkyl, chlorine, bromine or amino;
amino, mono- or dialkyl amino with 1 to 4 C-atoms in the alkyl radicals, monoacylamino, the acyl moiety being derived from i) an aliphatic Cl to C7-carboxylic acid or ii) an aromatic carboxylic acid optionally being substituted by OH, halogen, Cl to C4-alkyl, Cl to C4-alkoxy, nitro and/or amino or iii) a heterocyclic :
carboxylic acid optionally being substituted by Cl to C4-alkyl, chlorine, bromine or amino; mercapto or alkylthio having from 1 to 4 carbon atoms; halogen; alkylcarbonyl having from 1 to 4 carbon atoms in the alkyl moiety; carboxyl; nitro; cyano; an aldehyde group or a sulphonic acid group; a heterocyclic radical which is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally substituted in the heterocyclic moiety by Cl to C4 alkyl, chlorine, bromine or amino; a heterocyclic radical which is derived from a hexose or pentose, which is bonded to the alkyl moiety directly via a ring atom or via an -O-, -S- or -NH-bridge; naphthyl or phenyl, optionally having from 1 to 3, identical or different substituents each of which is -OH, ~NH2, Cl to C4-alkyl-NH-, Cl to C4-dialkyl-N-, Cl to C4-alkoxy, -NO2, -CN, -COOH, -COO-alkyl (Cl to C4), Cl to C6-alkyl, halogen, Cl to C4-alkylthio, -SH, Cl to C4-alkylsulphonyl, -SO3H, -SO2-NH2 and -SO2-NH-alkyl (Cl to C4); a monocyclic, bicyclic or tricyclic aliphatic substituent having from 3 to 10 carbon atoms, which in turn can be substituted by hydroxyl, amino, halogen or -COOH, and R2 is -H, -OH, -OR', -SH, -SR', -NH2, -NHR', -N ~
NH2CH2-, NHR'-CH2-, NRIR''-CH2-, -COOH, -COOR', HO-CH2-, R'CO-NHCH2-, R'CO-NR"CH2-, R'SO2NHCH2-, R'SO2-NR"CH2-~
~1 ~
i - ..
1~23~37 R~-NH-C-NH-CH2-, R'-NH-C-NH-CH- R'O-C-NH-CH - -SO H CN
-CONH2, -CONHR' or -CONR'R", wherein R'- and R" are the same or different and each has any of the meanings given above for Rl, provided that when R3 is -CH20H and R2 is H or OH; R3 is H and R2 is H, OH, SO3H, -CN or CH2-NH2; or R3 is -CH2-NH2 and R2 is OH, then R1 is other than hydrogen.
For the purpose of this specification the term 'pharmaceutically acceptable bioprecursor' of an active compound of the invention means a compound having a structural formula different from the active compound but which nonetheless, upon administration to a warm-blooded animal is converted in the patient's body to the active compound.
Suitable pharmaceutically acceptable salts are e.g.
chlorides, sulfates, acetates, carbonates and oxalates.
Rl, R' and R" are the same or different and preferably each is alkyl having from 1 to 30, desirably from 1 to 18, and more desirably from 1 to 10 C atoms, alkenyl or alkinyl having from 2 to 18, desirably from 3 to 10, C atoms, a monocyclic, bicyclic or tricyclic aliphatic radical having from 3 to 10 C
atoms, which can be saturated, mono-unsaturated or di-unsaturated, carbocyclic particularly cycloalkyl, cycloalkenyl or cycloalkinyl having 3 to 8 carbon atoms, such as cyclopentyl, cyclohexyl, -3a-B~ ~
~123437 cyclopentenyl, cyclohexenyl, cyclopentadienyl or cyclohexadienyl a~yl having 6 or 10 C atoms, such as phenyl or naphthyl, or a heterocyclic radical having from 3 to 8, in particular from 3 to 6, ring me~bers which can contain 1, 2, 3 or 4 hetero-atoms, each of which is preferably N, O or S, and to which a benzene ring or a further said heterocyclic radical can be fused, each of the akove groups being optionally substituted by from 1 to 5, most preferably by 1, 2 or 3, substituents.
Examples which may be mentioned of substituents for aIkyl are: hydroxyl, and aIkoxy having preferably from 1 to 4 carbon atoms, in p æ ticul æ methoxy and ethoxy; acyloxy, the acyl radical being derived from an aliphatic (particul æ ly alkane) carboxylic acid having from 1 to 7 C atoms, an aromatic carboxylic acid, most preferably a phenyl-carboxylic acid, such as benzoic acid, phthalic acid, etc, optionally substituted in the phenyl moiety by one, two or more of -OH, -halogen, preferably F, Cl or Br, Cl to C4-aIkyl, Cl to C4-alkoxy, nitro and/or amino, or a heterocyclic carboxylic acid which is derived from a 5-m~mkered or 6-~embered heterocyclic compound containing from 1 to 3 hetero-atoms each of which is N, O ~;
or S and optionally substituted in the heterocyclic ring moiety by Cl to C4-alkyl, chlorine, bromine or amino; amino, monoaIkylamino and dialkylamino having preferably from 1 to 4 carbon atoms in each alkyl moiety, m3st preferably mono~ethylamino, mon oe thylamino, di-methylamino and diethylamino, and monoacylamino, the acyl iety being derived from an aliphatic (particularly aIkane) carboxylic acid having f m m 1 to 7 C atoms, an aromatic carboxylic acid, most '., ' .~
1~39~37 preferably a phenyl-carboxylic acid, such as benzoic acid, phthalic acid, etc., optionally substituted in the phenyl moiety by -OH, -halogen, most preferably F, Cl or Br, Cl to C4-aIkyl, Cl to C4-alkoxy, nitro and/or am m o, or a heterocyclic carboxylic acid which is derived from a 5-m~mkered or 6-membered heterocyclic compound containing from 1 to 3 hetero-atoms each of which is N, O or S and optionally substituted in the heterocyclic ring moiety by Cl to C4-alkyl, chlorine, bromine or amino; me.rcapto, or alkylthio having preferably from 1 to 4 carbon atoms, in particular methylthio or ethylthio; halogen, preferably fluorine, chlorine or bromine; aIkyl-carbonyl having preferably from 1 to 4 carbon atoms in the alkyl moiety; carboxyl, nitro, cyano, an aldehyde group or a sulphonic acid group; or a heterocyclic radical of the above mentioned type, or m~st preferably, a heterocyclic radical which is derived from a sugar, preferentially from a hexose or pentose, which can be bonded to the aIkyl moiety directly via a ring atom or via an -C-, -S- or -NH- bridge.
Examples of heterocyclic substituents of the alkyl are:
phthalimido, pyridyl, thienyl, furyl, isoxazolyl, thiazolyl, glucopyranosyl, ribofuranosyl, oxiranyl and the like. Further suit- :
able substituents of the alkyl are aromatic radicals, such as naphthyl and in partic~Lar phenyl, optionally having one or more, preferably from 1 to 3, identical or different substituents each of
2' 1 C4 aIkyl-NH-, Cl to C -diaIkyl N C
C4-aLkoxy, N02, -CN, -OOOH, -COO-aIkyl (Cl to C4), Cl to & -aIkyl, halogen, most preferably fluorine, chlorine or bromine, Cl to C4-alkylthio, -SH, Cl to C4-alkylsulphonyl, -SO3H, -S02-NH2 and -S02-NH-alkyl (CL to C4).
.
- . , .
: . .
~ Z343~
The alkyl can also have a monocyclic, bicyclic or tri-cyclic aliphatic substituent having preferably from 3 to 10 carbon atoms, which in turn can be substituted by hydroxyl, amino, halogen, . most preferably fluorine, chlorine or bromine, or -COCH.
; The alkyl preferably is substituted by hydroxyl, alkoxy having from 1 to 4 carbon atoms, mercapto, alkylthio, havmg from 1 to 4 carbon atoms, halogen, nitro, amino, monoaIkylamino having fro~ 1 to 4 C atoms and acylamino, the acyl moiety being derived from an aliphatic carboxylic acid having from 1 to 6 C atoms.
Possible substituents for the monocyclic, bicyclic or tri-cyclic radicals ~, R' and R" are the substituents quoted herein-above for alkyl.
m e aryl radicals can have Qne or more, preferably from 1 ~; to 3, identical or different substituents. Ex~mples of substituents which may be mentioned æe: alkyl having from 1 to 10 C atoms, which can in turn themselves be substituted, for example by chlorine, nitro or cyano; optionally substituted aIkenyl having from 1 to 10 carbon ato~s; hydroxyl, aIkoxy having preferably from 1 to 4 carbon :~
atoms; amino, and monoalkylamino and di-aIkylamino having preferably from 1 to 4 OE bon atoms per aIkyl moiety; mercapto, and alkylthio having preferably from 1 to 4 carbon atoms; carboxyl, carbalkoxy having preferably from 1 to 4 carbon atoms, the sulphQnic acid group, aIkylsulphonyl having preferably from 1 to 4 carbon atoms and aryl-sulphonyl, preferably phenylsulphQnyl; aminosulphonylsulphonyl, and alkylaminosulphonyl and diaIkylaminosulphonyl having from 1 to 4 carbon atoms per aIkyl moiety, preferably methylaminosulphonyl and dimethylaminosulphonyl; nitro, cyano or the aldehyde group~ alkyl-- 6 - .~
. ~. ' .
' ' ; ~' ' ' ~ ' ~1~3~L3'7 cæbonylamino having preferably from 1 to 4 c æbon atoms; and alkyl-carbonyl having from 1 to 4 carbon atoms, benzoyl, benzylcæbonyl and p~enylethylc æbonyl, the last-mentioned alkyl, phenyl, benzyl and phenylethyl being in turn themselves optionally substitutedr for exa~!ple by chlorine, nitro or hydroxyl.
The heterocyclic radicals Rl are preferably derived from hetero-p æaffinic, hetero-aromatic or hetero-olefLnic 5-m~mbered or 6-membered rings having preferably from 1 to 3 identical or differ-ent hetero-atoms, each of which is oxygen, sulphur or nitrogen.
These ring systems can c æry further substituents, such as, for example, hydroxyl, amuno or Cl to C4-alkyl, or benzene or other, preferably 6-membered, heterocyclic rings of the type mentioned hereinabove can be fused to them.
P æticulæly preferred heterocyclic radicals are derived, for example, from furane, pyrane, pyrrolidine, piperidine, pyrazole, imidazole, pyrimidine, pyridazine, pyrazine, triazine, pyrrole, pyridine, benzimidazole, quinoline, isoquinoline or purine.
In the co~pounds of the formula I, R2 preferably repre-sents -H, -OH, -S03H, -CN, -CH2NH2, -CH2NH-(Cl to C14-alkyl), -CH2NH-c-(cl to C14-alkyl), -CH2-NH-S02(Cl to C14)-aLkyl or O :~
-CH2-NH-S02-phenyl. R2 very particularly preferably represents -H, -S03H or -CN.
R3 preferably represents hydrogen, -CH2-OH, -CH3, -CH2NH2, -CH2NH-(Cl to &-alkyl), -CH2NH-C-(Cl to C6-alkyl) or -CH2-0-O
(Cl-C6-alkyl). Eowever, R3 very particularly preferably represents
C4-aLkoxy, N02, -CN, -OOOH, -COO-aIkyl (Cl to C4), Cl to & -aIkyl, halogen, most preferably fluorine, chlorine or bromine, Cl to C4-alkylthio, -SH, Cl to C4-alkylsulphonyl, -SO3H, -S02-NH2 and -S02-NH-alkyl (CL to C4).
.
- . , .
: . .
~ Z343~
The alkyl can also have a monocyclic, bicyclic or tri-cyclic aliphatic substituent having preferably from 3 to 10 carbon atoms, which in turn can be substituted by hydroxyl, amino, halogen, . most preferably fluorine, chlorine or bromine, or -COCH.
; The alkyl preferably is substituted by hydroxyl, alkoxy having from 1 to 4 carbon atoms, mercapto, alkylthio, havmg from 1 to 4 carbon atoms, halogen, nitro, amino, monoaIkylamino having fro~ 1 to 4 C atoms and acylamino, the acyl moiety being derived from an aliphatic carboxylic acid having from 1 to 6 C atoms.
Possible substituents for the monocyclic, bicyclic or tri-cyclic radicals ~, R' and R" are the substituents quoted herein-above for alkyl.
m e aryl radicals can have Qne or more, preferably from 1 ~; to 3, identical or different substituents. Ex~mples of substituents which may be mentioned æe: alkyl having from 1 to 10 C atoms, which can in turn themselves be substituted, for example by chlorine, nitro or cyano; optionally substituted aIkenyl having from 1 to 10 carbon ato~s; hydroxyl, aIkoxy having preferably from 1 to 4 carbon :~
atoms; amino, and monoalkylamino and di-aIkylamino having preferably from 1 to 4 OE bon atoms per aIkyl moiety; mercapto, and alkylthio having preferably from 1 to 4 carbon atoms; carboxyl, carbalkoxy having preferably from 1 to 4 carbon atoms, the sulphQnic acid group, aIkylsulphonyl having preferably from 1 to 4 carbon atoms and aryl-sulphonyl, preferably phenylsulphQnyl; aminosulphonylsulphonyl, and alkylaminosulphonyl and diaIkylaminosulphonyl having from 1 to 4 carbon atoms per aIkyl moiety, preferably methylaminosulphonyl and dimethylaminosulphonyl; nitro, cyano or the aldehyde group~ alkyl-- 6 - .~
. ~. ' .
' ' ; ~' ' ' ~ ' ~1~3~L3'7 cæbonylamino having preferably from 1 to 4 c æbon atoms; and alkyl-carbonyl having from 1 to 4 carbon atoms, benzoyl, benzylcæbonyl and p~enylethylc æbonyl, the last-mentioned alkyl, phenyl, benzyl and phenylethyl being in turn themselves optionally substitutedr for exa~!ple by chlorine, nitro or hydroxyl.
The heterocyclic radicals Rl are preferably derived from hetero-p æaffinic, hetero-aromatic or hetero-olefLnic 5-m~mbered or 6-membered rings having preferably from 1 to 3 identical or differ-ent hetero-atoms, each of which is oxygen, sulphur or nitrogen.
These ring systems can c æry further substituents, such as, for example, hydroxyl, amuno or Cl to C4-alkyl, or benzene or other, preferably 6-membered, heterocyclic rings of the type mentioned hereinabove can be fused to them.
P æticulæly preferred heterocyclic radicals are derived, for example, from furane, pyrane, pyrrolidine, piperidine, pyrazole, imidazole, pyrimidine, pyridazine, pyrazine, triazine, pyrrole, pyridine, benzimidazole, quinoline, isoquinoline or purine.
In the co~pounds of the formula I, R2 preferably repre-sents -H, -OH, -S03H, -CN, -CH2NH2, -CH2NH-(Cl to C14-alkyl), -CH2NH-c-(cl to C14-alkyl), -CH2-NH-S02(Cl to C14)-aLkyl or O :~
-CH2-NH-S02-phenyl. R2 very particularly preferably represents -H, -S03H or -CN.
R3 preferably represents hydrogen, -CH2-OH, -CH3, -CH2NH2, -CH2NH-(Cl to &-alkyl), -CH2NH-C-(Cl to C6-alkyl) or -CH2-0-O
(Cl-C6-alkyl). Eowever, R3 very particularly preferably represents
3~3~
It has been found that the new compounds of the formula I
are potent inhibitors for ~-glucosidases, in p æ ticular for dis-accharidases~ The new co~lpounds are thus valuable agents for influ-encing a number of metabolic processes and thus constitute an enrichment of pharmacy.
Furthermore the compcunds of the foxmula I, especially those with ~=C6 to C10-n-alkyl are inhibitors for the trigylcerid and cholesterol absorption. Cc~,pared with 2-hydrox~nethyl-3,4,5-tri-hydrcxypiperidine, which is known fran DI'OS (German Published Specification) 2,656,602, the new compounds have advantageous ther-apeutic prcperties.
The present invention further provides a process for the production of a compound according to the invention in which a com-pound of the general fornNla II or IIa ,~
~3~3~
R - N - CH R. - N - OE1 ~: ~0 ~ ' ~ C~13 o ~
; CH3 ~,J
II IIa : in which Rl and R3 have the same meaning as defined hereinbefore in formula I, is subjected to acid hydrolysis so as to remove the isopropylidene or cyclo-hexylidene protective group, it sometimes keing advantageous to isolate the :. ca~pound of the formwla I in the form of an adduct of sulphurous acid or of hydrocyanic acid (R2 = SO3H or CN). me compounds of the formula I in which R2 is OH can be likerated fr the bisulphite addition products by treatment with bases, preferably alkaline earth metal hydroxides, such as Ca(OH)2 or Sr(OH)2, but most preferably Ba(OH)2. The compounds of the formula I in ~:
which R2 is H can be obtained from compounds of the formula I in which R2 is OH by reaction with hydrogen donor reducing agents, such as, for example, .
Furtherm~re, it has been found that a compound of the formLla I can be obtained when a oompound of the formula I in which R2 is OH is reacted ~ :
with hydrocyanic acid in a manner which is in itself knawn so as to produce a compound of the formula I in which R2 is CN, and a compound in which R2 is -CH2NH2 is optionally obtained from the products by catalytic hydrngenation of the nitrile group, and the amino group is optionally acylated, alkylated or sulphonylated in a m~nner which is in itself knawn so as to produce a cam-pound of the formula I in which R2 is R'CCNHCH2-, R'CCNR''CH2-, NHR'-CH2-, NR'R" -CH2- or R'SO2NHOE12-, wherein R' and R" have the same meaning as de-fined hereinbefore in formula I.
A campound of the formula I in which R2 is -OR', -SH, -SR', -NUI2, _ g _ . . - :. : . -:: . ; ; , . , . ,: ; ; ,-. . :: -~3~
-NHR' or -NR' R" can be obtained by reacting a compound of the formula I in which R2 is -OH with an alcohol (R'OH), H2S, mercaptan (R'SH), a~monia or amLne (H2NR' or HNR' R' ' ), wherein R' and R" have the same meaning as defined hereinbefore in formula I in a manner which is in itself known.
A ccmpound of the formula I in which R2 is -COOH may be obtained by hydrolysis of a compound of the formula I in which R2 is -CN in a manner which is in itself known.
In a manner which is in itself known, a compound of the formula I
in which R2 is -COOR' may be obtained from the resulting carboxylic acid by reaction with an alcohol (R'OH), and a ccnpound of -the formula I in which is -aCNHR' or -aONR'R' ' or - 0 NH2 may be obtained by aminolysis of a result-ing ester with NH3, R'NH2 or R'R' 'NH, wherein R' and R" have the same mean-ing as defined hereinbefore in formula I.
A compound of the formula I in which ~ is -OH may also be obtained when a compound of the formula II is reacted with trifluoroa oe tic anhydride (reaction step A) so as to produ oe a oompound of the formula III, the iso-propylidene protective group being then split off by acid hydrolysis (reac-tion step B) and the trifluoroa oe tyl group in the compound IV is subsequently re~Dved in a neutral to alkaline reaction medium (reaction step C).
The reaction sequence indicated may be illustrated as follows:
: R3 R13 Rl - N - CH Rl - N - CH
It has been found that the new compounds of the formula I
are potent inhibitors for ~-glucosidases, in p æ ticular for dis-accharidases~ The new co~lpounds are thus valuable agents for influ-encing a number of metabolic processes and thus constitute an enrichment of pharmacy.
Furthermore the compcunds of the foxmula I, especially those with ~=C6 to C10-n-alkyl are inhibitors for the trigylcerid and cholesterol absorption. Cc~,pared with 2-hydrox~nethyl-3,4,5-tri-hydrcxypiperidine, which is known fran DI'OS (German Published Specification) 2,656,602, the new compounds have advantageous ther-apeutic prcperties.
The present invention further provides a process for the production of a compound according to the invention in which a com-pound of the general fornNla II or IIa ,~
~3~3~
R - N - CH R. - N - OE1 ~: ~0 ~ ' ~ C~13 o ~
; CH3 ~,J
II IIa : in which Rl and R3 have the same meaning as defined hereinbefore in formula I, is subjected to acid hydrolysis so as to remove the isopropylidene or cyclo-hexylidene protective group, it sometimes keing advantageous to isolate the :. ca~pound of the formwla I in the form of an adduct of sulphurous acid or of hydrocyanic acid (R2 = SO3H or CN). me compounds of the formula I in which R2 is OH can be likerated fr the bisulphite addition products by treatment with bases, preferably alkaline earth metal hydroxides, such as Ca(OH)2 or Sr(OH)2, but most preferably Ba(OH)2. The compounds of the formula I in ~:
which R2 is H can be obtained from compounds of the formula I in which R2 is OH by reaction with hydrogen donor reducing agents, such as, for example, .
Furtherm~re, it has been found that a compound of the formLla I can be obtained when a oompound of the formula I in which R2 is OH is reacted ~ :
with hydrocyanic acid in a manner which is in itself knawn so as to produce a compound of the formula I in which R2 is CN, and a compound in which R2 is -CH2NH2 is optionally obtained from the products by catalytic hydrngenation of the nitrile group, and the amino group is optionally acylated, alkylated or sulphonylated in a m~nner which is in itself knawn so as to produce a cam-pound of the formula I in which R2 is R'CCNHCH2-, R'CCNR''CH2-, NHR'-CH2-, NR'R" -CH2- or R'SO2NHOE12-, wherein R' and R" have the same meaning as de-fined hereinbefore in formula I.
A campound of the formula I in which R2 is -OR', -SH, -SR', -NUI2, _ g _ . . - :. : . -:: . ; ; , . , . ,: ; ; ,-. . :: -~3~
-NHR' or -NR' R" can be obtained by reacting a compound of the formula I in which R2 is -OH with an alcohol (R'OH), H2S, mercaptan (R'SH), a~monia or amLne (H2NR' or HNR' R' ' ), wherein R' and R" have the same meaning as defined hereinbefore in formula I in a manner which is in itself known.
A ccmpound of the formula I in which R2 is -COOH may be obtained by hydrolysis of a compound of the formula I in which R2 is -CN in a manner which is in itself known.
In a manner which is in itself known, a compound of the formula I
in which R2 is -COOR' may be obtained from the resulting carboxylic acid by reaction with an alcohol (R'OH), and a ccnpound of -the formula I in which is -aCNHR' or -aONR'R' ' or - 0 NH2 may be obtained by aminolysis of a result-ing ester with NH3, R'NH2 or R'R' 'NH, wherein R' and R" have the same mean-ing as defined hereinbefore in formula I.
A compound of the formula I in which ~ is -OH may also be obtained when a compound of the formula II is reacted with trifluoroa oe tic anhydride (reaction step A) so as to produ oe a oompound of the formula III, the iso-propylidene protective group being then split off by acid hydrolysis (reac-tion step B) and the trifluoroa oe tyl group in the compound IV is subsequently re~Dved in a neutral to alkaline reaction medium (reaction step C).
The reaction sequence indicated may be illustrated as follows:
: R3 R13 Rl - N - CH Rl - N - CH
-4 4 ~ CH3 ~ CH3 R - N - CH
D 4 ~ OH
: OH
~ N ~ 1 D HO ~ HOH
HO HO
In the above formulae, Rl and R3 have ~he same meaning as de~ined hereinbefore in formula I, and R4 iS trifluoroa oe tyl and R5 is trifluoroa oe tyl or hydrogen.
An analogous reaction sequen oe is applicable to the compounds of the formula IIa.
~i~3~3~ `
It has also been found that a compound of the formula I
can be obtained when a compound of the general formula V
3\, NH
2 :
/~ V
OH OH
wherein R2 and R3 have the same meaning as defined hereinbefore in formula I, is reacted with a carbonyl compound of the general formula VI
O = C \ VI
in which R6 and R7, together with the carbon atom to which they are attached and a hydrogen atom, form the group Rlj in the presence of a hydrogen donor reducing agent, for example formic acid.
A compound of the formula I in which R2 is H may also be obtained by reaction of: :
an amide of the following general formula VII or a derivative thereof with hydroxyl-protective groups ,.,:
R~\~ 8 :~
r N VII
HO
HOOH
~ '"~, ;
~Z3~7 in which R3 has the same meaning as defined hereinbefore in formula I and R8 has the same possible meanings as given for R
in formula I, or a carbamate of the following general formula VIII or a derivative thereof provided with hydroxyl protective groups N - ICl - O - Alkyl ~ O VIII
HO HO
is reduced to the corresponding amine with an amide-reducing agent.
A further process for the preparation of compounds of the formula I comprises reaction of a compound of the formula V
with a reactive alkylating agent of the formula IX
wherein Rl is as defined above and Z is an easily eliminated leaving group, such as, for example, halide or ~O-SO3H, which is customary in alkylating agents.
In addition, in a compound of the formula I in which R3 is -CH2OH, the -CH2OH group can be selectively converted 2 2 ~ CH3 group in a manner which is in itself known and this then either converted into a -CH3 group by reduction or into an amino group by reduction, via a -CH2-N3 group. Compounds of the formula I may also be B~ ~
. .
. ~ . ...
~12343~
cbtained when, in a compound of the foll~ula I in which R3 is -CH2-NH2, deriva-tives of the amino group, are prepared by reaction with aldehydes or ketones in the presence of a hydrogen donor or with carboxylic acid chlorides or sul-phonic acid chlorides, chlorocarbonic acid esters, isocyanates, isothiocya-nates, and alkyl halides, in a manner which is in itself known.
Ccmpounds of the formula I in which ~ is an aliphatic or aromatic radical which is substituted by an acyla~Lno, sulphonylamino, alkoxycarbonyl-amino, ureido or thioureido group can be obtained starting from compounds of the formula I in which ~ is an aliphatic or aromatic radical which is sub-stituted by an amino group, by reacting this anino group with a carboxylicacid chloride or sulphonic acid chloride or with a chlorocarbonic acid ester, isocyanate or isothiocyanate in a manner which is in itself kncwn.
m e individual procedures for the preparation of the active com~
pounds according to the invention are illustrated, by way of example only, below:
If a compound of the formula II in which ~ is ethyl is used as a starting material, the course of a suitable reaction can be represented as follows:
HOCH
1 2 $2/H2 CH OH
H5C2 - N - C - H ~ -D ~2 H ~ H
H ~ o -CH3-C-CH3 ~ N~ 2 5 HO ~ SO
~, , ;
-- ~31.Z3~a3~
Ba(CH)2 \~N,C2H5 ~ "C2H5 -BaSO3 b HO ~ Pt/H2 ~ >
H20 /~\
OH OH OH OH
If l-desoxynojirimycin ~the compound of the general formula V in which R2 is hydrogen and R3 is -CH20H) and formaldehyde are used as starting materials, a suitable reaction can be represented as follows CH2OH .
NH OcH2/HcooH CH2H CH
HO ~ - H20 ~ HO ~
HO OH HO OH
If benzaldehyde is used as the carbonyl component, reductive alkylation may be carried out as follows:
~ NH NaBH3CN ~ -N - CH
HO - ~ + OCH ~ MeoH-- ~ HO ~ 2 OH OH OH OH
~; '.
,.... .
~Z3437 If an acid amide of the general formula VII is used as starting material, a suitable reaction can be described as follows:
~ N - C - CH2 - CH2 - CH2 - CH3 HO ~ > o NaBH3(~C~CF3) D
~ Dioxan OH OH
,20H
~ 2 2 2 3 HO ~
OH OH
Urethanes of the general formula VIII, optionally in the form of derivatives provided with hydroxyl-protective groups, may be reduoe d to N- ~.methyl-l-desoxynorjirimycin with LiAlH4:
' :~
CH20H CH~OH
~ N - CO - OC H ~ N - CH3 HO ~ LiAlH4 HO ~
OH OH OH OH ~ ~`
For the reaction of l-desoxynorjirimycin with an aIkylating agent, the reaction with allyl bromide can be indicated by way of example as follows:
,' 3~L37 HO ~ + Br - CH2 - CH = CH2 H-B---{>
OH OH
CH20H -.
~ N - CH - CH = CH
HO~
OH OH
Same of the compounds of the formula II used as starting materials are known. This is the case where R3 ~s H, -CH20H or -CH2NH2 and RL is H-Other compounds of the formula II or IIa are new; however, they can be pre-pared from compounds which are known from the literature by processes which are in themselves known.
m uS, for example, it is possible to use the compound of the forn~iLa X, which is known fram the literature, ~/ ~ O X
as a starting materia:L and to react this with a carbonyl cc~pcund of the fornLiLa Vl in the presence of a hydrogen donor reducing agent so as to pro-duce a compound of the formula II.
Furthermorer it is possible to react the ccmpcund X with reactive acid derivative so as to produce an acid amide or urethane and to reduce this to an amine with an amide-reducing agent.
~ - 17 -.. :. .~ . : :
~Z3~3~
This can ~e illustrated by the follcwing example:
HO ~ HOCH2 H N - CH Cl-C-C2H5 H5C2 1I N ~ o C~33 H 1 2 C13 LiAlH4 ~ o ~ H3 m e compound of the formula X can also be reacted with reactive alkylating agents of the following general formula IX as defined hereil~before Z ~
so as to produce a compound of formula II.
Et:tlYYcm~re, in the above mentioned reactions, instead of the com~
pound X it is also possible to employ kncwn partially protected derivatives of the formula XI ~
' 2 `
H2N - C ~ CH2 ~ XI
3 ;:
and then to remove the trityl and benzyl protective groups in a known manner, for example with sodium in liquid ammonia. To prepare compounds of the formLla II, it is also possible to react the compound of fonmula XII, which is likewise kncwn frcm the literature, . . ' . . , , : ~, . ~, , . , ~ , ~1~343~
Tr ~ -C~
with an amine of the general formula XIII
~ - NH2 XIII
wherein ~ has the same meaning as defined hereinbefore in formula II, in the presen oe of a hydrogen donor reducing agent, for example in the presence of NaBH3CN. As a rule, a diastereomer mixture is formed in this reaction. m e diastereomer which is not desired may be appropriately separated off at this stage or at a later stage by the custcmary chrcmatographic methods or by fractional crystalliza-tion. Finally, the trityl and benzyl protective groups can be split off in a known way, for example with sodium in liquid ammonia. -~
Moreover, new compounds of the formula II or IIa can also be obtained by reaction of one or more of the degradation products of D-glucose, which are kncwn from the literature, of the formulae XIV to XVI
... . . ~ .. : . ~ .
.. ~ . ... .
~2343~
O = C~ ~ O - CH ~ = C~ ~ C~2 ~
~ CH3 ~ ~ ~ CH3 ~ n:v xV XVI
with an appropriate reagent having a carbanion character, such as, for exa~,ple, aIkyl-Li or Grignard compounds or the Li salt of 1,3-dithiane, so as to introduce a group R3 as defined hereinkefore in formula I, and converting the resulting comFound(s) of formula XVII
XVII
~ CH3 3 -.
in which R3 has the same meaning as defined hereinkefore in formula I, into the corresponding amine(s~ in a m~nner which is in itself kncwn [S. INOUYE et al., Tetra~edron 23, 2125-2144] via the ketone and the oxime, whereupon, as a rule, a mixture of the gluco com, pound and ido compound forms, fr~m which the desired gluco compound of formula x~III
:
~Z343~
H N - CH 2 ~
XVIII
~ CH3 in which R3 has the same meaning as defined immediately hereinbefore, can be isolated by customary chromatographic methods.
R~moval of the benzyl protective group conveniently by catalytic hydrcgenation or with Na in liquid NH3, then gives the corresponding comr pound(s) of the formula II.
Ccmpounds of the fonmula XIX (belcw) can be obtained when an apprD-priate aldehyde of any of the formulae XIV to XVI is reacted with an appropri-ate amine and hydrocyanic acid in a n~nner which is in itself kncwn so as to produoe an aminonitrile thereby introducing a group Rl as defined herein-before in formula I. mus for example a compound of formula XVI is reacted to produce a oompound of formula XIX
CN
Rl - N,HC 2 ~
XIX
~ .
Z3~37 wherein ~ has the same meaning as defined hereinbefore in formula I, and in this case also, as a rule, the desired gluco compound must be separated off from the ido compound by customary chromato-graphic methods. Further conversion of the nitrile group by hydro-genation or hydrolysis before or after the removal of the benzyl protective group leads to further compounds of the formula II.
The reaction of a co~,pound of forn~la XIV, XV or XVI with a CH-acid comçound, such as, for example, a nitroalkane, aIkyl-nitrile, CH-acid ester or ketone can also lead to compounds of the formula II. In this case, unsaturated compounds, for example com-pounds of the formula XX, can be obtained:
X,Y
C ~'' CH
XX
0~ ~
wherein X is -N02, -CN or -CCOaIkyl, and Y is H, alkyl or aryl, either directly or by dehydration of the aldol addition product, and these compol~nds yield compounds of the formula IIa by a Michael addition reaction with an amine, after chromatographic separation of gluco and ido isomers.
The isopropylidene protective group can be split off from a compound of the formula II in a moderately strongly acid to : .
.
. .
~IZ3~37 weakly acid solution, preferably at a pH in the range from 1 to 4, in aqueous solution or in a water-miscible, water-containing organic solvent. Acids which can be used are dilute mineral acids, such as, for example, sulphuric acid, or also organic acids, such as a oe tic acid. The reaction is preferably carried out under atmos-pheric pressure and at a temperature from room temperature to the boiling point of the solvent.
In order to work up the reaction mixture, the acid is desirably neutralized and separated off as a salt or with the aid of a basic ion exchanger. The isolation of the compounds of formula I in which R2 is OH may then appropriately be effected by careful removal of the solvent, for example by lyophilisation.
A preferred embodiment of the pro oe ss of splitting off of the isopropylidene protective group from a conpound of the formula II comprises saturation of the aqueous or water-containing alcoholic solution of the compound of the formula II with SO2 and storing the saturated solution at a temperature of from 20 to 50C
for several days. The ccmpounds of the formula I can then be ob, tained as bisulphite adducts (R2 = -SO3H), which in most cases readily crystallize, from which the comFounds of the formula I can be liberated with the aid of, for example, aqueous Ba(OH)2.
A compound of the formula I in which R2 is OH can be re-duced to a ccmpound of the formula I in which R2 is H by using an aIkali metal borohydride, alkali metal cyanoborohydride or dialkyl-aminoborane. It is preferable to use sodium borohydride in aqueous ~;, solution or in a water-miscible water-containing organic solvent, - . . . - . ~ . , ~. . .i .
,. . . , ~
~3~37 such as, for example, dioxane, at room temperature or optionally elevated temperature. However, the reduction is very particularly preferably carried out catalytically with Pt or Pd as the catalyst or in the presence of Raney Ni. In this pro oe dure, it is preferably carried out in an aqueous solution at room temperature.
Compounds of the formula I are further obtained from oompounds of the formula CHyl CE3 R ~ - N - CH~ (XX:[ ) OH
by hydrolysis with strong mineral acid of pH <1 at -20 to +20& and sub-sequent hydrogenation at pH 4 to 6 with for instance H2/Raney-Nickel, H2~P+O2 or sodium borohydride.
The oompound of the formNla XXI can be prepared from compounds of the formLla yO
1~ o ~ : :, R O - CH ~
wherein ~ is hydrogen or acetyl and ~ 0 is mesyl or tesyl, by reaction with amines of the formula Rl - NH2 at 20 to 150C in a polar solvent, e.g. an alcohol, dimethylsulfoxide or in an excess of the amune.
.. ~ . .
~Z3~3~
The starting material of the general formula V, in which R3 is -CH2CH, is known and can be obtained either by eatalytie hydrogenation of nojirimyein, which is obtainable by fermentation ~S. INOU~ et al., Tetrahedron 23, 2125-2144 (1968)], or by extrac-tion from mulberry tree bark (see ~T-OS (German Published Specifica-tion) 2,656,602), or entirely synthetically. l-Desoxynojirimyein can also be conveniently prepared by a new advantageous process com-prising cultiva~ing an organism of the Bacillaeeae family in a custcmary fer~entation vessel in a customary nutrient medium at a temperature of fr~m about 15 to about 80& for from about 1 to about 8 days, with aeration, oentrifuging off the cells and isolat-ing the desoxy cGmpcund from the culture broth or the cell extracts by a customary purifieation process (see Germ~n Patent Applieation P 26 58 563.7).
m e carbonyl compounds of the formula VI are either known or can be prepared by standard processes. Typical examples which may be mentioned and preferably contain up to 8 earbon atoms, are:
straight-chain or branehed alkylaldehydes, such as formaldehyde, aoetaldehyde, n-propanal, n-butanal, 2-methylpropanal, n-pentanal, 2-methylbutanal, 3-methylbutanal, 2,2-dimethyl-propanal, n-hexanal, 2-ethylbutanal, n-heptanal and n-octanal; alkenylaldehydes, such as ~.
prcpenal, 2-methylpropenal, 2-butenal, 2-methyl-2-butenal and ... . . .... . ... .. .
~23~37 2-ethyl-2-hexenal; cyclie (particularly cyeloaIkyl aldehydes) aldehydes, such as eyclopropanecarbaldehyde, cyclopentanecarbal-dehyde, eyclopentaneacetaldehyde and cyclohexanecarbaldehyde;
benzaldehyde, o-, ~r and p-toluenecarbaldehyde and phenylacetal-dehyde; straight-ehain and branehed alkylaldehydes whieh are sub-stituted by hydroxyl, such as 5-hydroxypentanal, 2-hydro~y-3-methyl-butanal, 2-hydroxy-2-methylpropanal, 4-hydroxybutanal, 2-hydroxy-propanal and 8-hydroxyoctanal; straight-chain and branched alkyl- ~; ;
aldehydes which are substituted by amino, such as 5-aminopentanal, 2-aminopropanal, 3-aminopropanal, 4-aminobutanal, 2-amino-3-methyl-butanal, 8-amino-octanal and mono-N-alkyl derivatives thereof; and straight-chain and branched alkylaldehydes whieh are disubstituted by amino and hydroxyl, such as 2-hydroxy-5-aminopentanal, 3-hydroxy-3-methyl-4-aminobutanal, 2-hydroxy-4-aminobutanal, 2-hydroxy-3-aminopropanal, 2-hydroxy-2-methyl-3-aminopropanal, 2-amino-3-hydroxyoctanal and mono-N-alkyl derivatives, particularly Cl-C8-N-aIkyl, thereof.
F`urthermore: methoxy-a oe taldehyde, ethoxy-acetaldehyde, n-propoxy-acetaldehyde, i-propoxy-a oe taldehyde, n-butoxy-a oe tal- ~ -dehyde, i-butoxy-a oe taldehyde, tert.-butoxy-acetaldehyde, cyelo-prcpylmethoxy-aoe taldehyde, cyclopropoxy-acetaldehyde, 2-methoxy- ~ ;
ethoxy-acetaldehyde, 2-ethoxy-ethoxy-a oe taldehyde, 2-methoxy (l-methyl-ethoxy)-a oe taldehyde, 2-ethoxy(l-methyl-ethoxy)-aoe tal-dehyde, phenoxy-a oe taldehyde, 2-methoxy-2-methyl-a oe taldehyde, 2-ethoxy-2-methyl-a oe taldehyde, 2-n-propoxy-2-methyl-a oe taldehyde, 2-(i-propoxy)-2-methyl-a oe taldehyde, 2-(n-butoxy)-2-methyl-aoe tal-dehyde, 2-(i-butoxy)-2-methyl-acetaldehyde, 2-(tert.-butoxy)-2-methyl-a oe taldehyde, 2-cyclopropylmethoxy-2-methyl-acetaldehyde, :' .
1~23~37 2-cyclopropoxy-2-methyl-acetaldehyde, 2-methoxy-ethoxy-a-methyl-acetaldehyde, 2-ethoxy-ethoxy-a-methyl-acetaldehyde, 2-methoxy-(l-methyl-ethoxy)-a-methyl-acetaldehyde, 2-methoxy-2,2-dimethyl-a oe taldehyde, 2-ethoxy-2,2-dimethyl-a oetaldehyde, 2-cyclopropyl-methoxy-a oe taldehyde, 2-~-butoxy-2,2-dimethyl-acetaldehyde, methyl-thio-acetaldehyde, ethylthio-acetaldehyde, n-propylthio-acetal-dehyde, i-propylthio-acetaldehyde, cyclopropyl-methylthio-aoe tal-dehyde, 3-methoxy-propanal, 3-ethoxy-propanal, 3-n- and 3-i-propoxy-propanal, 3-n-, 3-i- and 3-tert.-butoxy-propanal, 3-cyclopropoxy-propanal, 3-cyclopropylmethoxy-propanal, 3-methoxy-3-methyl-pro-panal, 3-ethoxy-3-methyl-propanal, 3-n- and 3-i-propoxy-3-methyl-propanal, 3-n-, 3-i- and 3-tert.-butoxy-3-methyl-propanal, 2,3- and 4-methoxy-butanal, 2-,3- and 4-ethoxy-butanal, 2-methylthio-pro-panal, 2-ethylthio-propanal, 3-methylthio-propanal, 3-ethylthio-propanal, 2-methylthio-butanal, 3-methylthio-butanal, 4-methylthio-butanal, furfurol, tetrahydrofurfurol, thiophene, 5-bromo-thiophene,
D 4 ~ OH
: OH
~ N ~ 1 D HO ~ HOH
HO HO
In the above formulae, Rl and R3 have ~he same meaning as de~ined hereinbefore in formula I, and R4 iS trifluoroa oe tyl and R5 is trifluoroa oe tyl or hydrogen.
An analogous reaction sequen oe is applicable to the compounds of the formula IIa.
~i~3~3~ `
It has also been found that a compound of the formula I
can be obtained when a compound of the general formula V
3\, NH
2 :
/~ V
OH OH
wherein R2 and R3 have the same meaning as defined hereinbefore in formula I, is reacted with a carbonyl compound of the general formula VI
O = C \ VI
in which R6 and R7, together with the carbon atom to which they are attached and a hydrogen atom, form the group Rlj in the presence of a hydrogen donor reducing agent, for example formic acid.
A compound of the formula I in which R2 is H may also be obtained by reaction of: :
an amide of the following general formula VII or a derivative thereof with hydroxyl-protective groups ,.,:
R~\~ 8 :~
r N VII
HO
HOOH
~ '"~, ;
~Z3~7 in which R3 has the same meaning as defined hereinbefore in formula I and R8 has the same possible meanings as given for R
in formula I, or a carbamate of the following general formula VIII or a derivative thereof provided with hydroxyl protective groups N - ICl - O - Alkyl ~ O VIII
HO HO
is reduced to the corresponding amine with an amide-reducing agent.
A further process for the preparation of compounds of the formula I comprises reaction of a compound of the formula V
with a reactive alkylating agent of the formula IX
wherein Rl is as defined above and Z is an easily eliminated leaving group, such as, for example, halide or ~O-SO3H, which is customary in alkylating agents.
In addition, in a compound of the formula I in which R3 is -CH2OH, the -CH2OH group can be selectively converted 2 2 ~ CH3 group in a manner which is in itself known and this then either converted into a -CH3 group by reduction or into an amino group by reduction, via a -CH2-N3 group. Compounds of the formula I may also be B~ ~
. .
. ~ . ...
~12343~
cbtained when, in a compound of the foll~ula I in which R3 is -CH2-NH2, deriva-tives of the amino group, are prepared by reaction with aldehydes or ketones in the presence of a hydrogen donor or with carboxylic acid chlorides or sul-phonic acid chlorides, chlorocarbonic acid esters, isocyanates, isothiocya-nates, and alkyl halides, in a manner which is in itself known.
Ccmpounds of the formula I in which ~ is an aliphatic or aromatic radical which is substituted by an acyla~Lno, sulphonylamino, alkoxycarbonyl-amino, ureido or thioureido group can be obtained starting from compounds of the formula I in which ~ is an aliphatic or aromatic radical which is sub-stituted by an amino group, by reacting this anino group with a carboxylicacid chloride or sulphonic acid chloride or with a chlorocarbonic acid ester, isocyanate or isothiocyanate in a manner which is in itself kncwn.
m e individual procedures for the preparation of the active com~
pounds according to the invention are illustrated, by way of example only, below:
If a compound of the formula II in which ~ is ethyl is used as a starting material, the course of a suitable reaction can be represented as follows:
HOCH
1 2 $2/H2 CH OH
H5C2 - N - C - H ~ -D ~2 H ~ H
H ~ o -CH3-C-CH3 ~ N~ 2 5 HO ~ SO
~, , ;
-- ~31.Z3~a3~
Ba(CH)2 \~N,C2H5 ~ "C2H5 -BaSO3 b HO ~ Pt/H2 ~ >
H20 /~\
OH OH OH OH
If l-desoxynojirimycin ~the compound of the general formula V in which R2 is hydrogen and R3 is -CH20H) and formaldehyde are used as starting materials, a suitable reaction can be represented as follows CH2OH .
NH OcH2/HcooH CH2H CH
HO ~ - H20 ~ HO ~
HO OH HO OH
If benzaldehyde is used as the carbonyl component, reductive alkylation may be carried out as follows:
~ NH NaBH3CN ~ -N - CH
HO - ~ + OCH ~ MeoH-- ~ HO ~ 2 OH OH OH OH
~; '.
,.... .
~Z3437 If an acid amide of the general formula VII is used as starting material, a suitable reaction can be described as follows:
~ N - C - CH2 - CH2 - CH2 - CH3 HO ~ > o NaBH3(~C~CF3) D
~ Dioxan OH OH
,20H
~ 2 2 2 3 HO ~
OH OH
Urethanes of the general formula VIII, optionally in the form of derivatives provided with hydroxyl-protective groups, may be reduoe d to N- ~.methyl-l-desoxynorjirimycin with LiAlH4:
' :~
CH20H CH~OH
~ N - CO - OC H ~ N - CH3 HO ~ LiAlH4 HO ~
OH OH OH OH ~ ~`
For the reaction of l-desoxynorjirimycin with an aIkylating agent, the reaction with allyl bromide can be indicated by way of example as follows:
,' 3~L37 HO ~ + Br - CH2 - CH = CH2 H-B---{>
OH OH
CH20H -.
~ N - CH - CH = CH
HO~
OH OH
Same of the compounds of the formula II used as starting materials are known. This is the case where R3 ~s H, -CH20H or -CH2NH2 and RL is H-Other compounds of the formula II or IIa are new; however, they can be pre-pared from compounds which are known from the literature by processes which are in themselves known.
m uS, for example, it is possible to use the compound of the forn~iLa X, which is known fram the literature, ~/ ~ O X
as a starting materia:L and to react this with a carbonyl cc~pcund of the fornLiLa Vl in the presence of a hydrogen donor reducing agent so as to pro-duce a compound of the formula II.
Furthermorer it is possible to react the ccmpcund X with reactive acid derivative so as to produce an acid amide or urethane and to reduce this to an amine with an amide-reducing agent.
~ - 17 -.. :. .~ . : :
~Z3~3~
This can ~e illustrated by the follcwing example:
HO ~ HOCH2 H N - CH Cl-C-C2H5 H5C2 1I N ~ o C~33 H 1 2 C13 LiAlH4 ~ o ~ H3 m e compound of the formula X can also be reacted with reactive alkylating agents of the following general formula IX as defined hereil~before Z ~
so as to produce a compound of formula II.
Et:tlYYcm~re, in the above mentioned reactions, instead of the com~
pound X it is also possible to employ kncwn partially protected derivatives of the formula XI ~
' 2 `
H2N - C ~ CH2 ~ XI
3 ;:
and then to remove the trityl and benzyl protective groups in a known manner, for example with sodium in liquid ammonia. To prepare compounds of the formLla II, it is also possible to react the compound of fonmula XII, which is likewise kncwn frcm the literature, . . ' . . , , : ~, . ~, , . , ~ , ~1~343~
Tr ~ -C~
with an amine of the general formula XIII
~ - NH2 XIII
wherein ~ has the same meaning as defined hereinbefore in formula II, in the presen oe of a hydrogen donor reducing agent, for example in the presence of NaBH3CN. As a rule, a diastereomer mixture is formed in this reaction. m e diastereomer which is not desired may be appropriately separated off at this stage or at a later stage by the custcmary chrcmatographic methods or by fractional crystalliza-tion. Finally, the trityl and benzyl protective groups can be split off in a known way, for example with sodium in liquid ammonia. -~
Moreover, new compounds of the formula II or IIa can also be obtained by reaction of one or more of the degradation products of D-glucose, which are kncwn from the literature, of the formulae XIV to XVI
... . . ~ .. : . ~ .
.. ~ . ... .
~2343~
O = C~ ~ O - CH ~ = C~ ~ C~2 ~
~ CH3 ~ ~ ~ CH3 ~ n:v xV XVI
with an appropriate reagent having a carbanion character, such as, for exa~,ple, aIkyl-Li or Grignard compounds or the Li salt of 1,3-dithiane, so as to introduce a group R3 as defined hereinkefore in formula I, and converting the resulting comFound(s) of formula XVII
XVII
~ CH3 3 -.
in which R3 has the same meaning as defined hereinkefore in formula I, into the corresponding amine(s~ in a m~nner which is in itself kncwn [S. INOUYE et al., Tetra~edron 23, 2125-2144] via the ketone and the oxime, whereupon, as a rule, a mixture of the gluco com, pound and ido compound forms, fr~m which the desired gluco compound of formula x~III
:
~Z343~
H N - CH 2 ~
XVIII
~ CH3 in which R3 has the same meaning as defined immediately hereinbefore, can be isolated by customary chromatographic methods.
R~moval of the benzyl protective group conveniently by catalytic hydrcgenation or with Na in liquid NH3, then gives the corresponding comr pound(s) of the formula II.
Ccmpounds of the fonmula XIX (belcw) can be obtained when an apprD-priate aldehyde of any of the formulae XIV to XVI is reacted with an appropri-ate amine and hydrocyanic acid in a n~nner which is in itself kncwn so as to produoe an aminonitrile thereby introducing a group Rl as defined herein-before in formula I. mus for example a compound of formula XVI is reacted to produce a oompound of formula XIX
CN
Rl - N,HC 2 ~
XIX
~ .
Z3~37 wherein ~ has the same meaning as defined hereinbefore in formula I, and in this case also, as a rule, the desired gluco compound must be separated off from the ido compound by customary chromato-graphic methods. Further conversion of the nitrile group by hydro-genation or hydrolysis before or after the removal of the benzyl protective group leads to further compounds of the formula II.
The reaction of a co~,pound of forn~la XIV, XV or XVI with a CH-acid comçound, such as, for example, a nitroalkane, aIkyl-nitrile, CH-acid ester or ketone can also lead to compounds of the formula II. In this case, unsaturated compounds, for example com-pounds of the formula XX, can be obtained:
X,Y
C ~'' CH
XX
0~ ~
wherein X is -N02, -CN or -CCOaIkyl, and Y is H, alkyl or aryl, either directly or by dehydration of the aldol addition product, and these compol~nds yield compounds of the formula IIa by a Michael addition reaction with an amine, after chromatographic separation of gluco and ido isomers.
The isopropylidene protective group can be split off from a compound of the formula II in a moderately strongly acid to : .
.
. .
~IZ3~37 weakly acid solution, preferably at a pH in the range from 1 to 4, in aqueous solution or in a water-miscible, water-containing organic solvent. Acids which can be used are dilute mineral acids, such as, for example, sulphuric acid, or also organic acids, such as a oe tic acid. The reaction is preferably carried out under atmos-pheric pressure and at a temperature from room temperature to the boiling point of the solvent.
In order to work up the reaction mixture, the acid is desirably neutralized and separated off as a salt or with the aid of a basic ion exchanger. The isolation of the compounds of formula I in which R2 is OH may then appropriately be effected by careful removal of the solvent, for example by lyophilisation.
A preferred embodiment of the pro oe ss of splitting off of the isopropylidene protective group from a conpound of the formula II comprises saturation of the aqueous or water-containing alcoholic solution of the compound of the formula II with SO2 and storing the saturated solution at a temperature of from 20 to 50C
for several days. The ccmpounds of the formula I can then be ob, tained as bisulphite adducts (R2 = -SO3H), which in most cases readily crystallize, from which the comFounds of the formula I can be liberated with the aid of, for example, aqueous Ba(OH)2.
A compound of the formula I in which R2 is OH can be re-duced to a ccmpound of the formula I in which R2 is H by using an aIkali metal borohydride, alkali metal cyanoborohydride or dialkyl-aminoborane. It is preferable to use sodium borohydride in aqueous ~;, solution or in a water-miscible water-containing organic solvent, - . . . - . ~ . , ~. . .i .
,. . . , ~
~3~37 such as, for example, dioxane, at room temperature or optionally elevated temperature. However, the reduction is very particularly preferably carried out catalytically with Pt or Pd as the catalyst or in the presence of Raney Ni. In this pro oe dure, it is preferably carried out in an aqueous solution at room temperature.
Compounds of the formula I are further obtained from oompounds of the formula CHyl CE3 R ~ - N - CH~ (XX:[ ) OH
by hydrolysis with strong mineral acid of pH <1 at -20 to +20& and sub-sequent hydrogenation at pH 4 to 6 with for instance H2/Raney-Nickel, H2~P+O2 or sodium borohydride.
The oompound of the formNla XXI can be prepared from compounds of the formLla yO
1~ o ~ : :, R O - CH ~
wherein ~ is hydrogen or acetyl and ~ 0 is mesyl or tesyl, by reaction with amines of the formula Rl - NH2 at 20 to 150C in a polar solvent, e.g. an alcohol, dimethylsulfoxide or in an excess of the amune.
.. ~ . .
~Z3~3~
The starting material of the general formula V, in which R3 is -CH2CH, is known and can be obtained either by eatalytie hydrogenation of nojirimyein, which is obtainable by fermentation ~S. INOU~ et al., Tetrahedron 23, 2125-2144 (1968)], or by extrac-tion from mulberry tree bark (see ~T-OS (German Published Specifica-tion) 2,656,602), or entirely synthetically. l-Desoxynojirimyein can also be conveniently prepared by a new advantageous process com-prising cultiva~ing an organism of the Bacillaeeae family in a custcmary fer~entation vessel in a customary nutrient medium at a temperature of fr~m about 15 to about 80& for from about 1 to about 8 days, with aeration, oentrifuging off the cells and isolat-ing the desoxy cGmpcund from the culture broth or the cell extracts by a customary purifieation process (see Germ~n Patent Applieation P 26 58 563.7).
m e carbonyl compounds of the formula VI are either known or can be prepared by standard processes. Typical examples which may be mentioned and preferably contain up to 8 earbon atoms, are:
straight-chain or branehed alkylaldehydes, such as formaldehyde, aoetaldehyde, n-propanal, n-butanal, 2-methylpropanal, n-pentanal, 2-methylbutanal, 3-methylbutanal, 2,2-dimethyl-propanal, n-hexanal, 2-ethylbutanal, n-heptanal and n-octanal; alkenylaldehydes, such as ~.
prcpenal, 2-methylpropenal, 2-butenal, 2-methyl-2-butenal and ... . . .... . ... .. .
~23~37 2-ethyl-2-hexenal; cyclie (particularly cyeloaIkyl aldehydes) aldehydes, such as eyclopropanecarbaldehyde, cyclopentanecarbal-dehyde, eyclopentaneacetaldehyde and cyclohexanecarbaldehyde;
benzaldehyde, o-, ~r and p-toluenecarbaldehyde and phenylacetal-dehyde; straight-ehain and branehed alkylaldehydes whieh are sub-stituted by hydroxyl, such as 5-hydroxypentanal, 2-hydro~y-3-methyl-butanal, 2-hydroxy-2-methylpropanal, 4-hydroxybutanal, 2-hydroxy-propanal and 8-hydroxyoctanal; straight-chain and branched alkyl- ~; ;
aldehydes which are substituted by amino, such as 5-aminopentanal, 2-aminopropanal, 3-aminopropanal, 4-aminobutanal, 2-amino-3-methyl-butanal, 8-amino-octanal and mono-N-alkyl derivatives thereof; and straight-chain and branched alkylaldehydes whieh are disubstituted by amino and hydroxyl, such as 2-hydroxy-5-aminopentanal, 3-hydroxy-3-methyl-4-aminobutanal, 2-hydroxy-4-aminobutanal, 2-hydroxy-3-aminopropanal, 2-hydroxy-2-methyl-3-aminopropanal, 2-amino-3-hydroxyoctanal and mono-N-alkyl derivatives, particularly Cl-C8-N-aIkyl, thereof.
F`urthermore: methoxy-a oe taldehyde, ethoxy-acetaldehyde, n-propoxy-acetaldehyde, i-propoxy-a oe taldehyde, n-butoxy-a oe tal- ~ -dehyde, i-butoxy-a oe taldehyde, tert.-butoxy-acetaldehyde, cyelo-prcpylmethoxy-aoe taldehyde, cyclopropoxy-acetaldehyde, 2-methoxy- ~ ;
ethoxy-acetaldehyde, 2-ethoxy-ethoxy-a oe taldehyde, 2-methoxy (l-methyl-ethoxy)-a oe taldehyde, 2-ethoxy(l-methyl-ethoxy)-aoe tal-dehyde, phenoxy-a oe taldehyde, 2-methoxy-2-methyl-a oe taldehyde, 2-ethoxy-2-methyl-a oe taldehyde, 2-n-propoxy-2-methyl-a oe taldehyde, 2-(i-propoxy)-2-methyl-a oe taldehyde, 2-(n-butoxy)-2-methyl-aoe tal-dehyde, 2-(i-butoxy)-2-methyl-acetaldehyde, 2-(tert.-butoxy)-2-methyl-a oe taldehyde, 2-cyclopropylmethoxy-2-methyl-acetaldehyde, :' .
1~23~37 2-cyclopropoxy-2-methyl-acetaldehyde, 2-methoxy-ethoxy-a-methyl-acetaldehyde, 2-ethoxy-ethoxy-a-methyl-acetaldehyde, 2-methoxy-(l-methyl-ethoxy)-a-methyl-acetaldehyde, 2-methoxy-2,2-dimethyl-a oe taldehyde, 2-ethoxy-2,2-dimethyl-a oetaldehyde, 2-cyclopropyl-methoxy-a oe taldehyde, 2-~-butoxy-2,2-dimethyl-acetaldehyde, methyl-thio-acetaldehyde, ethylthio-acetaldehyde, n-propylthio-acetal-dehyde, i-propylthio-acetaldehyde, cyclopropyl-methylthio-aoe tal-dehyde, 3-methoxy-propanal, 3-ethoxy-propanal, 3-n- and 3-i-propoxy-propanal, 3-n-, 3-i- and 3-tert.-butoxy-propanal, 3-cyclopropoxy-propanal, 3-cyclopropylmethoxy-propanal, 3-methoxy-3-methyl-pro-panal, 3-ethoxy-3-methyl-propanal, 3-n- and 3-i-propoxy-3-methyl-propanal, 3-n-, 3-i- and 3-tert.-butoxy-3-methyl-propanal, 2,3- and 4-methoxy-butanal, 2-,3- and 4-ethoxy-butanal, 2-methylthio-pro-panal, 2-ethylthio-propanal, 3-methylthio-propanal, 3-ethylthio-propanal, 2-methylthio-butanal, 3-methylthio-butanal, 4-methylthio-butanal, furfurol, tetrahydrofurfurol, thiophene, 5-bromo-thiophene,
5-methylfurfurol and pyrane-carbaldehyde.
In addition, examples of ketones which may be mentioned æ e particul æ ly those which æe hydrocarbon ex oe pt for the oxo groups but also those containing additional substituents, such as Cl-C4-alkoxy and nitro: a oe tone, methyl ethyl ketone, methyl n-propyl ketone, diethyl ketone, methyl butyl ketone, cyclopentanone, di-n-propyl ketone, cyclohexano.ne, 3-methylcyclohexanone, 4-methyl-cyclohexanone, a oe tophenone, propiophenone, butyrophenone, phenyl-a oe tone, p-meth~yacetophenone and m-nitroacetophenone.
' ~ ' ~23~37 Formic acid, for example, can be usecl as the hydrogen donor reducing agent (Leuckart-Wallach reaction). The for~ic acid is generally used in a large excess. If formaldehyde is used as the carbanyl reaction component, the reaction can be carried out in aqueous solution, and if ketones and less reactive aldehydes are used, it can be carried out in anhydrous formic acid. m e reaction temperature is generally from 100 to 200 &, and if appropriate the reaction should be carried out in an autoclave.
Catalytically activated hydrogen can also be used as the hydrogen donor reducing agent. A possible catalyst is most prefer-ably, Raney nickel, but noble metal catalysts, particularly those of Group VIII of the Periodic System, can also be used. In general, the reaction is carried out under a pressure of from 80 to 150 atmospheres of H2 pressure and at a te~perature of from 70 to 150 &.
Preferred solvents are protic, polar solvents, especially alcohols, `;
more particularly alkanols, such as methanol, ethanol, propanol and isopropanol.
Alkali metal cyanoborohydrides, dialkylaminoboranes and alkali metal borohyclrides can also be used as hydrogen donor reduc-ing agents. In this process variant, the use of sodium cyanoboro-hydride is parcicularly preferred.
In general, the reaction is carried out at room tempera-ture. However, it can also ke advantageous to heat the mixture to the reflux temperature of the reaction medium.
m e process is usually carried out in an inert sol~ent.
Although anhydrous aprotic solvents can be employed (for example tetrahydrofurane, when the reducing agent is rpholinokorane), a .- . - , .' - . :' 3~37 protic solvent is usually used. A suitable protic solvent is, in partieular, a lcwer aIkanol. However, water or an aqueous lower aIkanol (for example aqueous me~hanol or ethanol) or other aqueous solvent system, such as, for example, aqueous dimethylformamide, aqueous hexa~ethylphosphoric acid triamide, aqueous tetrahydro-furane or aqueous ethylene glycol dimethyl ether, may also be used.
The pro oess is usually carried out in a pH range of from 1 to 11, though a pH range of from 4 ~o 7 is preferred.
The aeid amides of the general formLla VII and urethanes of the general formLla VIII are kncwn in some eases, or they ean be obtained by known proeesses from a compound of formula V and a reac-tive acid derivative, whieh ean also be formed in situ from the correspcnding free aeid.
In this proeedure, the reaetion ean be earried out in a manner sueh that only the amino group of the compound of formula V
reaets with the acid derivative, for exa~ple by using exeess aeid anhydride in an aqueous or aleoholic (e.g. Cl-C3~alkanolic) solu-tion, or sueh that the peraeylated eompounds first form and are then converted into the N-acylated ecmpounds by reaetion with aleoholic ammonia or by trans-esterifieation catalyzed by aIkali metal alcoholate. The latter proeess ean be illustrated by way of example by the following reaetion seheme:
~' .
1~3~3~
CH2H CH20Ac Ac CH2H
~ N~H Ac2 >-- N~NaOC~I ~N~
HO ~ ~ D AcO ~ ) 3 D HO-~
~ Pyridine ~ MeOH ~
HO OH OAc OAc-4CH3CCCCH3 OEl OH
Ac = - C - CH
o An acid amide of the general formula II can be reduced to the corresponding am~ne of the formula I (R = H) with a complex metal hydride or with a horon hydride compound. It is preferable to use NaBH4 in pyridine or a sodium acyloxyborohydride, particul-arly sodium trifluoroacetoxyborohydride. In general, the reducing agent is employed in excess. Sodium trifluoroacetoxyborohydride can be produced in situ from sodium borohydride and trifluoroaoetic acid. Possible solvents are, in addition to pyridine, polar aprotic solvents, such as dioxane, tetrahydrofurane or diglyme.
The reaction is preferably carried out at the boiling point of the ;
solvent used. LiAlH4 can also optionally be used for the reduction, preferably when the hydroxyl groups are first protected in the customary way.
., -. . .
llZ343~
The reactive alkylating agents of the general formula IX
are kncwn or can be prepared by customary processes. The reaction with a oompound of formula V can be carried out in an inert organic solvent, generally at from room temFerature up to the boiling point of the reaction medium, with or without the addition of an acid-binding agent.
Specific new active compounds according to the invention which may be mentioned are:
compounds of the formula: HO ~ N
HO ~ I
,,,_ Rl ,, CH3CHCH3 :
CH3 I CH2-CH3 :
,. , . , .. , ,.. : . ,, - ...
. ~z3~37 R
H3 C`CH-CH2 -H~ C
H3 C ~
H3C~- .
CH3 (cH2 )3-CH2- , 5 H3C~CH C 2 2 .
CH3~:HCH2 CH2 CH3 CY,3 CP:2-C, -C~2 CrI3 CH3 CHC~2 CH2--C~3 CH3 (cH2 )~-CH2- -C1~3 (CH2 )5-CH2- .
CH3 ~CHCH2 CH2 CH2 -CH3 .
CH3 CH- ( CH2 ) 3 -CH2 -CH3 (C~i2 )6-CH2-CH3 CH- ( CH2 j 4 -CH2 ~ ;~
. CH3 - (-CHz ) B -CHz--CH3-(cHz ?lo~CH2~ . ~
Ci~3--(cH2 )l 2--CH2~ ~; r.
CH3 - ~ CH2 ) 1 4 -C~2 ~ ~' CH3 - ( CH2 ) 1 6 -C~2 ~
O-CH2-- , ~CH
O-~H2 -CY2 -HO-C.H2 -C.i2 -H3 C-CH-CH2 ~
OH
Le A 18 389 - 32 ~ , ~Z34~7 1~
HOH2 C-CH2 -CH2 - , - HOH2 C-CH.z -cH2 -CH2 -HOH2C-(CH2 )~-C~2- ' CH3 -CH- ICH-CH2 ~ : :
CY~ OH
HO-CH2 - ,CH-CY'2 - .
OH
- C3 }I, OCH2 -CH2 -c~ScooC~72-CE~-2- , ~C-OCH2 CH2 CH2 CH2 - ,~
H2 N-cH2 -CH2 - i H3 C ~ -,N-CH2-CH2-CH3 CONH-CH2 -CH2 ~
~-~ -NH-C H2 -C-~2 - ~, C2 H5 0 IC~ r~-CH2 -C.~z -ICH3 . ~ .-CH3 CO-N-C~2 -CH2 ~ P
C~3 NH-co-NH-cH2 CH2 - ~ ' H-50-NH-CH2 CH2 - }
C~3 ~I~H-cs-NH-cH2 C~2 - ~:
. ~NH-CS-NH-CH2-5H2- .
CH3 CO~HCH2 CH2 CH2 -~j-CONHCH2 CH2 CH2 - .
CH3 ~ ICONHCH2 CH2 CH2 -', " ' ' Le A lQ -,8~ _ 33 _ -- ~
., ' ' ~
l~Z3437 ~:
R
H2 N-CHz CHz CH2 CH2 - -H2 C=CH-CH2 -~ c Hc=cH cH2-- e H2 C=CH-CH2 -CH2 - ~?
H2 C=CH-CH2 -CH2 -CH2 -CH2 - . ~.
- H2 C=CH- ( CH2 ) 7 -CH2 - .
HOOC-CH2 ~
HOOC -CH2 -5 H2 ~ .
~ ~ Hs C2 OOC-CH2 -CH2 - .
~2 N-C-CH2 - . b O ~ r C2 ~5 ~--5-5H2 C~, Hg -HN-C-CH2 O
HO3 S-CH2 CHz CH2-- , H2 ~02 S-CH2 CH2 CH2 - , C~2-~C COH
.. NO2 ~
~C~2- ' ~;
B~ ~ .
-CH2-- , ,.
~3CO ~;
ZO HO~CH2-- 1 H-C~C-CH2- ~ t HO~CH2- ~, H3CO .
HO-~CH2 - .
Le A ~ 8 ~39 - _ 34 llZ343'7 ~:
R
HO3 S~CHz -N2 ` ' . .
,~H ~:
H3 CO~OCH~ ~ 12 ~" L
C H ' Na 03 S~CH2 _ $~
S03 Na .
$~-CH2--. - ~ t ~C H2 ~ ' Cl~CH2_ , X
~CH2:
Cl ~gj-cH
Br ~CH
~, Le A 18389 _ 35 _ ~
,.
39~37 , '' .
Br~CH2- . ,i ~CHz-~CHz- ~
~ Cl~CH2- ~, k _ ~CH2- ~.
F~CH2-2 N~-C~2 ~
HO~CH2_ ~ ,.
~NO2 HO i.
.' ' . ~:
~CH2 HO~CH2- ~, OH
Le A 18 38, -36 ~ -, !
~ 3~37 .
R
OH
~ 2 . .
OH . '. ~
HO ;, Ho~5H2- .
HOOC~_CH
< o ' HO~CH
COOH
~CH2-H3 C~CH2 - .
~CH~ ~, CH2 - ' . .~
OC~13 ~ .
rHO~CH2 - . h _~_ ' H3 . .
OH
H3 CO~CH2 -CH3 CO~rrl~CH2 -Le A 18 ~89 37 . . .
1~23437 . ~! ~
:~ ~CH2- ~
CH3 ~ .
~jC2H5 H3 CO~cH2_ OCH3 ~
. ~C~2- _ OC~3 0~
OC~H ) 1l i .. OC~3 , ~
H3 CO~C~-2 - ~.s o~ , ~ . f CHe-~Hz-C~Az-~ (~ N-CH2 -CHz -CH
~ CH2_ 1 _ Le A 13 ,39 - 38-.
- . . .
; - - ~ ,, ... .
3~37 `~ 1 HO~OH
HO~
O-C.Y2 -C H2 -~CH
,_ ~3--CH2 _ ' ~CH2- 1' .
Br~ CH2 - ¦
~RCH2-CH2 - ' ~
CH2-- - .~ ,, ~CH2 - ' .
.' ' ' . . .
-' Le A 1~ 389 _ 3 9 _ - ~
" , , , ~.
$
llZ3~.37 C~=pounds of the formula HO~
Rl` R3 ~~ CH C~2-CH3 CH2 CH2 - i H- CH ( CH2 ) 6 -CH2 -H- ~ ~ . H3 C-O-CH2 ~
H- . H5 C2 -O-CH2 - -lQ . . H-- ~-COO-CH~- ¦
H-- CH3 CO-NH-CH2 ~
H- ~CO-~H-CH2- .
~ H- . ~CO-N-CH2-H- CH3 ~HCONH-CH2 ~
~, H- ~NHCONH-CH2-H-- CH3-CH2-N-IC~CH2~
H-- . . C2T~5 OCONH-CH2 ~
HO-CH2 -CH2 - i ., ~: ' H- ~ . _ H- -COOH
H- ~3 C-S2 ~ -CH2 -H- H3 C-H2 C-SO2 -r~-CH2 -~.
H ~ SO2-N-CH2-Le A 18 ~39 .. . ~ ~ ~ ~' ' ~' .
..
~lZ343'7 Rl ~3 ~`
{~H3 - C}~3 - ' ~, CH3--, . CH3 CH2 - .
~CH3 ~ CH3 CH2 ~H2 . ~
C-~3 - ~ C1~3 ( C~-2 ) 6 -CH2 -CH3 - H3 C-O-C~2 - ~ 6 ~` - CH3 - . H5 C2 -O--CH2-- ' C.t}3 - H3 c-COO-CH2 - ~ . _ CH3-- ~COO-CH2-lO ~ CY.3 - H2 N-CH2 ~
CH3 - C~3 CO-l`rH-CH2 -CH3-- ~CO-NH-CH2-. ~ CH3 CH3- ~CO-~I-CH2- ~
CH3 - CH3 N~CO~H-CH2 - ~ E
: 15 C~3- ~NHCONH,-CH2-CH3 - CH3 -CH2 -~- ,C,-NH-CH2 ~ ~ ~, C~3 - C2 Hs OCONH-CH2 -C-~.3-C.~3- -COOH
c~3-- --COt`JH2 ;
-CH3 - H3 C-SO2 -N-CHz ~
CH3-- H3 C-H2 C-H2 C-SO2 -~-CH2 -H
CH~ H. .
_ Le A 18 ~8~ ~ 41 - ~
~Z3~37 ~ ~
Co~pounds of the formula H~
~ With respect to the configuration at,the C-1 atom, the examples listed below include both the -form and the ~-form . . ~ .
R2 , _ . . . . .
H- . H2N-CH2--~ CH3CO-NH-CH2-H- ~)-CO~ CH2-CH3 ~ ~
- H- ~ C0-N-CH2- j H- CH3~HCONH-CH2-H~ HCO~H-CH2- !i, H- CH3 -CH2-N-Icl-NH-cH2- ~ "
H- C2H50cONH-cH2- , H- -COOH .
H- -COOc2Hs- -~
~ -CONH2 H- ~ H3C-S02-N-CH2 .
H ~3 C-H2 C-~-2 C-S02 -~ -CH2 - ~ ;
X-- ~-SOz~N~CH2 ~ ~
H- H0-CH2- _ -20 . H- H5C2-C00-C~2-C~.3 - ` CH3Co-NHCH2~
CH3- , ~ -C0-NH-CH2-CH3- ~CO-i~-C~2-2~ CH3- CH3NHCONH-CH2-Le A 18 ~89 _ 42_ llZ3437 Rl R2 ~, ~
~ L
- ~CH~- ~ NTHCONH~-CH2-~CH3-- . CH3-CH2-H-C-NH-~
CH3- ~2~soco~rH-cH
: 5 CH3- -COOH
CH~- -CONH2 .
H3C-H~C-HzC~s02-H-cH
CH3- ~ SO2-N-CH2-CH3- HO-CH2_ CH3- HsC2-COO-c~2-C~3- -SO3H ~ ' .
CH3- -O-CH,-CH2-CH2-CH3 C~3- -S-CH2-CH3 t,l ,~
CH3 - - ~TH2 ~ r c~3- -NH-CH3 .
, - , - ~; .
Compounds o~ the ~ormula H ~HO H,R~ ~ _ ~ith respect to the configuration at the C-2 atom, the examples listed below include both the a-form and the ~-Lor~ .
_ Le ~ 18 389 - - -~
-t, . R2 ., _ . .
H2 I~-CH2 -~CO-~I-c~2 -CH
~CO-~-C~2 -CH3 N}HCONH-CH2 ~
~\~NHC ONH-CH2 ~
CH3 -CH2 - - ,C-hH-CH2 ~ .
C2 Hs OCONH-CH2 --COO~I - , , --CONH2 ~ ~A
H3 C-SO2 -N-CH2 - ~ --~3 C-H2 C Hz C-SO2 -N-CH2 - r - ~SO2-N-CH2-~O-C~12 - . . ~:
Hs C2 -- ~C, -O-CH2 -' O . . ~.
r 1~ R2 R2 ~ g ~ ~
-OH -O-CH2-CH2-CH2-CH~
-C~ -SH
, . ' ' . _ Le A ~ ~89 _ 44- -- I
`
.~ .
343~ ~
' HO CH2 0~ ~ ~f Compounds of the formula ~N-R1 r HO ~H,OH
OH
Rl ' ,' -CH2-CH3 . ,; ~, -CH2 -CH2 -C~ -C ~3 - .
-CH2-(CH2 )16 )-CH3- ';
~CH3 CH3 . ~ .
-C~2~ ~' ~
-CH2-CH=CH2-- -CH2-CH2-()C~3--CH2 -CH2 -N~ CCH~3 i r~
-CH2 ~
Com~ounds of the formula HO CH2 OH ~ ,.
HO~ \H ~0 S r' R~
~ .
-CH2 -C ~3 - CH2 -CH2 -CH2 -c~-3 -CH2 - ( CHz ) 1 6 -CH3 - ~ CH3 CH "
_C~,2~
-CH2 -CH=CH2 . -C.Y2-CH2-OCH3 !.e A 18 ,89 _ 4S_ .
! .
:- ' ' ' '. . .. ~ , , ', :
l~Z3~37 .
-CH2-CH2-N ~ 3 HO
-CH2~
CH OH
Ccmpounds of the formLla HO ~ M
HO ~ -- R~
OH H, CN
Rl :- 2 2 2 3 -CH2- (CH2) 16-CH
CH3 ~:
-CH
`;
C 2 ~
-CH2-CH=CH2 ~ CH
-CH2-CH2-N~C 3 HO : :~
2 ~
The inhibitors according to the invention are suitable for use as therapeutic agents for the following indications: prediabetes, gastritis, constipation, infactions of the gastro intestinal tract, meteorismus, flatulence, caries, atherosclerosis, hypertension and in particular obesity, .~ :
1~341~37 diabetes and hyperlipoproteinaemia. To broaden the activity spec-trum, it is possible to ccmbine inhibitors for glycoside-hydrolases w~ich cc~plement one another in their action, the combinations be-ing either combinations of two or more compounds according to the invention with one another or cQmbinations of the compounds accord-ing to the invention with inhibitors ~hich are already known. m us, for example, it can be appropria~e to combine saccharase inhibitor compounds according to the invention ~ith amylase inhibitors which are already known.
In some cases, combinations of the compounds according to the invention with kncwn oral antidiabetic agents (~i-cytotropic sul-phonylurea derivatives and/or biguanides having an action on the blood sugar) and with blood lipid-lowering active co~lpounds, such as, for example, clofibrate, nicotinic acid, cholestyramine and others, are advantageous.
m e ccmpounds can be administered without dilution, for example as a powder or in a gelatine casing, or in ccmbination with an excipient in a pharma oe utical composition.
The present invention provides a pharmaceutical composi-tion containing as active ingredient a co~pound of the invention in admixture with a solid or liquefied gaseous diluent, or in admix-ture with a liquid diluent other than a solvent of a molecul æ ~ ~
weight less than 200 (preferably less than 350) ex oe pt in the pre- -sen oe of a surfa oe active agent.
m e invention further provides a pharmaceutical c~mposi-tion CQntaining as active ingredient a ccmpound of the invention in the form of a sterile and/or physiologically isotonic aqueous solu-tion.
m e invention also provides a medicament in dosage unit form comprising a compound of the invention.
, - 47 - ;~
.. , .. .. , , ~ ~
~23~37 The invention also provides a medicament in the form of tablets (including lozenges and granules), dragees, capsules, pills, ampoules or suppositories comprising a compound of the invention.
"Medicament" as used in this specification means physic-ally discrete coherent portions suitable for medical administration.
"Medicament in dosage unit form" as used in this speciflcation means physically discrete coherent units suitable for medical admin-istration each containing a daily dose or a multiple (up to four times) or sub-multiple (down to a fortieth) of a daily dose of the ccmpound of the invention in association with a carrier and/or en-closed within an envelope. Whether the medicament contains a daily dose, or for example, a half, a third, or a quarter of a daily dose will depend on whether the medicament is to be administered on oe or, for example, twice, three times or four times a day respectively.
The pharmaceutical ccmpositions accordLng to the inven-tion may, for example, take the form of suspensions, solutions and emulsions of the active ingredient in aqueous or non-aqueous dilu-ents, syrups, granulates or pcwders.
m e diluents to be used in pharma oe utical compositions ~ ;
(e.g. granulates) adapted to be formed into tablets, dragees, cap-sules and pills include the following: (a) fillers and extenders, e.g. starch, sug æ s, mannitol, and silicic acid; (b) binding agents, e.g. carboxymethyl oe llulose and other oe llulose derivatives, alginates, gelatine and polyvinyl pyrrolidone; (c) moisturizing agents, e.g. gly oe rol; (d) disintegrating agents, e.g. agar-agar, ~: . . :` .
l~Z3D~3~7 calcium carb~late and sodium bicarbonate; (e) agents for retarding dissolution e.g. paraffin; (f) resorption accelerators, e.g.
quaternary a~monium ccmpounds; (g) surfa oe active agents, e.g.
oe tyl alcohol, gly oe rol monostearate; (h) adsorptive carriers, e.g.
kaolin and bentonite; (i) lubricants, e.g. talc, calcium and magnesium stearate and solid polyethylene glycols.
Ihe tablets, dragees, capsules and pills formed from the pharma oe utical compositions of the in~ention can have the customary coatings, envelopes and protective matri oe s, which may contain cpacifiers. m ey can be so constituted that they release the active ingredient only or preferably in a particular part of the intestinal tract, possibly over a period of time. me coatings, envelopes and protective matrices may be made, for example, of polymeric substances or waxes.
m e ingredient can also be made up in microencapsulated form together with one or several of the above mentioned diluents.
m e diluents to be used in pharmaceutical compositions adapted to be formed into suppositories can, for example, be the usual water-soluble or water-insoluble diluents, such as poly-ethylene glycols and fats (e.g. cocoa oil and high esters [e.g.
C14-alcohol with C16-fatty acid]) or mixtures of these diluents.
.
., ~ . :
:llZ34~'7 The pharm~ceutical compositions which are solutions and emulsions can, for example, contain the customary diluents (with, of course, the above mentioned exclusion of solvents having a mole-cular weight belcw 200 except in the presen oe of a surfaoe-active agent), such as solvents, dissolving agents and emulsifiers;
specific examples of such diluents are water, ethyl alcohol, iso-propyl alcohol, ethyl carbonate, ethyl aoetate, benzyl alcohol, benzyl benzoate, propylene glycol, 1,3-butylene glycol, dimethyl-formamide, oils [for example sround nut oil], gly oerol, tetrahydro-furfuryl alcohol, polyethylene glycols and fatty acid esters of sorbitol or mixtures thereof.
For parenteral administration, solutions and emulsions should be sterile, and, if appropriate, blood-isotonic.
The pharmaoeutical compositions which are suspensions can CQntain the usual diluents, such as liquid diluents, e.g. water, ethyl alcohol, propylene glycol, surfaoe-active agents (e.g. ethoxy-lated isostearyl alcohols, polyoxyethylene sorbite and sorbitane esters), microcrystalline cellulose, aluminium metahydroxide, bentonite, agar-agar and tragacanth or mixtures thereof.
All the pharmaoeutical comFositiQns according to the ~Z3437 invention can also contain colouring agents and preservatives as well as perfumes and flavouring additions (e.g. peppermint oil and eucalyptus oil) and sweetening agents (e.g. sacch æ in).
m e pharmaceutical compositions according to the inven-tion generally contain from 0.1 to 99.5, usually from 0.5 to 95~ of the active ingredient by weight of the total composition.
In addition to a compound of the invention, the pharma oe u-tical co~positions and medicaments according to the invention can also contain other ph æ maceutically active compounds. m ey may also contain a plurality of compounds of the invention.
Any diluent in the medicaments of the present invention may be any of those mentioned above in relation to the pharma oe u-tical compositions of the present invention. Such medicaments may include solvents of molecular weight less than 200 as sole diluent.
m e discrete coherent portions constituting the medica-ment according to the invention will generally be adapted, by virtue of their shape or packaging, for medical administration and may be, for example, any of the following: tablets, (including lozenges and granulates), pills, dragees, capsules, suppositories and ampoules. Sc~e of these forms may be made up for delayed re-lease of the active ingredient. Some, such as capsules, include a protective envelope which renders the portions of the medicament physically discrete and coherent.
m e preferred daily dose for adminis-tration of the medica-ments of the invention is from 500 to 5 x 106 SIU (as defined , , ~L~Z3437 hereinbelow) or from 1 to 3500 mg, most preferably from 10 to 500 mg active ingredient.
; The production of the above mentioned pharmaceutical com-positions and medicaments is carried out by any method known in the art, for example, by mixing the active ingredient(s) with the diluent(s) to for,n a pharmaceutical ccmposition ~e.g. a granulate) and then forming the co~position into the ~edicament (e.g. tablets).
This invention further provides a method of combating (including prevention, relief and cure of) the above mentioned diseases in warm-blooded animals, which comprises administering to the anLmals a oompound of the invention alone or in admixture with a diluent or in the form of a medicament according to the invention.
It is envisaged that these active compounds will be administered perorally, parenterally (for example intramuscularly, intraperitoneally, subcutaneously or intravenously), rectally or locally, preferably orally. Preferred pharmaceutical compositions and medicaments are therefore those adapted for oral administration, such as tablets, capsules, powders, dragees, granules, suspensions and solutions. Administration in the method of the invention is pre~erably orally.
In general it has proved advantageous to administer amounts of from 10 to 1 x 104 SIU (as defined hereinbelow) or amounts of from 0.01 mg to 100 mg, preferably from 0,1 to 10 mg, per kg of body weight per day to achieve effective results. Never-theless, it can at times be ne oe ssary to deviate fr~n those dogage rates, and in particular to do so as a function of the nature and body weight of the human or animal subject to be treated, the ;;
~ ,:
1~3437 individual reaction of this subject to the treatment, the type of formulation in which the active ingredient is c~dministered and the mode in which the administraticn is carried out, and the point in the progress of the disease or interval at which it is to be admin-istered. m us it may in some case suffice to use less than the above mentioned mLnimwm dosage rate, whilst other cases the upper l;mit mentioned must be exceeded to achieve the desired ~esults.
Where l æ ger amounts are administered it can be advisable to divide these into several individual administrations over the course of the day.
In addition to the above mentioned pharmaceutical co~posi-tions, foodstuffs containing these active compounds can also be pre-pared; for example sugar, bread potato products, fruit juice, beer, chocolate and other confectionery, and preserves, such as, for example, jam, a therapeutically active amount of at least one of the inhibitors according to the invention having been added to these products.
The food products produ oe d using the active cc~,pounds according to the invention are suitable for use both in the diet of patients suffering from metabolic disorders and for the nutrition of healthy persons in the sense of a method of nutrition for the prophylaxis of metabolic disorders.
Further~ore, the inhibitors according to the invention have the property, in animals, of influencing to a high degree the ratio of the proportion of undesired fat to the proportion of de- ;
sired meat of lcw fat content (lean meat) in favour of the lean meat. This is of particular importance for the rearing and keeping of agricultural stock animals, for example in the fattening of pigs, ~ . .
- , ~3437 but is also of considerable importance for the rearing and keeping of other stock animals and pets. Furthermore, the use of the inhibitors can lead to a considerable rationalisation of the feed-ing of the animals, both in respect of time, quantity and quality.
Since they cause a certain delay in cligestion, the residence time of the nutrients in the digestive tract is extended, whereby ad libitum feeding associated with less expense is made possible.
Furthermore, in many cases there is a considerable saving of valu-able protein feed when the inhibitors according to the invention are used.
m e active c~m~ounds can thus be used in virtually all spheres of ani~al nutrition as agents for reducing the formation of fatty layers and for the conservation of feed protein.
The activity of the active compounds here is essentially independent of the nature and the sex of the animals. The active compounds prove particularly valuable in species of animals which tend generally to deposit relatively large amounts of fat, or tend to do so during certain stages of their life.
The following stock animals and pets may be mentic~ned as examples of animals for which the inhibitors for reducing the forma-tion of fatty layers and/or for conserving feed protein can be employed: warm~blooded animals, such as cattle, pigs, horses, sheep, goats, cats, dogs, rabbits, fur-bearing animals, for example mink and chinchillas, and other pets, for example guineapigs and hamsters, laborator~ animals and zoo animals, for example rats, mi oe , monkeys and the like, poultry, for example broilers, chickens, ~I
. ~
~Z343~
geese, ducks, turkeys and pigeons, parrots and canaries, and cold-blocded animals, such as fish, for example carp, and reptiles, for example snakes.
Because of the advantageous properties of the active com-pounds of the invention, the amount of active compound administered to the animals in order to achieve the desired effect can be varied within broad limits. It is preferably frc~ 0,1 to 1000 mg most pre- ~;
ferably from 1.0 to 100 mg/kg of feed per day. The period over which the active cc~pound is administered can be from a few hours or days io several years. The appropriate amount of active ccmpound and the appropriate period over which it is administered are closely connected with the object of feeding. In particular, they depend on the nature, the age, the sex and the state of health and the method of keeping the animals and can be easily determined by any expert.
m e active compounds according to the invention may be administered to the animal by customary methods. m e nature of the administration route depends, in particular, on the nature, the behaviour and the general condition of the animals. Thus it is possible to carry out the administration orally once or several times ~;ly, at regul æ or irregul æ intervals. In most cases, oral administration, in particular in synchromism with the food and/
of drink intake of the animals, is to be preferred for reasons of expediency.
m e active ccmpounds of the invention may be administered as pure substan oe s or in a formulated form, the expression "formul- ;
ated fokm" incluc~ng both a premix for admixture with the animal .::, .
: - .
~W~3'7 feed or drinking water, that is to say mixed with a non-toxic inert carrier of any desired nat~lre, and also as part of a total ration in the form of a supplementary feed and as a constituent of the mix-ture of a mixed feed by itself. Administration of suitable formula-tions by means of the animal drinking water is also included.
The active co~pounds accordLng to the invention, option-ally in the formulated form, can also be administered, in a suit-able form, together with other nutrients and active compounds, for exa~ple mineral salts, trace elements, vitamins, proteins, energy carriers (for example starch, sugar or fats), dyestuffs and/or flavouring substances or other feedstuff additives, such as, for example, growth promoters. The active compo~nds of the invention can be administered to the animals before, during or after their food intake.
Oral administration together with the feed and/or drink- `
ing water is advisable, the active conpounds being added to the total amount or only to certain parts of the feed and/or drinking water, depending on the requirement.
The active conpounds of the invention can be added to the feed and/or the drinking water according to customary methods by simple admixture of the pure conpound, preferably in a finely divided form, or in a formulated form mixed with edible, non-toxic carriers, and optionally also in the form of a premix or a feed CQn-centrate. --m e feed and/or drinking water can, for example, contain the active compo~mds according to the invention in a concentration of f m m 0.001 to 5.0 % o, most preferably from 0.01 to 2.0/oo (by weight). The optimNm level of the CQncentration of the active com-:
', :. , :: . .
~3437 pound in the feed and/or drinking water depends, in partic~lar, on the size of the feed and/or drinking water intake of the animals and can be easily determined by any person skilled in the art.
~ he nature of the feed itself and its composition does not normally influence the utilisation of the campounds of the invention. m us it is possible to use all the current, co~merci-ally available or special feed compositions, which preferably con-tain the custamary prop~rtions of energy substances and proteins, including vitamins and mineral substan oe s, necessary for balanced nutrition. me feed can be composed, for example, of vegetable sub-stan oe s, for example shredded oil-cake, shredded cereal and cereal by-prcducts, but also of hay, sila~e fodder, beets, and other forage plants, of animal substances, for example meat and fish pro-ducts, bonemeal, fats and vitamins, for example A, D, E, K and B-ccmr plex, as well as special sour oe s of protein, for example yeasts and oertain amino-acids, and mineral substances and trace elements, such as, for example, phosphorus and iron, zinc, manganese, oopper, cobalt, iodine and the like.
Premixes can preferably contain frQm 0.1 to 50%, most pre-ferably fram 0.5 to 5.0% (by weight) of, for example, N-methyl-l-desoxynorjirimycin, in addition to any desired edible carrier and/or mineral salt, for example carb~nated feed lime, and may be prepared by customary mixing metho~s.
Mixed feeds preferably contain from 0.001 to 5.0/oo, in particular from 0.02 to 2.0 % o (by weight), for example, of N-methyl-l-desoxynorjirimycin, in addition to the custamary raw mate-rial camponents of a mixed feed, for example shredded cereal or ' ~
~ ~23~37 oereal by-products, shredded oilcake, animal protein, minerals, trace elements and vitamins. mey can be prepared by customary mixing methods.
me active compounds of the invention when in pr~mixes and mixed feedstuffs can preferably also be appropriately protected from air, light and/or moisture by suitable agents which cover their surface, for example with non-toxic waxes or gelatine.
me following is an example of a co~,position of a finished mixed feed, for poultry, containing an active ccmpound according to the invention: 200 g of wheat, 340 g of maize, 360.3 g of coarse soya bean meal, 60 g of beef tallow, 15 g of dicalcium phosphate, 10 g of calcium carbonate, 4 g of iodinated sodium chloride, 7.5 g of a vitamin/mineral mixture and 3.2 g of an active comFound premix yielding, after careful mixing, 1 kg of feed.
The vitamin/mineral mixture consists of: 6,000 I.U. of vitamin A, 1,000 I.U. of vitamin D3, 10 mg of vitamin E, 1 mg of vitamin K3, 3 mg of riboflavin, 2 mg of pyridoxine, 20 mcg of vitamin B12, 5 mg of calcium pantothenate, 30 mg of nicotinic acid, 200 mg of choline chloride, 200 mg of MnSO4 x H20, 140 mg of ZnSO4 x 7H2O, 100 mg of Fe ~ x 7H20 and 20 mg of CuSO4 x 5H20. The - --active ccmpound premix contains, for example, N-methyl-l-desoxynojirimycin in the desired amount, for example 1,600 mg, and in ~ tion 1 g of DLrmethionine and encugh soya bean flour to form 3.2 g of premix.
m e follcwing is an example of the composition of a mixed feed for pigs, which feed contains an active compound of the formula I: 630 g of shredded oereal feed (cc~posed of 200 g of ., . . :. , .
~23~3~
shredded maize, 150 g of shredded barley, 150 g of shredded oats and 130 g of shredded wheat), 80 g of fish-meal, 60 g of coarse soya bean meal, 58.B g of tapioca flour, 38 g of brewer's yeast, 50 g of a vitamin/mineral mixture for pigs (constitution for example, as in the chicken feed above), 30 g of linseed cake meal, 30 g of maize gluten feed, 10 g of soya bean oil, 10 g of cane sugar molasses and 2 g of active ccmpound premix (constitution for example, as in the chicken feed above~ yield, after careful mixing, 1 kg of feed.
The feed mixtures indicated are intended, preferably, for the rearing and fattenLng of chickens or pigs respectively; however, they can also be used in identical or similar compositions for the rearing and fattenLng of other animals.
The oQmpounds of the invention can be used individually or in any desired mixture with one another.
In vitro saccharase inhibition test The in vitro saccharase inhibition test makes it possible to determine the enzyme-inhibitory activity of a substan oe by com-parison of the activity of the solubilised intestinal disaccharidase ccmplex in the presence and in the absen oe (so-called 100~ value) of the inhibitor (compcund under scrutiny). A virtually gl-ucose-free sucrose (glucose clOO ppm) is used here as the substrate which determines the specificity of the inhibition test; the determina- ;
tion of enzyme activity is based on the spectrophotometric deter-mination of glucose liberated, using glucose dehydrogenase and nicotinamide-adenine dinucleotide as the cofactor.
One saccharase inhibitor unit (SIU) is defined as that - . ~
`~3437 inhibitory activity which, in a defined test batch, reduces a given saccharolytic activity by one unit (saccharase unit - SU); the saccharase unit being defined here as that enzyme activity which splits off one ~mol of sucrose per minute under given conditions and thus leads to the liberation of o~e ~mol each of glucose, which is determined in the test, and fructose, which is not recorded in the test.
The intestinal disaccharidase co~,plex is obtained from swine small intestine mucosa by tryptic digestion, precipitation from 66% strength ethanol at -20 &, taking up of the precipitate in 100 mM phosphate buffer, pH 7.0, and finally dialysis against the same buffer.
100 ~1 of a dilution of the intestinal disaccharidase com~
plex in 0.1 M maleate buffer, pH 6.25, æ e added to 10 ~1 of a sample solution, which is prep æ ed so that the extinction of the test batch is at least 10%, but not re than 25%, below that of the 100% value, and the mixture is pre-incubated at 37C for 10 minutes. The dilution of the disaccharidase complex should norm~lly be adjusted to an activity of 0.1 SU/ml.
The sacch æ olytic reaction is st æted by adding 100 ~1 of a 0.4 M solution of sucrose ("SERU~ 35579") in 0.1 M maleate buffer, pH 6.25, and, after an incubation period of 20 minutes at 37C, is stopped by adding 1 ml of glucose dehydrcgenase reagent (1 small bottle of lyophilised glucose dehydrogenase/mut æ otase mixture ("MERCK 14053") and 331.7 n~ of ~-nicotinamide-adenine dinucleotide (free aeid "BOE~rgnNOE R" degree of purity I) dissolved in 250 ml of 0.5 M tris buffer, pH 7.6). In order to determine the glucose con-.~
- ,, ~ ; ~ : .
~L:Z3~37 centration, the mixture is incubated at 37C for 30 minutes and finally is measured photGmetrically at 340 nm against a reagent blank ~containing enzyme b~t without sucrose).
me calculation of the inhibitory activity of inhibitors is made difficult by the fact that even sli~ht changes in the test system, for example a 100% value which varies slightly from deter-mination to deter~ination, can have a sig~ificant effect on the test result which cannot be ignored. These difficulties may be avoided by running a standarl with every determinationj a saccharase inhibitor of the formula C25H43O18N whi~h has a specific inhibitory activity of 77,700 SIU/g and, when employed in the test in amounts of 10 to 20 ng, leads to an inhibition of the order of size specified above, is conveniently used as the standard. If the differen oe between the extinctions at 340 nm of the 100% value and of the batch inhibited by the standard is knGwn, the specific inhibitory activity of the inhibitor, expressed in saccharase inhibitor units per gram (SIU/g), can be calculated in a knGwn manner from the extinction difference between the 100% value and ` the batch inhibited by the sample solutiGn, taking into considera-tion the amount of inhibitor employed.
` Specific saccharase-inhibitory activity in vitro l-Desoxynojirimycin465,000 SIU/g - N-Methyl-l-desoxynojirimycin2,330,000 SIU/g Preparation Examples -Example 1 N-Methyl-l-deso~ynojirimycin 3~37 OEl OH
; N\- ~H3 HO ~
HO OH
3.2 g of l-desoxynojirimycin and 2 ml of 30~ strength a~ueous formaldehyde are added to 4 ~ of 98~ strength fo~mic acid, whilst cooling with i oe. The mixture is then heated ~mder reflux for 8 hours. After cooling, the reaction mixture is diluted with a oe tone. A resinous precipitate separates out. The acetone solu-tion is decanted off and the resin is rinsed several times with ace-tone. The residue is then dissolved in distilled water and the solution is freed from formic acid by adding a basic ion eYchanger in the OH form (Amberlite JRA 410). m e ion exchanger is filtered off and the aqueous solution is brought to dryness under reduced pressure. 3.0 g of resinous N-methyl-l-desoxynojirimycin remain.
The compound can be further purified by chromatography on oe llulose.
; Water-containing butanol is used as the running agent. m e com- p~und may be cristallized from ethanol. M.P.: 153 &.
~lass spectrum: The most important peak in the upper mass range is at m/e = 146 (M~CH20H)-For further characterisation, the ccmpound is converted into the pera oe tylated compound, N-methyl-2,3,4,6-tetra-O-acetyl-l-desoxynojirimycin, with acetic anhydride/pyridine 1:1 at ro~m temperature. A proton magnetic resonance spectrum of this deriva-tive in CDC13 was reasuIed at 100 M3z: 4 singlets Eor t e total of .
;~ ~
.
~
1~
12 protons, which correspond to the methyl groups of the O-acetyl groups (CH3-O-C-), are found between ~ = 2.0 and 2.1 ppm. The o methyl group bonded to N (CH3-N<) is found as a singlet at ~ = 2.45 ppm. Two protons on a C atom bonded l:o nitrogen (H-C-N<) absorb as poorly resolved multiplets between ~ = 2.1 and 2.5 ppm. A further proton of this type appears as a doublet of a doublet (Jl = 11 HZ;
J2 = 4 HZ) at ~ = 3.18 ppm. A methylene group (-CH2-O-C-C~3) .
absorbs as an AB system at ~ = 4.16 and ~ = 4.22 ppm. The remain-ing three protons (-C-O-C-CH3) are found as a mul-tiplet between ll H O
10 ~ = 4.9 and 5.2 ppm.
Example 2 N-n-Butyl-l-desoxynojirimycin CH20H , ~ N - CH2 - CH2 - CH2 C 3 HO ~
HO OH
12.5 r~ of n-butyraldehyde, 0.01 mols of methanolic HCl and 1.5 g of NaCNBH3 are added sucoessively to 3.2 g of l-desoxyno-jirimycin (0.02 mol) in 40 rnl of absolute methanol, whilst cooling with ice and stirring. The reaction mlxture is stirred at room temperature for 12 hours. It is then concentrated to dryness on a rotary evaporator. The residue is dissolved in 50 ml of water and extracted 3 times with 30 ml of CHC13 each time. me aqueous phase is again brought to dryness, the residue is taken up in 30 ml of . ~ . ~ .
~Z343~7 H2O and the solution is discharged onto a column 50 cm long and 2 cm wide which is filled with a strongly basic ion exchange resin in the OH form (A~berlite IRA 400 or Dowex 1 x 2).
The reaction product is eluted with water and the indivi-dual fractions are investigated by thin layer chromatography.
(Silica gel plates; running agent: ethyl acetate/methanol/water/25%
strength ammcnia 100:60:40:2; spray reagent: KMnO4 solution). The fractions which contain N-n-butyl-l-desoxynojirimycin are collected and the aqueous solution is concentrated on a rotary evaporator.
Acetone is added to the residue, whereupon crystallisation occurs. ~ -The crystals are filtered off, rinsed briefly with ace-tone and dried. 3 g of N-n-butyl-l-descxynojirimycin of melting point 126-127& are obtained.
Mass spectrum: The most im~ortant peaks in the upper mass range are found at m/e = 188 (M~CH20H) and m/e = 176 (M-CH2-CH2-CH3).
In the case of less reactive aldehydes, a molecular sieve 3A was added to the reaction mixture in order to bind the water of reaction.
The following compounds were prepared by methods analogous to those of the above proo_dure:
N-Ethyl-l-desoxynojirimycin CH20H . .
~ \ 2 3 HO ~
HO OH
-3~37 ~ss spectrum: Intense peak at m/e = 160 (M-CH20H).
N-n-Propyl-l-desa~ynojiri~7cin ~ N - CH2 - CH2 - CH3 HO ~
HO OH
Mass spectrum: Intense Feak at m~e = 174 (M-CH20H).
Peaks also at m/e = 206 (M~H) and m/e = 204 (M~H).
N iso-Butyl-l-desoxynojirim~cin ~ N - CH2 - CH 3 HO ~ 3 :
~IO OH
Mass spectrum: The most important peaks in the upper mass range are found at ~ :
m/e = 188 (M~CH2OH), m/e = 176 (mrCH ~ 3), m/e = 220 (M~H) and m/e = 218 CH
(~H). 3 N-n-Heptyl-l-desoxynojirimycin , CH OH :
~N - CH2 - (CH2)5 - CH3 HO~ >
r~ .
HO OH
melting point: 111 - 113& (from aoe ton) Mass spectrum: The ~st important peak in the upper mass range is at m/e =
230 (M~CH20H). Peaks are also found at m/e = 262 (M~H) and 260 (M~H).
. ~
3~37 N-Benzyl-l-desoxynojirimycin CH OH
~-- CH2 ~
HO OH
melting point: 183 - 184 & (from methanol) Mass sprectrun: m e most important peak in the upper rnass range is found at ~/e = 222 (M~CH20H).
N-(2-Pyridyl)-methyl-l-de~oxynojirimycin ~-- CH2 ~
HO OH
melting point: 174 - 175 & (from ethanol) ~ass spectrum: The most important peaks in the upper rnass range are found at r~/e = 255 (M~H), r4~e = 236 (M-H20) and m/e = 223 (M~CH20H).
N-2-Hydroxyethyl-l-desoxynojirimycin ~ 2 2 HO ~
HO OH
melting point: 114 & (from ethanol) Mass spectrum: The most important peak in the upper rnass range is at m/e =
176 (M~CH20H).
N-2,3-DLhydroxy-n-propyl-l-desoxynojirimycin C~12H
HO ~ N ~ CH2 - CH - CH2 - OH ~:
~ OH
HO OH
3~
Mass spectrum: The m~st Lmportant peaks in the upper mass range are at m/e = 206 (M-CH20H) and m/e = 176. me substance is a mix-ture of two diastereomeric compounds.
N-(S-B-~ Glucopyranosyl-2-mercaptoethyl)-1-desoxy.nojirimycin HO CH
CH20H >--~
; \ CH2 - C~12 - S ~ ~ OH
HO ~ ~
HO OH
Mass spectr~m: The mass spectrum of the compound peracetylated in pyridine/acetic anhydride was measured. me most important peaks in the upper mass range are found at m/e = 648 (M~CH20-C-CH3), o m~e = 588 and mJe = 344.
me aldehyde required for the reaction was obtained from O-aoetylated l-thioglucose and chloroaoetaldehyde. me acetyl groups in the end product were split off by transesterification with catalytic amounts of NaOCH3 in MeOH.
N-Oxiranyl-methyl-l-desoxynojirimycin ,, CH OH
_~N ~ CH2CH -~CH2 ~_~ O ~ ~ :
OH OH
Yass spectrum: The most important peaks in the upper mass range are found at m/e = 219 (M), m/e = 202, m/e - 188 (M~CH20H) and m/e = 176 (M-CH - CH2). ;~
O ' '~
,~
:~Z3~3~7 ~ he substance is a mLxture of two diastereomeric com-pounds.
N-(3-N-Phthalimido-n-propyl)-1-desoxynojirimycin HOH~ CH - CH - CH - N~
OH OH
Mass spectrun: m e most important peaks in the upper mass range were ~ound at m/e = 348, m/e = 319 (M-CH20H), ~e = 301, m~e = 200, m/e = 188, m/Q = 174, m/e = 160 and m/e = 147.
In this case, chromatography on a basic ion exchange resin was dispensed with and the compound was purified by boiling up with a oe tone and recrystallisation from ethanol.
Melting point: 208 - 210 C. ~ -~
~-(3-Amino-n-propyl)-l-desoxynojirimycin CH OH
HO ~- CH2 - CH2 - CH2 N 2 HO OH :
Mass spectrum: m e most important peaks in the upper mass range are at m/e = 189 (M-CH20H) and m/e = 146. -m e compound was obtained from the above phthalimido com-pound by hydrazinolysis in methanol.
N-(l-Desoxynojirin~in-yl)-acetic acid ~`
:
^ ~ . - .
- .
3~3~
C~2 ~ N - CH - COCH
HO ~ 2 H~ OH
Mass spectrum: The most important peaks in the upper mass range are found at m/e = 203 tM-H2O), ~/e = 159, m/e = 145 and m/e = 100.
The oo~pound was not purified by chromatography over a basic ion exchange resin but by recrystallisation from methanol/water.
~lelting point: 187 - 188C.
N-o-Nitrobenzyl-l-desoxynojirimycin _~ CH2 ~ ~,, N2 1' HO OH
Rf value: 0.85 (on thin layer chrcmatography ready-to-use silica gel 60 plates from Messrs. Merck; running agent: ethyl acetate/methanol/H20/25~ ,~
strength ammonia 100:60:40:2).
For ocmparison: Rf value of l-desoxynojirimycin: 0.3. `::.
N-o,Car}o=ybenzyl-l-desoxynojirimycin , , - CH
CCOH
HO OH
Rf value: 0.7 ~lates and running agent as indicated for the above ccmpound).
''' ..
~Z~37 For purification, the co~lpound was chromatographed over a basic ion exchange resin as indicated above, but finally was eluted with 1% strength acetic acid.
N-p-Carboxybenzyl-l-desoxynojirimycin _ _ .
HO - CH
~ N - CH2 ~COOH
HO ~
OH OH
m.p.: 280 - 281 C (from H2O/methanol) Rf value: 0.7 (plates and running agent as indicated above).
In this case also, the co~pound was eluted from the basic ion exchange resin with 1% strength a oe tic acid.
N-p-Sulfobenzyl-l-desoxynojirimycin ~ ~ 2 ~SO3H
HO
HO OH .
4.8 g of benzaldehyd-4-sulfonic acid, 1.8 ml of a oe tic acid and 0.8 g of NaCNBH3 are added to 2 g of l-desoxynojirimycin in 40 ml methanol. The mixture was refluxed for 4 hours and stirred for 12 hours at room temperature. The precipitate was filtered off and recrystallized from water. 1.2 g of N-p-sulfobenzyl-l-desoxy-nojirimycin of melting point ~ 320C (dec.) are obtained.
. . : - ..
,~,~37 Example 3 N-~-Phenylethyl-l-desoxynojirimycin ~ H
HO ~
HO OH
3 g of phenylacetaldehyd and 0.8 g of NaCNBH3 are added to 2 g of l-desoxynojirimycin and 1.8 ml acetic acid in 40 ml of methanol.
The mixture is stirred for 12 hours at room temperature and evapor-ated on a rotary evaporator. The residue is dissolved in ethanol/
water (2:1) and discharged onto a column which is filled with a strongly acidic ion exchange resin in the ~- form. me column is washed with 2 1 of ethanol and water (2:1). Then the product is eluted with ethanol/2~ strength aqueous ammonia (2:1). me frac-tions are investigated by thin layer chromatography and those which contain the product are collected and dried. The residue is cry-stallized from 100 ml ethanol. 2.5 g of N-~-phenyl-ethyl-l-desoxy-nojirimycin with a melting point 179 - 181C are obtained.
me follcwnng compounds were prepared analogously: ~-N-n-Pentyl-l-desoxynojirimycin ;~
.~
( 2)4 H3 HO ~ j~
HO OH
m.p. 97C (from acetone) ;:
. . . .
~IZ~gl3'7 N-n-Hexyl-1-desoxynojirimycin ~ ~ ( 2)5 3 HO ~
HO OH
m.p. 112 - 113C (from ethanol/acetone) N-n-Octyl-l~esc~ynojir~lT~cin ~ N\- (CE12)7 - CH3 HO ~ ~`
HO OH :
m.p. 115 - 117& (from eth~ol/aoetone) N-n-Nonyl-l-deso~ynojiri~cin C~H20H
r N - (CH ) - CH
HO ~ ~
HO OH
"
m.p. 105 - 107& (from ethanol/aoetone) : `
, - - . . . ., , , :
,, :",. : . . .,: .
~L12~37 - ~ :
N-n-Decyl-1-~esoxynojirimycin CH20H ~;
~ ~ ~ N-(CH2)9-CH3 '_ ~.0~
HO OH
m.p. 151C (sinters at 91C from ~eOH/acetone) N-n-Undecyl-1 desoxynojirimycin ( CH 7 ) 1 o ~CH 3 E~O ~ ~ , ~, ~0 OH
m.~. 162C (sinters at 91C from ethanol/acetone) ~; :
; N-n-Dodecyl-1-desoxynojirimycin ~-CH20~
~N-(CH2) 1 l--CH3 P
HO~
HO OH ~:
.
m.p. 164C (sinters at 97C from ethanol/acetone) ,3A
, Le A 18 389 - 73-~ 23 4 37 1 !
N-n-T~tradecyl-1-desoxynojlrimycin HO ~ -~CH2)13-CH3 i~
HO OH
-m.p. 105-107C (from methanol) ~-n(5'-Hydroxypentyl)-1 desoxynojirimycin HOC';~
~ W-(CH-) 4-CH.-O'~
XO--~ >
' ..
~o ~o .p. 8~-S7C (from butanol) ~-Cyclohexylmethyl-1-desoxynojirimycin H~CH
,- ~-CH.
HO OH
~';'' m.p. 138-140C (from acetone) Le A 18 389 _ 74- ~
3~
N-(3'-Cyclohexenylmethyl)-1-desoxynojirimycin , ~ -CH2- ~ t HO OH
m.p. 142-i44C (from acetone) ' N-(2'-Norbornen-5'-yl-methyl)-1-desoxynojirimycin HOCH
~ N - CH2 HO ~
- HO OH
,;
m.p. i60-162C (from ethanol) t .
~J-~-C~.lorben~yl-1-d~soxynojirimycin HOCH2 r-~
\- N - CH2 ~ Cl ~0 ~
~ HO OH
m.p. 153-155C (from acetone) Le A 18 389 - 75-.
~-m-Metnylbenzyl-1-desoxynojirimycin - ~-N ~ CHz-~
'rlO--` ~> C~3 HO OH
m.p. 134-136V (from methanol) - N-(p-3iphenylmethyl)-1-desoxynojirimycin ~ - C:~2- ~ `
HO OH
m.p. 240-245C (from water/ethanol) , .
~-(n-3'-phenylpropyl)-1-desoxynojirimycin HOC~ 2 _~ N--CH2--CH2-CH2--<~ ~
HO OH r m.p. 125-127C (from ethanol) Le ~ 18 339 - 76 _ ?
, Ex~mple ~
- . ' N-Allyl-1-desoxynojirimycin CH20H r-C~2-CH=CH~
- HO
EIO. OE~
~.
5 g of 1-desoxynojirimycin, 5 g of Ag20 and 5 g of ~_ allylbromide are stirred in 30 ml of dimethylformamide and 'O ml of water for 3 hours at room temperature~ The silver salts are filtered off and the filtrate is evaporated at the rotary eva~orator. The residue is recrystallized from ethanol.
'.5 g of N-allyl-1-desoxynojirimycin of melting point 131 to 132~C are obtained.
The following products are obtained analogously, tne isolation and purification optionally carried out by chro~to-grap:ny on a s~rongly acidic ion exchange resin (H~-form).
~-Propargyl-1-desoxynojirimycin ~OCH, r ~I-CH2-C-CH
~10--< >
HO OH
m.p. 160C (from acetone) - ' ~ .
Le .~ 1~ 3&9 - 77--.
~12343~
' N-(3',4'-Dichlorbenzyl)-1-desoxynojirimycin ~-CH2 ~Cl HO OEI e~
m.p. 130-132C
N-(p-Nitrobenzyl)-1-desoxynojirimycin r N-C~-2 ~ NO2 E~(! ~
HO OH
..p. 144-146 C
. .
~-~.~-Nitrobenzyl)-l-desoxynojirimycin rOCE~2 ~-CH2 -/~ , ~32 ,.-~iO OP.
m.p. 168-170C
Le .~ l~ 389 _ 78 - _ , ~
.' . j ... .
343~
.
. Exam~le 5 l-Cyano-1-desoxynojirimycin HOCHz S \ NH
HO ~ CN
HO OH
~;~
17.5 g of nojirimycin bisulfite adduct are added to 200 ml of water and 21.2 of Ba(OH)2 8 H20. The mixture is stirred for 1 hour and the solid is filtered off. 12 ml of liquid HCN are added to the filtrate and the mixture is stirred for 30 minutes. The solution is filtered and concen- t trated on the rotary evaporator to 20 ml. 20 ml of methanol are added whereby the crystallization of the product starts.
100 ml of ethanol are added to complete crystallization.
~fter filtration 12.0 g of l-cyano-l-desoxynojirimycin are obtained m.p. 155-156C (from methanol/water).;' ~xa~ple 6 N-h.ethyl-l-cyano-l-desoxynojirimycin I~OCH2 r ~ N-CH3 E~O ~y~crT
HO OH
The compound is obtained from l-cyano-l-descxyno~iri-mycin with 35 ~ strength aqueous formaldehyd solution and ~aC`I~H3 in methanol according to example 3.
Le A 18 389 - 79 -~37 Mass spectrum: The most important peaks in the upper mass `.an~e are at m/e = 17~ (M-CH20H), m/e-157 and m/e = 144.
Example 7 1-Desoxynojirimycin-1-carboxvlic acid \ NH
HO ~ - COOH
~o OH ~k 10 g of 1-cyano-1-desoxynojirimycin are refluxed with ~ g of sodium hydroxide in 100 ml of water for one hour. Hydro-chloric acid is added up to pH 4. The mixture is dried on the rotary evaporator and the residue is extracted with hot methanol, sodiu~ chloride is separated and the methanolic t5 solu_ion is evaporated. The residue is recrystallized from wa~er and water/methanol. 10.5 g of 1-desoxynojiri~ycin-1- r ca-boxy 1 ic acid OI m.p. 268-270C are obtai~ed.
Ex~mpie 8 ,;
1-Desoxynojirimycin-1-carboxylic acid ethyl es.er C ~ 2 t~
~0 ~ ~-COOC2H5 ~:0 OEi 7 ~ of 1-desoxynojirimycin-1- carboxylic ~c~d are re,~l~lYcd with 100 ml of ethanolic hydrochloric acid for 2 hours and evaporated at .he rotary evaporator. The residue is treated Witil ethanol and ethanolic ammonia. The solution was filtered and concentrated. 8 ~ of 1-desoxynojirim~-in-1-ca~oxylic a^id Le A 1~ 389 - 80 -- ~. ;: . - . ~
1~3~37 ethyl ester are obtained. NHR-Spectrum 100 MHz:
triplet at 5 = 1.3 ppm (3H, -COO-CH2-CH3);
multiplet at5 =2.4-2.6 ppm (1 H~ -N-CH CH OH);
multiplet at~ = 3.2-3.5ppm (4 H);
multiplet a_5 =2.6-3.9ppm (2H, ~CH2-OH);
qu~rtet at 6 =4.25 ppm ~2 H, -COO-CH2-CH3).
~xam~le 9 N-~eth~l-1-desoxynojirimycin-1-carboxylic acid eth~lester CH
\ N-CH 3 -.0 ~,~> COOC2 ;~5 ' HO OH
From 1-desoxynojirimycin-1-carboxylic acid ethyl ester according to example 6. r ,~lass spectrum: The most important peaks in the upper mass range are at m/e=218(M-CH20H), m/e= 200, m/e=176, m/e=158 and m/e=126.
Example 10 1-Desoxynojir-mycin-1-carbox~lic acid amide ~OCY.
\r-~'H
HO ~ ~-CO~H
Y~O, OY~
In addition, examples of ketones which may be mentioned æ e particul æ ly those which æe hydrocarbon ex oe pt for the oxo groups but also those containing additional substituents, such as Cl-C4-alkoxy and nitro: a oe tone, methyl ethyl ketone, methyl n-propyl ketone, diethyl ketone, methyl butyl ketone, cyclopentanone, di-n-propyl ketone, cyclohexano.ne, 3-methylcyclohexanone, 4-methyl-cyclohexanone, a oe tophenone, propiophenone, butyrophenone, phenyl-a oe tone, p-meth~yacetophenone and m-nitroacetophenone.
' ~ ' ~23~37 Formic acid, for example, can be usecl as the hydrogen donor reducing agent (Leuckart-Wallach reaction). The for~ic acid is generally used in a large excess. If formaldehyde is used as the carbanyl reaction component, the reaction can be carried out in aqueous solution, and if ketones and less reactive aldehydes are used, it can be carried out in anhydrous formic acid. m e reaction temperature is generally from 100 to 200 &, and if appropriate the reaction should be carried out in an autoclave.
Catalytically activated hydrogen can also be used as the hydrogen donor reducing agent. A possible catalyst is most prefer-ably, Raney nickel, but noble metal catalysts, particularly those of Group VIII of the Periodic System, can also be used. In general, the reaction is carried out under a pressure of from 80 to 150 atmospheres of H2 pressure and at a te~perature of from 70 to 150 &.
Preferred solvents are protic, polar solvents, especially alcohols, `;
more particularly alkanols, such as methanol, ethanol, propanol and isopropanol.
Alkali metal cyanoborohydrides, dialkylaminoboranes and alkali metal borohyclrides can also be used as hydrogen donor reduc-ing agents. In this process variant, the use of sodium cyanoboro-hydride is parcicularly preferred.
In general, the reaction is carried out at room tempera-ture. However, it can also ke advantageous to heat the mixture to the reflux temperature of the reaction medium.
m e process is usually carried out in an inert sol~ent.
Although anhydrous aprotic solvents can be employed (for example tetrahydrofurane, when the reducing agent is rpholinokorane), a .- . - , .' - . :' 3~37 protic solvent is usually used. A suitable protic solvent is, in partieular, a lcwer aIkanol. However, water or an aqueous lower aIkanol (for example aqueous me~hanol or ethanol) or other aqueous solvent system, such as, for example, aqueous dimethylformamide, aqueous hexa~ethylphosphoric acid triamide, aqueous tetrahydro-furane or aqueous ethylene glycol dimethyl ether, may also be used.
The pro oess is usually carried out in a pH range of from 1 to 11, though a pH range of from 4 ~o 7 is preferred.
The aeid amides of the general formLla VII and urethanes of the general formLla VIII are kncwn in some eases, or they ean be obtained by known proeesses from a compound of formula V and a reac-tive acid derivative, whieh ean also be formed in situ from the correspcnding free aeid.
In this proeedure, the reaetion ean be earried out in a manner sueh that only the amino group of the compound of formula V
reaets with the acid derivative, for exa~ple by using exeess aeid anhydride in an aqueous or aleoholic (e.g. Cl-C3~alkanolic) solu-tion, or sueh that the peraeylated eompounds first form and are then converted into the N-acylated ecmpounds by reaetion with aleoholic ammonia or by trans-esterifieation catalyzed by aIkali metal alcoholate. The latter proeess ean be illustrated by way of example by the following reaetion seheme:
~' .
1~3~3~
CH2H CH20Ac Ac CH2H
~ N~H Ac2 >-- N~NaOC~I ~N~
HO ~ ~ D AcO ~ ) 3 D HO-~
~ Pyridine ~ MeOH ~
HO OH OAc OAc-4CH3CCCCH3 OEl OH
Ac = - C - CH
o An acid amide of the general formula II can be reduced to the corresponding am~ne of the formula I (R = H) with a complex metal hydride or with a horon hydride compound. It is preferable to use NaBH4 in pyridine or a sodium acyloxyborohydride, particul-arly sodium trifluoroacetoxyborohydride. In general, the reducing agent is employed in excess. Sodium trifluoroacetoxyborohydride can be produced in situ from sodium borohydride and trifluoroaoetic acid. Possible solvents are, in addition to pyridine, polar aprotic solvents, such as dioxane, tetrahydrofurane or diglyme.
The reaction is preferably carried out at the boiling point of the ;
solvent used. LiAlH4 can also optionally be used for the reduction, preferably when the hydroxyl groups are first protected in the customary way.
., -. . .
llZ343~
The reactive alkylating agents of the general formula IX
are kncwn or can be prepared by customary processes. The reaction with a oompound of formula V can be carried out in an inert organic solvent, generally at from room temFerature up to the boiling point of the reaction medium, with or without the addition of an acid-binding agent.
Specific new active compounds according to the invention which may be mentioned are:
compounds of the formula: HO ~ N
HO ~ I
,,,_ Rl ,, CH3CHCH3 :
CH3 I CH2-CH3 :
,. , . , .. , ,.. : . ,, - ...
. ~z3~37 R
H3 C`CH-CH2 -H~ C
H3 C ~
H3C~- .
CH3 (cH2 )3-CH2- , 5 H3C~CH C 2 2 .
CH3~:HCH2 CH2 CH3 CY,3 CP:2-C, -C~2 CrI3 CH3 CHC~2 CH2--C~3 CH3 (cH2 )~-CH2- -C1~3 (CH2 )5-CH2- .
CH3 ~CHCH2 CH2 CH2 -CH3 .
CH3 CH- ( CH2 ) 3 -CH2 -CH3 (C~i2 )6-CH2-CH3 CH- ( CH2 j 4 -CH2 ~ ;~
. CH3 - (-CHz ) B -CHz--CH3-(cHz ?lo~CH2~ . ~
Ci~3--(cH2 )l 2--CH2~ ~; r.
CH3 - ~ CH2 ) 1 4 -C~2 ~ ~' CH3 - ( CH2 ) 1 6 -C~2 ~
O-CH2-- , ~CH
O-~H2 -CY2 -HO-C.H2 -C.i2 -H3 C-CH-CH2 ~
OH
Le A 18 389 - 32 ~ , ~Z34~7 1~
HOH2 C-CH2 -CH2 - , - HOH2 C-CH.z -cH2 -CH2 -HOH2C-(CH2 )~-C~2- ' CH3 -CH- ICH-CH2 ~ : :
CY~ OH
HO-CH2 - ,CH-CY'2 - .
OH
- C3 }I, OCH2 -CH2 -c~ScooC~72-CE~-2- , ~C-OCH2 CH2 CH2 CH2 - ,~
H2 N-cH2 -CH2 - i H3 C ~ -,N-CH2-CH2-CH3 CONH-CH2 -CH2 ~
~-~ -NH-C H2 -C-~2 - ~, C2 H5 0 IC~ r~-CH2 -C.~z -ICH3 . ~ .-CH3 CO-N-C~2 -CH2 ~ P
C~3 NH-co-NH-cH2 CH2 - ~ ' H-50-NH-CH2 CH2 - }
C~3 ~I~H-cs-NH-cH2 C~2 - ~:
. ~NH-CS-NH-CH2-5H2- .
CH3 CO~HCH2 CH2 CH2 -~j-CONHCH2 CH2 CH2 - .
CH3 ~ ICONHCH2 CH2 CH2 -', " ' ' Le A lQ -,8~ _ 33 _ -- ~
., ' ' ~
l~Z3437 ~:
R
H2 N-CHz CHz CH2 CH2 - -H2 C=CH-CH2 -~ c Hc=cH cH2-- e H2 C=CH-CH2 -CH2 - ~?
H2 C=CH-CH2 -CH2 -CH2 -CH2 - . ~.
- H2 C=CH- ( CH2 ) 7 -CH2 - .
HOOC-CH2 ~
HOOC -CH2 -5 H2 ~ .
~ ~ Hs C2 OOC-CH2 -CH2 - .
~2 N-C-CH2 - . b O ~ r C2 ~5 ~--5-5H2 C~, Hg -HN-C-CH2 O
HO3 S-CH2 CHz CH2-- , H2 ~02 S-CH2 CH2 CH2 - , C~2-~C COH
.. NO2 ~
~C~2- ' ~;
B~ ~ .
-CH2-- , ,.
~3CO ~;
ZO HO~CH2-- 1 H-C~C-CH2- ~ t HO~CH2- ~, H3CO .
HO-~CH2 - .
Le A ~ 8 ~39 - _ 34 llZ343'7 ~:
R
HO3 S~CHz -N2 ` ' . .
,~H ~:
H3 CO~OCH~ ~ 12 ~" L
C H ' Na 03 S~CH2 _ $~
S03 Na .
$~-CH2--. - ~ t ~C H2 ~ ' Cl~CH2_ , X
~CH2:
Cl ~gj-cH
Br ~CH
~, Le A 18389 _ 35 _ ~
,.
39~37 , '' .
Br~CH2- . ,i ~CHz-~CHz- ~
~ Cl~CH2- ~, k _ ~CH2- ~.
F~CH2-2 N~-C~2 ~
HO~CH2_ ~ ,.
~NO2 HO i.
.' ' . ~:
~CH2 HO~CH2- ~, OH
Le A 18 38, -36 ~ -, !
~ 3~37 .
R
OH
~ 2 . .
OH . '. ~
HO ;, Ho~5H2- .
HOOC~_CH
< o ' HO~CH
COOH
~CH2-H3 C~CH2 - .
~CH~ ~, CH2 - ' . .~
OC~13 ~ .
rHO~CH2 - . h _~_ ' H3 . .
OH
H3 CO~CH2 -CH3 CO~rrl~CH2 -Le A 18 ~89 37 . . .
1~23437 . ~! ~
:~ ~CH2- ~
CH3 ~ .
~jC2H5 H3 CO~cH2_ OCH3 ~
. ~C~2- _ OC~3 0~
OC~H ) 1l i .. OC~3 , ~
H3 CO~C~-2 - ~.s o~ , ~ . f CHe-~Hz-C~Az-~ (~ N-CH2 -CHz -CH
~ CH2_ 1 _ Le A 13 ,39 - 38-.
- . . .
; - - ~ ,, ... .
3~37 `~ 1 HO~OH
HO~
O-C.Y2 -C H2 -~CH
,_ ~3--CH2 _ ' ~CH2- 1' .
Br~ CH2 - ¦
~RCH2-CH2 - ' ~
CH2-- - .~ ,, ~CH2 - ' .
.' ' ' . . .
-' Le A 1~ 389 _ 3 9 _ - ~
" , , , ~.
$
llZ3~.37 C~=pounds of the formula HO~
Rl` R3 ~~ CH C~2-CH3 CH2 CH2 - i H- CH ( CH2 ) 6 -CH2 -H- ~ ~ . H3 C-O-CH2 ~
H- . H5 C2 -O-CH2 - -lQ . . H-- ~-COO-CH~- ¦
H-- CH3 CO-NH-CH2 ~
H- ~CO-~H-CH2- .
~ H- . ~CO-N-CH2-H- CH3 ~HCONH-CH2 ~
~, H- ~NHCONH-CH2-H-- CH3-CH2-N-IC~CH2~
H-- . . C2T~5 OCONH-CH2 ~
HO-CH2 -CH2 - i ., ~: ' H- ~ . _ H- -COOH
H- ~3 C-S2 ~ -CH2 -H- H3 C-H2 C-SO2 -r~-CH2 -~.
H ~ SO2-N-CH2-Le A 18 ~39 .. . ~ ~ ~ ~' ' ~' .
..
~lZ343'7 Rl ~3 ~`
{~H3 - C}~3 - ' ~, CH3--, . CH3 CH2 - .
~CH3 ~ CH3 CH2 ~H2 . ~
C-~3 - ~ C1~3 ( C~-2 ) 6 -CH2 -CH3 - H3 C-O-C~2 - ~ 6 ~` - CH3 - . H5 C2 -O--CH2-- ' C.t}3 - H3 c-COO-CH2 - ~ . _ CH3-- ~COO-CH2-lO ~ CY.3 - H2 N-CH2 ~
CH3 - C~3 CO-l`rH-CH2 -CH3-- ~CO-NH-CH2-. ~ CH3 CH3- ~CO-~I-CH2- ~
CH3 - CH3 N~CO~H-CH2 - ~ E
: 15 C~3- ~NHCONH,-CH2-CH3 - CH3 -CH2 -~- ,C,-NH-CH2 ~ ~ ~, C~3 - C2 Hs OCONH-CH2 -C-~.3-C.~3- -COOH
c~3-- --COt`JH2 ;
-CH3 - H3 C-SO2 -N-CHz ~
CH3-- H3 C-H2 C-H2 C-SO2 -~-CH2 -H
CH~ H. .
_ Le A 18 ~8~ ~ 41 - ~
~Z3~37 ~ ~
Co~pounds of the formula H~
~ With respect to the configuration at,the C-1 atom, the examples listed below include both the -form and the ~-form . . ~ .
R2 , _ . . . . .
H- . H2N-CH2--~ CH3CO-NH-CH2-H- ~)-CO~ CH2-CH3 ~ ~
- H- ~ C0-N-CH2- j H- CH3~HCONH-CH2-H~ HCO~H-CH2- !i, H- CH3 -CH2-N-Icl-NH-cH2- ~ "
H- C2H50cONH-cH2- , H- -COOH .
H- -COOc2Hs- -~
~ -CONH2 H- ~ H3C-S02-N-CH2 .
H ~3 C-H2 C-~-2 C-S02 -~ -CH2 - ~ ;
X-- ~-SOz~N~CH2 ~ ~
H- H0-CH2- _ -20 . H- H5C2-C00-C~2-C~.3 - ` CH3Co-NHCH2~
CH3- , ~ -C0-NH-CH2-CH3- ~CO-i~-C~2-2~ CH3- CH3NHCONH-CH2-Le A 18 ~89 _ 42_ llZ3437 Rl R2 ~, ~
~ L
- ~CH~- ~ NTHCONH~-CH2-~CH3-- . CH3-CH2-H-C-NH-~
CH3- ~2~soco~rH-cH
: 5 CH3- -COOH
CH~- -CONH2 .
H3C-H~C-HzC~s02-H-cH
CH3- ~ SO2-N-CH2-CH3- HO-CH2_ CH3- HsC2-COO-c~2-C~3- -SO3H ~ ' .
CH3- -O-CH,-CH2-CH2-CH3 C~3- -S-CH2-CH3 t,l ,~
CH3 - - ~TH2 ~ r c~3- -NH-CH3 .
, - , - ~; .
Compounds o~ the ~ormula H ~HO H,R~ ~ _ ~ith respect to the configuration at the C-2 atom, the examples listed below include both the a-form and the ~-Lor~ .
_ Le ~ 18 389 - - -~
-t, . R2 ., _ . .
H2 I~-CH2 -~CO-~I-c~2 -CH
~CO-~-C~2 -CH3 N}HCONH-CH2 ~
~\~NHC ONH-CH2 ~
CH3 -CH2 - - ,C-hH-CH2 ~ .
C2 Hs OCONH-CH2 --COO~I - , , --CONH2 ~ ~A
H3 C-SO2 -N-CH2 - ~ --~3 C-H2 C Hz C-SO2 -N-CH2 - r - ~SO2-N-CH2-~O-C~12 - . . ~:
Hs C2 -- ~C, -O-CH2 -' O . . ~.
r 1~ R2 R2 ~ g ~ ~
-OH -O-CH2-CH2-CH2-CH~
-C~ -SH
, . ' ' . _ Le A ~ ~89 _ 44- -- I
`
.~ .
343~ ~
' HO CH2 0~ ~ ~f Compounds of the formula ~N-R1 r HO ~H,OH
OH
Rl ' ,' -CH2-CH3 . ,; ~, -CH2 -CH2 -C~ -C ~3 - .
-CH2-(CH2 )16 )-CH3- ';
~CH3 CH3 . ~ .
-C~2~ ~' ~
-CH2-CH=CH2-- -CH2-CH2-()C~3--CH2 -CH2 -N~ CCH~3 i r~
-CH2 ~
Com~ounds of the formula HO CH2 OH ~ ,.
HO~ \H ~0 S r' R~
~ .
-CH2 -C ~3 - CH2 -CH2 -CH2 -c~-3 -CH2 - ( CHz ) 1 6 -CH3 - ~ CH3 CH "
_C~,2~
-CH2 -CH=CH2 . -C.Y2-CH2-OCH3 !.e A 18 ,89 _ 4S_ .
! .
:- ' ' ' '. . .. ~ , , ', :
l~Z3~37 .
-CH2-CH2-N ~ 3 HO
-CH2~
CH OH
Ccmpounds of the formLla HO ~ M
HO ~ -- R~
OH H, CN
Rl :- 2 2 2 3 -CH2- (CH2) 16-CH
CH3 ~:
-CH
`;
C 2 ~
-CH2-CH=CH2 ~ CH
-CH2-CH2-N~C 3 HO : :~
2 ~
The inhibitors according to the invention are suitable for use as therapeutic agents for the following indications: prediabetes, gastritis, constipation, infactions of the gastro intestinal tract, meteorismus, flatulence, caries, atherosclerosis, hypertension and in particular obesity, .~ :
1~341~37 diabetes and hyperlipoproteinaemia. To broaden the activity spec-trum, it is possible to ccmbine inhibitors for glycoside-hydrolases w~ich cc~plement one another in their action, the combinations be-ing either combinations of two or more compounds according to the invention with one another or cQmbinations of the compounds accord-ing to the invention with inhibitors ~hich are already known. m us, for example, it can be appropria~e to combine saccharase inhibitor compounds according to the invention ~ith amylase inhibitors which are already known.
In some cases, combinations of the compounds according to the invention with kncwn oral antidiabetic agents (~i-cytotropic sul-phonylurea derivatives and/or biguanides having an action on the blood sugar) and with blood lipid-lowering active co~lpounds, such as, for example, clofibrate, nicotinic acid, cholestyramine and others, are advantageous.
m e ccmpounds can be administered without dilution, for example as a powder or in a gelatine casing, or in ccmbination with an excipient in a pharma oe utical composition.
The present invention provides a pharmaceutical composi-tion containing as active ingredient a co~pound of the invention in admixture with a solid or liquefied gaseous diluent, or in admix-ture with a liquid diluent other than a solvent of a molecul æ ~ ~
weight less than 200 (preferably less than 350) ex oe pt in the pre- -sen oe of a surfa oe active agent.
m e invention further provides a pharmaceutical c~mposi-tion CQntaining as active ingredient a ccmpound of the invention in the form of a sterile and/or physiologically isotonic aqueous solu-tion.
m e invention also provides a medicament in dosage unit form comprising a compound of the invention.
, - 47 - ;~
.. , .. .. , , ~ ~
~23~37 The invention also provides a medicament in the form of tablets (including lozenges and granules), dragees, capsules, pills, ampoules or suppositories comprising a compound of the invention.
"Medicament" as used in this specification means physic-ally discrete coherent portions suitable for medical administration.
"Medicament in dosage unit form" as used in this speciflcation means physically discrete coherent units suitable for medical admin-istration each containing a daily dose or a multiple (up to four times) or sub-multiple (down to a fortieth) of a daily dose of the ccmpound of the invention in association with a carrier and/or en-closed within an envelope. Whether the medicament contains a daily dose, or for example, a half, a third, or a quarter of a daily dose will depend on whether the medicament is to be administered on oe or, for example, twice, three times or four times a day respectively.
The pharmaceutical ccmpositions accordLng to the inven-tion may, for example, take the form of suspensions, solutions and emulsions of the active ingredient in aqueous or non-aqueous dilu-ents, syrups, granulates or pcwders.
m e diluents to be used in pharma oe utical compositions ~ ;
(e.g. granulates) adapted to be formed into tablets, dragees, cap-sules and pills include the following: (a) fillers and extenders, e.g. starch, sug æ s, mannitol, and silicic acid; (b) binding agents, e.g. carboxymethyl oe llulose and other oe llulose derivatives, alginates, gelatine and polyvinyl pyrrolidone; (c) moisturizing agents, e.g. gly oe rol; (d) disintegrating agents, e.g. agar-agar, ~: . . :` .
l~Z3D~3~7 calcium carb~late and sodium bicarbonate; (e) agents for retarding dissolution e.g. paraffin; (f) resorption accelerators, e.g.
quaternary a~monium ccmpounds; (g) surfa oe active agents, e.g.
oe tyl alcohol, gly oe rol monostearate; (h) adsorptive carriers, e.g.
kaolin and bentonite; (i) lubricants, e.g. talc, calcium and magnesium stearate and solid polyethylene glycols.
Ihe tablets, dragees, capsules and pills formed from the pharma oe utical compositions of the in~ention can have the customary coatings, envelopes and protective matri oe s, which may contain cpacifiers. m ey can be so constituted that they release the active ingredient only or preferably in a particular part of the intestinal tract, possibly over a period of time. me coatings, envelopes and protective matrices may be made, for example, of polymeric substances or waxes.
m e ingredient can also be made up in microencapsulated form together with one or several of the above mentioned diluents.
m e diluents to be used in pharmaceutical compositions adapted to be formed into suppositories can, for example, be the usual water-soluble or water-insoluble diluents, such as poly-ethylene glycols and fats (e.g. cocoa oil and high esters [e.g.
C14-alcohol with C16-fatty acid]) or mixtures of these diluents.
.
., ~ . :
:llZ34~'7 The pharm~ceutical compositions which are solutions and emulsions can, for example, contain the customary diluents (with, of course, the above mentioned exclusion of solvents having a mole-cular weight belcw 200 except in the presen oe of a surfaoe-active agent), such as solvents, dissolving agents and emulsifiers;
specific examples of such diluents are water, ethyl alcohol, iso-propyl alcohol, ethyl carbonate, ethyl aoetate, benzyl alcohol, benzyl benzoate, propylene glycol, 1,3-butylene glycol, dimethyl-formamide, oils [for example sround nut oil], gly oerol, tetrahydro-furfuryl alcohol, polyethylene glycols and fatty acid esters of sorbitol or mixtures thereof.
For parenteral administration, solutions and emulsions should be sterile, and, if appropriate, blood-isotonic.
The pharmaoeutical compositions which are suspensions can CQntain the usual diluents, such as liquid diluents, e.g. water, ethyl alcohol, propylene glycol, surfaoe-active agents (e.g. ethoxy-lated isostearyl alcohols, polyoxyethylene sorbite and sorbitane esters), microcrystalline cellulose, aluminium metahydroxide, bentonite, agar-agar and tragacanth or mixtures thereof.
All the pharmaoeutical comFositiQns according to the ~Z3437 invention can also contain colouring agents and preservatives as well as perfumes and flavouring additions (e.g. peppermint oil and eucalyptus oil) and sweetening agents (e.g. sacch æ in).
m e pharmaceutical compositions according to the inven-tion generally contain from 0.1 to 99.5, usually from 0.5 to 95~ of the active ingredient by weight of the total composition.
In addition to a compound of the invention, the pharma oe u-tical co~positions and medicaments according to the invention can also contain other ph æ maceutically active compounds. m ey may also contain a plurality of compounds of the invention.
Any diluent in the medicaments of the present invention may be any of those mentioned above in relation to the pharma oe u-tical compositions of the present invention. Such medicaments may include solvents of molecular weight less than 200 as sole diluent.
m e discrete coherent portions constituting the medica-ment according to the invention will generally be adapted, by virtue of their shape or packaging, for medical administration and may be, for example, any of the following: tablets, (including lozenges and granulates), pills, dragees, capsules, suppositories and ampoules. Sc~e of these forms may be made up for delayed re-lease of the active ingredient. Some, such as capsules, include a protective envelope which renders the portions of the medicament physically discrete and coherent.
m e preferred daily dose for adminis-tration of the medica-ments of the invention is from 500 to 5 x 106 SIU (as defined , , ~L~Z3437 hereinbelow) or from 1 to 3500 mg, most preferably from 10 to 500 mg active ingredient.
; The production of the above mentioned pharmaceutical com-positions and medicaments is carried out by any method known in the art, for example, by mixing the active ingredient(s) with the diluent(s) to for,n a pharmaceutical ccmposition ~e.g. a granulate) and then forming the co~position into the ~edicament (e.g. tablets).
This invention further provides a method of combating (including prevention, relief and cure of) the above mentioned diseases in warm-blooded animals, which comprises administering to the anLmals a oompound of the invention alone or in admixture with a diluent or in the form of a medicament according to the invention.
It is envisaged that these active compounds will be administered perorally, parenterally (for example intramuscularly, intraperitoneally, subcutaneously or intravenously), rectally or locally, preferably orally. Preferred pharmaceutical compositions and medicaments are therefore those adapted for oral administration, such as tablets, capsules, powders, dragees, granules, suspensions and solutions. Administration in the method of the invention is pre~erably orally.
In general it has proved advantageous to administer amounts of from 10 to 1 x 104 SIU (as defined hereinbelow) or amounts of from 0.01 mg to 100 mg, preferably from 0,1 to 10 mg, per kg of body weight per day to achieve effective results. Never-theless, it can at times be ne oe ssary to deviate fr~n those dogage rates, and in particular to do so as a function of the nature and body weight of the human or animal subject to be treated, the ;;
~ ,:
1~3437 individual reaction of this subject to the treatment, the type of formulation in which the active ingredient is c~dministered and the mode in which the administraticn is carried out, and the point in the progress of the disease or interval at which it is to be admin-istered. m us it may in some case suffice to use less than the above mentioned mLnimwm dosage rate, whilst other cases the upper l;mit mentioned must be exceeded to achieve the desired ~esults.
Where l æ ger amounts are administered it can be advisable to divide these into several individual administrations over the course of the day.
In addition to the above mentioned pharmaceutical co~posi-tions, foodstuffs containing these active compounds can also be pre-pared; for example sugar, bread potato products, fruit juice, beer, chocolate and other confectionery, and preserves, such as, for example, jam, a therapeutically active amount of at least one of the inhibitors according to the invention having been added to these products.
The food products produ oe d using the active cc~,pounds according to the invention are suitable for use both in the diet of patients suffering from metabolic disorders and for the nutrition of healthy persons in the sense of a method of nutrition for the prophylaxis of metabolic disorders.
Further~ore, the inhibitors according to the invention have the property, in animals, of influencing to a high degree the ratio of the proportion of undesired fat to the proportion of de- ;
sired meat of lcw fat content (lean meat) in favour of the lean meat. This is of particular importance for the rearing and keeping of agricultural stock animals, for example in the fattening of pigs, ~ . .
- , ~3437 but is also of considerable importance for the rearing and keeping of other stock animals and pets. Furthermore, the use of the inhibitors can lead to a considerable rationalisation of the feed-ing of the animals, both in respect of time, quantity and quality.
Since they cause a certain delay in cligestion, the residence time of the nutrients in the digestive tract is extended, whereby ad libitum feeding associated with less expense is made possible.
Furthermore, in many cases there is a considerable saving of valu-able protein feed when the inhibitors according to the invention are used.
m e active c~m~ounds can thus be used in virtually all spheres of ani~al nutrition as agents for reducing the formation of fatty layers and for the conservation of feed protein.
The activity of the active compounds here is essentially independent of the nature and the sex of the animals. The active compounds prove particularly valuable in species of animals which tend generally to deposit relatively large amounts of fat, or tend to do so during certain stages of their life.
The following stock animals and pets may be mentic~ned as examples of animals for which the inhibitors for reducing the forma-tion of fatty layers and/or for conserving feed protein can be employed: warm~blooded animals, such as cattle, pigs, horses, sheep, goats, cats, dogs, rabbits, fur-bearing animals, for example mink and chinchillas, and other pets, for example guineapigs and hamsters, laborator~ animals and zoo animals, for example rats, mi oe , monkeys and the like, poultry, for example broilers, chickens, ~I
. ~
~Z343~
geese, ducks, turkeys and pigeons, parrots and canaries, and cold-blocded animals, such as fish, for example carp, and reptiles, for example snakes.
Because of the advantageous properties of the active com-pounds of the invention, the amount of active compound administered to the animals in order to achieve the desired effect can be varied within broad limits. It is preferably frc~ 0,1 to 1000 mg most pre- ~;
ferably from 1.0 to 100 mg/kg of feed per day. The period over which the active cc~pound is administered can be from a few hours or days io several years. The appropriate amount of active ccmpound and the appropriate period over which it is administered are closely connected with the object of feeding. In particular, they depend on the nature, the age, the sex and the state of health and the method of keeping the animals and can be easily determined by any expert.
m e active compounds according to the invention may be administered to the animal by customary methods. m e nature of the administration route depends, in particular, on the nature, the behaviour and the general condition of the animals. Thus it is possible to carry out the administration orally once or several times ~;ly, at regul æ or irregul æ intervals. In most cases, oral administration, in particular in synchromism with the food and/
of drink intake of the animals, is to be preferred for reasons of expediency.
m e active ccmpounds of the invention may be administered as pure substan oe s or in a formulated form, the expression "formul- ;
ated fokm" incluc~ng both a premix for admixture with the animal .::, .
: - .
~W~3'7 feed or drinking water, that is to say mixed with a non-toxic inert carrier of any desired nat~lre, and also as part of a total ration in the form of a supplementary feed and as a constituent of the mix-ture of a mixed feed by itself. Administration of suitable formula-tions by means of the animal drinking water is also included.
The active co~pounds accordLng to the invention, option-ally in the formulated form, can also be administered, in a suit-able form, together with other nutrients and active compounds, for exa~ple mineral salts, trace elements, vitamins, proteins, energy carriers (for example starch, sugar or fats), dyestuffs and/or flavouring substances or other feedstuff additives, such as, for example, growth promoters. The active compo~nds of the invention can be administered to the animals before, during or after their food intake.
Oral administration together with the feed and/or drink- `
ing water is advisable, the active conpounds being added to the total amount or only to certain parts of the feed and/or drinking water, depending on the requirement.
The active conpounds of the invention can be added to the feed and/or the drinking water according to customary methods by simple admixture of the pure conpound, preferably in a finely divided form, or in a formulated form mixed with edible, non-toxic carriers, and optionally also in the form of a premix or a feed CQn-centrate. --m e feed and/or drinking water can, for example, contain the active compo~mds according to the invention in a concentration of f m m 0.001 to 5.0 % o, most preferably from 0.01 to 2.0/oo (by weight). The optimNm level of the CQncentration of the active com-:
', :. , :: . .
~3437 pound in the feed and/or drinking water depends, in partic~lar, on the size of the feed and/or drinking water intake of the animals and can be easily determined by any person skilled in the art.
~ he nature of the feed itself and its composition does not normally influence the utilisation of the campounds of the invention. m us it is possible to use all the current, co~merci-ally available or special feed compositions, which preferably con-tain the custamary prop~rtions of energy substances and proteins, including vitamins and mineral substan oe s, necessary for balanced nutrition. me feed can be composed, for example, of vegetable sub-stan oe s, for example shredded oil-cake, shredded cereal and cereal by-prcducts, but also of hay, sila~e fodder, beets, and other forage plants, of animal substances, for example meat and fish pro-ducts, bonemeal, fats and vitamins, for example A, D, E, K and B-ccmr plex, as well as special sour oe s of protein, for example yeasts and oertain amino-acids, and mineral substances and trace elements, such as, for example, phosphorus and iron, zinc, manganese, oopper, cobalt, iodine and the like.
Premixes can preferably contain frQm 0.1 to 50%, most pre-ferably fram 0.5 to 5.0% (by weight) of, for example, N-methyl-l-desoxynorjirimycin, in addition to any desired edible carrier and/or mineral salt, for example carb~nated feed lime, and may be prepared by customary mixing metho~s.
Mixed feeds preferably contain from 0.001 to 5.0/oo, in particular from 0.02 to 2.0 % o (by weight), for example, of N-methyl-l-desoxynorjirimycin, in addition to the custamary raw mate-rial camponents of a mixed feed, for example shredded cereal or ' ~
~ ~23~37 oereal by-products, shredded oilcake, animal protein, minerals, trace elements and vitamins. mey can be prepared by customary mixing methods.
me active compounds of the invention when in pr~mixes and mixed feedstuffs can preferably also be appropriately protected from air, light and/or moisture by suitable agents which cover their surface, for example with non-toxic waxes or gelatine.
me following is an example of a co~,position of a finished mixed feed, for poultry, containing an active ccmpound according to the invention: 200 g of wheat, 340 g of maize, 360.3 g of coarse soya bean meal, 60 g of beef tallow, 15 g of dicalcium phosphate, 10 g of calcium carbonate, 4 g of iodinated sodium chloride, 7.5 g of a vitamin/mineral mixture and 3.2 g of an active comFound premix yielding, after careful mixing, 1 kg of feed.
The vitamin/mineral mixture consists of: 6,000 I.U. of vitamin A, 1,000 I.U. of vitamin D3, 10 mg of vitamin E, 1 mg of vitamin K3, 3 mg of riboflavin, 2 mg of pyridoxine, 20 mcg of vitamin B12, 5 mg of calcium pantothenate, 30 mg of nicotinic acid, 200 mg of choline chloride, 200 mg of MnSO4 x H20, 140 mg of ZnSO4 x 7H2O, 100 mg of Fe ~ x 7H20 and 20 mg of CuSO4 x 5H20. The - --active ccmpound premix contains, for example, N-methyl-l-desoxynojirimycin in the desired amount, for example 1,600 mg, and in ~ tion 1 g of DLrmethionine and encugh soya bean flour to form 3.2 g of premix.
m e follcwing is an example of the composition of a mixed feed for pigs, which feed contains an active compound of the formula I: 630 g of shredded oereal feed (cc~posed of 200 g of ., . . :. , .
~23~3~
shredded maize, 150 g of shredded barley, 150 g of shredded oats and 130 g of shredded wheat), 80 g of fish-meal, 60 g of coarse soya bean meal, 58.B g of tapioca flour, 38 g of brewer's yeast, 50 g of a vitamin/mineral mixture for pigs (constitution for example, as in the chicken feed above), 30 g of linseed cake meal, 30 g of maize gluten feed, 10 g of soya bean oil, 10 g of cane sugar molasses and 2 g of active ccmpound premix (constitution for example, as in the chicken feed above~ yield, after careful mixing, 1 kg of feed.
The feed mixtures indicated are intended, preferably, for the rearing and fattenLng of chickens or pigs respectively; however, they can also be used in identical or similar compositions for the rearing and fattenLng of other animals.
The oQmpounds of the invention can be used individually or in any desired mixture with one another.
In vitro saccharase inhibition test The in vitro saccharase inhibition test makes it possible to determine the enzyme-inhibitory activity of a substan oe by com-parison of the activity of the solubilised intestinal disaccharidase ccmplex in the presence and in the absen oe (so-called 100~ value) of the inhibitor (compcund under scrutiny). A virtually gl-ucose-free sucrose (glucose clOO ppm) is used here as the substrate which determines the specificity of the inhibition test; the determina- ;
tion of enzyme activity is based on the spectrophotometric deter-mination of glucose liberated, using glucose dehydrogenase and nicotinamide-adenine dinucleotide as the cofactor.
One saccharase inhibitor unit (SIU) is defined as that - . ~
`~3437 inhibitory activity which, in a defined test batch, reduces a given saccharolytic activity by one unit (saccharase unit - SU); the saccharase unit being defined here as that enzyme activity which splits off one ~mol of sucrose per minute under given conditions and thus leads to the liberation of o~e ~mol each of glucose, which is determined in the test, and fructose, which is not recorded in the test.
The intestinal disaccharidase co~,plex is obtained from swine small intestine mucosa by tryptic digestion, precipitation from 66% strength ethanol at -20 &, taking up of the precipitate in 100 mM phosphate buffer, pH 7.0, and finally dialysis against the same buffer.
100 ~1 of a dilution of the intestinal disaccharidase com~
plex in 0.1 M maleate buffer, pH 6.25, æ e added to 10 ~1 of a sample solution, which is prep æ ed so that the extinction of the test batch is at least 10%, but not re than 25%, below that of the 100% value, and the mixture is pre-incubated at 37C for 10 minutes. The dilution of the disaccharidase complex should norm~lly be adjusted to an activity of 0.1 SU/ml.
The sacch æ olytic reaction is st æted by adding 100 ~1 of a 0.4 M solution of sucrose ("SERU~ 35579") in 0.1 M maleate buffer, pH 6.25, and, after an incubation period of 20 minutes at 37C, is stopped by adding 1 ml of glucose dehydrcgenase reagent (1 small bottle of lyophilised glucose dehydrogenase/mut æ otase mixture ("MERCK 14053") and 331.7 n~ of ~-nicotinamide-adenine dinucleotide (free aeid "BOE~rgnNOE R" degree of purity I) dissolved in 250 ml of 0.5 M tris buffer, pH 7.6). In order to determine the glucose con-.~
- ,, ~ ; ~ : .
~L:Z3~37 centration, the mixture is incubated at 37C for 30 minutes and finally is measured photGmetrically at 340 nm against a reagent blank ~containing enzyme b~t without sucrose).
me calculation of the inhibitory activity of inhibitors is made difficult by the fact that even sli~ht changes in the test system, for example a 100% value which varies slightly from deter-mination to deter~ination, can have a sig~ificant effect on the test result which cannot be ignored. These difficulties may be avoided by running a standarl with every determinationj a saccharase inhibitor of the formula C25H43O18N whi~h has a specific inhibitory activity of 77,700 SIU/g and, when employed in the test in amounts of 10 to 20 ng, leads to an inhibition of the order of size specified above, is conveniently used as the standard. If the differen oe between the extinctions at 340 nm of the 100% value and of the batch inhibited by the standard is knGwn, the specific inhibitory activity of the inhibitor, expressed in saccharase inhibitor units per gram (SIU/g), can be calculated in a knGwn manner from the extinction difference between the 100% value and ` the batch inhibited by the sample solutiGn, taking into considera-tion the amount of inhibitor employed.
` Specific saccharase-inhibitory activity in vitro l-Desoxynojirimycin465,000 SIU/g - N-Methyl-l-desoxynojirimycin2,330,000 SIU/g Preparation Examples -Example 1 N-Methyl-l-deso~ynojirimycin 3~37 OEl OH
; N\- ~H3 HO ~
HO OH
3.2 g of l-desoxynojirimycin and 2 ml of 30~ strength a~ueous formaldehyde are added to 4 ~ of 98~ strength fo~mic acid, whilst cooling with i oe. The mixture is then heated ~mder reflux for 8 hours. After cooling, the reaction mixture is diluted with a oe tone. A resinous precipitate separates out. The acetone solu-tion is decanted off and the resin is rinsed several times with ace-tone. The residue is then dissolved in distilled water and the solution is freed from formic acid by adding a basic ion eYchanger in the OH form (Amberlite JRA 410). m e ion exchanger is filtered off and the aqueous solution is brought to dryness under reduced pressure. 3.0 g of resinous N-methyl-l-desoxynojirimycin remain.
The compound can be further purified by chromatography on oe llulose.
; Water-containing butanol is used as the running agent. m e com- p~und may be cristallized from ethanol. M.P.: 153 &.
~lass spectrum: The most important peak in the upper mass range is at m/e = 146 (M~CH20H)-For further characterisation, the ccmpound is converted into the pera oe tylated compound, N-methyl-2,3,4,6-tetra-O-acetyl-l-desoxynojirimycin, with acetic anhydride/pyridine 1:1 at ro~m temperature. A proton magnetic resonance spectrum of this deriva-tive in CDC13 was reasuIed at 100 M3z: 4 singlets Eor t e total of .
;~ ~
.
~
1~
12 protons, which correspond to the methyl groups of the O-acetyl groups (CH3-O-C-), are found between ~ = 2.0 and 2.1 ppm. The o methyl group bonded to N (CH3-N<) is found as a singlet at ~ = 2.45 ppm. Two protons on a C atom bonded l:o nitrogen (H-C-N<) absorb as poorly resolved multiplets between ~ = 2.1 and 2.5 ppm. A further proton of this type appears as a doublet of a doublet (Jl = 11 HZ;
J2 = 4 HZ) at ~ = 3.18 ppm. A methylene group (-CH2-O-C-C~3) .
absorbs as an AB system at ~ = 4.16 and ~ = 4.22 ppm. The remain-ing three protons (-C-O-C-CH3) are found as a mul-tiplet between ll H O
10 ~ = 4.9 and 5.2 ppm.
Example 2 N-n-Butyl-l-desoxynojirimycin CH20H , ~ N - CH2 - CH2 - CH2 C 3 HO ~
HO OH
12.5 r~ of n-butyraldehyde, 0.01 mols of methanolic HCl and 1.5 g of NaCNBH3 are added sucoessively to 3.2 g of l-desoxyno-jirimycin (0.02 mol) in 40 rnl of absolute methanol, whilst cooling with ice and stirring. The reaction mlxture is stirred at room temperature for 12 hours. It is then concentrated to dryness on a rotary evaporator. The residue is dissolved in 50 ml of water and extracted 3 times with 30 ml of CHC13 each time. me aqueous phase is again brought to dryness, the residue is taken up in 30 ml of . ~ . ~ .
~Z343~7 H2O and the solution is discharged onto a column 50 cm long and 2 cm wide which is filled with a strongly basic ion exchange resin in the OH form (A~berlite IRA 400 or Dowex 1 x 2).
The reaction product is eluted with water and the indivi-dual fractions are investigated by thin layer chromatography.
(Silica gel plates; running agent: ethyl acetate/methanol/water/25%
strength ammcnia 100:60:40:2; spray reagent: KMnO4 solution). The fractions which contain N-n-butyl-l-desoxynojirimycin are collected and the aqueous solution is concentrated on a rotary evaporator.
Acetone is added to the residue, whereupon crystallisation occurs. ~ -The crystals are filtered off, rinsed briefly with ace-tone and dried. 3 g of N-n-butyl-l-descxynojirimycin of melting point 126-127& are obtained.
Mass spectrum: The most im~ortant peaks in the upper mass range are found at m/e = 188 (M~CH20H) and m/e = 176 (M-CH2-CH2-CH3).
In the case of less reactive aldehydes, a molecular sieve 3A was added to the reaction mixture in order to bind the water of reaction.
The following compounds were prepared by methods analogous to those of the above proo_dure:
N-Ethyl-l-desoxynojirimycin CH20H . .
~ \ 2 3 HO ~
HO OH
-3~37 ~ss spectrum: Intense peak at m/e = 160 (M-CH20H).
N-n-Propyl-l-desa~ynojiri~7cin ~ N - CH2 - CH2 - CH3 HO ~
HO OH
Mass spectrum: Intense Feak at m~e = 174 (M-CH20H).
Peaks also at m/e = 206 (M~H) and m/e = 204 (M~H).
N iso-Butyl-l-desoxynojirim~cin ~ N - CH2 - CH 3 HO ~ 3 :
~IO OH
Mass spectrum: The most important peaks in the upper mass range are found at ~ :
m/e = 188 (M~CH2OH), m/e = 176 (mrCH ~ 3), m/e = 220 (M~H) and m/e = 218 CH
(~H). 3 N-n-Heptyl-l-desoxynojirimycin , CH OH :
~N - CH2 - (CH2)5 - CH3 HO~ >
r~ .
HO OH
melting point: 111 - 113& (from aoe ton) Mass spectrum: The ~st important peak in the upper mass range is at m/e =
230 (M~CH20H). Peaks are also found at m/e = 262 (M~H) and 260 (M~H).
. ~
3~37 N-Benzyl-l-desoxynojirimycin CH OH
~-- CH2 ~
HO OH
melting point: 183 - 184 & (from methanol) Mass sprectrun: m e most important peak in the upper rnass range is found at ~/e = 222 (M~CH20H).
N-(2-Pyridyl)-methyl-l-de~oxynojirimycin ~-- CH2 ~
HO OH
melting point: 174 - 175 & (from ethanol) ~ass spectrum: The most important peaks in the upper rnass range are found at r~/e = 255 (M~H), r4~e = 236 (M-H20) and m/e = 223 (M~CH20H).
N-2-Hydroxyethyl-l-desoxynojirimycin ~ 2 2 HO ~
HO OH
melting point: 114 & (from ethanol) Mass spectrum: The most important peak in the upper rnass range is at m/e =
176 (M~CH20H).
N-2,3-DLhydroxy-n-propyl-l-desoxynojirimycin C~12H
HO ~ N ~ CH2 - CH - CH2 - OH ~:
~ OH
HO OH
3~
Mass spectrum: The m~st Lmportant peaks in the upper mass range are at m/e = 206 (M-CH20H) and m/e = 176. me substance is a mix-ture of two diastereomeric compounds.
N-(S-B-~ Glucopyranosyl-2-mercaptoethyl)-1-desoxy.nojirimycin HO CH
CH20H >--~
; \ CH2 - C~12 - S ~ ~ OH
HO ~ ~
HO OH
Mass spectr~m: The mass spectrum of the compound peracetylated in pyridine/acetic anhydride was measured. me most important peaks in the upper mass range are found at m/e = 648 (M~CH20-C-CH3), o m~e = 588 and mJe = 344.
me aldehyde required for the reaction was obtained from O-aoetylated l-thioglucose and chloroaoetaldehyde. me acetyl groups in the end product were split off by transesterification with catalytic amounts of NaOCH3 in MeOH.
N-Oxiranyl-methyl-l-desoxynojirimycin ,, CH OH
_~N ~ CH2CH -~CH2 ~_~ O ~ ~ :
OH OH
Yass spectrum: The most important peaks in the upper mass range are found at m/e = 219 (M), m/e = 202, m/e - 188 (M~CH20H) and m/e = 176 (M-CH - CH2). ;~
O ' '~
,~
:~Z3~3~7 ~ he substance is a mLxture of two diastereomeric com-pounds.
N-(3-N-Phthalimido-n-propyl)-1-desoxynojirimycin HOH~ CH - CH - CH - N~
OH OH
Mass spectrun: m e most important peaks in the upper mass range were ~ound at m/e = 348, m/e = 319 (M-CH20H), ~e = 301, m~e = 200, m/e = 188, m/Q = 174, m/e = 160 and m/e = 147.
In this case, chromatography on a basic ion exchange resin was dispensed with and the compound was purified by boiling up with a oe tone and recrystallisation from ethanol.
Melting point: 208 - 210 C. ~ -~
~-(3-Amino-n-propyl)-l-desoxynojirimycin CH OH
HO ~- CH2 - CH2 - CH2 N 2 HO OH :
Mass spectrum: m e most important peaks in the upper mass range are at m/e = 189 (M-CH20H) and m/e = 146. -m e compound was obtained from the above phthalimido com-pound by hydrazinolysis in methanol.
N-(l-Desoxynojirin~in-yl)-acetic acid ~`
:
^ ~ . - .
- .
3~3~
C~2 ~ N - CH - COCH
HO ~ 2 H~ OH
Mass spectrum: The most important peaks in the upper mass range are found at m/e = 203 tM-H2O), ~/e = 159, m/e = 145 and m/e = 100.
The oo~pound was not purified by chromatography over a basic ion exchange resin but by recrystallisation from methanol/water.
~lelting point: 187 - 188C.
N-o-Nitrobenzyl-l-desoxynojirimycin _~ CH2 ~ ~,, N2 1' HO OH
Rf value: 0.85 (on thin layer chrcmatography ready-to-use silica gel 60 plates from Messrs. Merck; running agent: ethyl acetate/methanol/H20/25~ ,~
strength ammonia 100:60:40:2).
For ocmparison: Rf value of l-desoxynojirimycin: 0.3. `::.
N-o,Car}o=ybenzyl-l-desoxynojirimycin , , - CH
CCOH
HO OH
Rf value: 0.7 ~lates and running agent as indicated for the above ccmpound).
''' ..
~Z~37 For purification, the co~lpound was chromatographed over a basic ion exchange resin as indicated above, but finally was eluted with 1% strength acetic acid.
N-p-Carboxybenzyl-l-desoxynojirimycin _ _ .
HO - CH
~ N - CH2 ~COOH
HO ~
OH OH
m.p.: 280 - 281 C (from H2O/methanol) Rf value: 0.7 (plates and running agent as indicated above).
In this case also, the co~pound was eluted from the basic ion exchange resin with 1% strength a oe tic acid.
N-p-Sulfobenzyl-l-desoxynojirimycin ~ ~ 2 ~SO3H
HO
HO OH .
4.8 g of benzaldehyd-4-sulfonic acid, 1.8 ml of a oe tic acid and 0.8 g of NaCNBH3 are added to 2 g of l-desoxynojirimycin in 40 ml methanol. The mixture was refluxed for 4 hours and stirred for 12 hours at room temperature. The precipitate was filtered off and recrystallized from water. 1.2 g of N-p-sulfobenzyl-l-desoxy-nojirimycin of melting point ~ 320C (dec.) are obtained.
. . : - ..
,~,~37 Example 3 N-~-Phenylethyl-l-desoxynojirimycin ~ H
HO ~
HO OH
3 g of phenylacetaldehyd and 0.8 g of NaCNBH3 are added to 2 g of l-desoxynojirimycin and 1.8 ml acetic acid in 40 ml of methanol.
The mixture is stirred for 12 hours at room temperature and evapor-ated on a rotary evaporator. The residue is dissolved in ethanol/
water (2:1) and discharged onto a column which is filled with a strongly acidic ion exchange resin in the ~- form. me column is washed with 2 1 of ethanol and water (2:1). Then the product is eluted with ethanol/2~ strength aqueous ammonia (2:1). me frac-tions are investigated by thin layer chromatography and those which contain the product are collected and dried. The residue is cry-stallized from 100 ml ethanol. 2.5 g of N-~-phenyl-ethyl-l-desoxy-nojirimycin with a melting point 179 - 181C are obtained.
me follcwnng compounds were prepared analogously: ~-N-n-Pentyl-l-desoxynojirimycin ;~
.~
( 2)4 H3 HO ~ j~
HO OH
m.p. 97C (from acetone) ;:
. . . .
~IZ~gl3'7 N-n-Hexyl-1-desoxynojirimycin ~ ~ ( 2)5 3 HO ~
HO OH
m.p. 112 - 113C (from ethanol/acetone) N-n-Octyl-l~esc~ynojir~lT~cin ~ N\- (CE12)7 - CH3 HO ~ ~`
HO OH :
m.p. 115 - 117& (from eth~ol/aoetone) N-n-Nonyl-l-deso~ynojiri~cin C~H20H
r N - (CH ) - CH
HO ~ ~
HO OH
"
m.p. 105 - 107& (from ethanol/aoetone) : `
, - - . . . ., , , :
,, :",. : . . .,: .
~L12~37 - ~ :
N-n-Decyl-1-~esoxynojirimycin CH20H ~;
~ ~ ~ N-(CH2)9-CH3 '_ ~.0~
HO OH
m.p. 151C (sinters at 91C from ~eOH/acetone) N-n-Undecyl-1 desoxynojirimycin ( CH 7 ) 1 o ~CH 3 E~O ~ ~ , ~, ~0 OH
m.~. 162C (sinters at 91C from ethanol/acetone) ~; :
; N-n-Dodecyl-1-desoxynojirimycin ~-CH20~
~N-(CH2) 1 l--CH3 P
HO~
HO OH ~:
.
m.p. 164C (sinters at 97C from ethanol/acetone) ,3A
, Le A 18 389 - 73-~ 23 4 37 1 !
N-n-T~tradecyl-1-desoxynojlrimycin HO ~ -~CH2)13-CH3 i~
HO OH
-m.p. 105-107C (from methanol) ~-n(5'-Hydroxypentyl)-1 desoxynojirimycin HOC';~
~ W-(CH-) 4-CH.-O'~
XO--~ >
' ..
~o ~o .p. 8~-S7C (from butanol) ~-Cyclohexylmethyl-1-desoxynojirimycin H~CH
,- ~-CH.
HO OH
~';'' m.p. 138-140C (from acetone) Le A 18 389 _ 74- ~
3~
N-(3'-Cyclohexenylmethyl)-1-desoxynojirimycin , ~ -CH2- ~ t HO OH
m.p. 142-i44C (from acetone) ' N-(2'-Norbornen-5'-yl-methyl)-1-desoxynojirimycin HOCH
~ N - CH2 HO ~
- HO OH
,;
m.p. i60-162C (from ethanol) t .
~J-~-C~.lorben~yl-1-d~soxynojirimycin HOCH2 r-~
\- N - CH2 ~ Cl ~0 ~
~ HO OH
m.p. 153-155C (from acetone) Le A 18 389 - 75-.
~-m-Metnylbenzyl-1-desoxynojirimycin - ~-N ~ CHz-~
'rlO--` ~> C~3 HO OH
m.p. 134-136V (from methanol) - N-(p-3iphenylmethyl)-1-desoxynojirimycin ~ - C:~2- ~ `
HO OH
m.p. 240-245C (from water/ethanol) , .
~-(n-3'-phenylpropyl)-1-desoxynojirimycin HOC~ 2 _~ N--CH2--CH2-CH2--<~ ~
HO OH r m.p. 125-127C (from ethanol) Le ~ 18 339 - 76 _ ?
, Ex~mple ~
- . ' N-Allyl-1-desoxynojirimycin CH20H r-C~2-CH=CH~
- HO
EIO. OE~
~.
5 g of 1-desoxynojirimycin, 5 g of Ag20 and 5 g of ~_ allylbromide are stirred in 30 ml of dimethylformamide and 'O ml of water for 3 hours at room temperature~ The silver salts are filtered off and the filtrate is evaporated at the rotary eva~orator. The residue is recrystallized from ethanol.
'.5 g of N-allyl-1-desoxynojirimycin of melting point 131 to 132~C are obtained.
The following products are obtained analogously, tne isolation and purification optionally carried out by chro~to-grap:ny on a s~rongly acidic ion exchange resin (H~-form).
~-Propargyl-1-desoxynojirimycin ~OCH, r ~I-CH2-C-CH
~10--< >
HO OH
m.p. 160C (from acetone) - ' ~ .
Le .~ 1~ 3&9 - 77--.
~12343~
' N-(3',4'-Dichlorbenzyl)-1-desoxynojirimycin ~-CH2 ~Cl HO OEI e~
m.p. 130-132C
N-(p-Nitrobenzyl)-1-desoxynojirimycin r N-C~-2 ~ NO2 E~(! ~
HO OH
..p. 144-146 C
. .
~-~.~-Nitrobenzyl)-l-desoxynojirimycin rOCE~2 ~-CH2 -/~ , ~32 ,.-~iO OP.
m.p. 168-170C
Le .~ l~ 389 _ 78 - _ , ~
.' . j ... .
343~
.
. Exam~le 5 l-Cyano-1-desoxynojirimycin HOCHz S \ NH
HO ~ CN
HO OH
~;~
17.5 g of nojirimycin bisulfite adduct are added to 200 ml of water and 21.2 of Ba(OH)2 8 H20. The mixture is stirred for 1 hour and the solid is filtered off. 12 ml of liquid HCN are added to the filtrate and the mixture is stirred for 30 minutes. The solution is filtered and concen- t trated on the rotary evaporator to 20 ml. 20 ml of methanol are added whereby the crystallization of the product starts.
100 ml of ethanol are added to complete crystallization.
~fter filtration 12.0 g of l-cyano-l-desoxynojirimycin are obtained m.p. 155-156C (from methanol/water).;' ~xa~ple 6 N-h.ethyl-l-cyano-l-desoxynojirimycin I~OCH2 r ~ N-CH3 E~O ~y~crT
HO OH
The compound is obtained from l-cyano-l-descxyno~iri-mycin with 35 ~ strength aqueous formaldehyd solution and ~aC`I~H3 in methanol according to example 3.
Le A 18 389 - 79 -~37 Mass spectrum: The most important peaks in the upper mass `.an~e are at m/e = 17~ (M-CH20H), m/e-157 and m/e = 144.
Example 7 1-Desoxynojirimycin-1-carboxvlic acid \ NH
HO ~ - COOH
~o OH ~k 10 g of 1-cyano-1-desoxynojirimycin are refluxed with ~ g of sodium hydroxide in 100 ml of water for one hour. Hydro-chloric acid is added up to pH 4. The mixture is dried on the rotary evaporator and the residue is extracted with hot methanol, sodiu~ chloride is separated and the methanolic t5 solu_ion is evaporated. The residue is recrystallized from wa~er and water/methanol. 10.5 g of 1-desoxynojiri~ycin-1- r ca-boxy 1 ic acid OI m.p. 268-270C are obtai~ed.
Ex~mpie 8 ,;
1-Desoxynojirimycin-1-carboxylic acid ethyl es.er C ~ 2 t~
~0 ~ ~-COOC2H5 ~:0 OEi 7 ~ of 1-desoxynojirimycin-1- carboxylic ~c~d are re,~l~lYcd with 100 ml of ethanolic hydrochloric acid for 2 hours and evaporated at .he rotary evaporator. The residue is treated Witil ethanol and ethanolic ammonia. The solution was filtered and concentrated. 8 ~ of 1-desoxynojirim~-in-1-ca~oxylic a^id Le A 1~ 389 - 80 -- ~. ;: . - . ~
1~3~37 ethyl ester are obtained. NHR-Spectrum 100 MHz:
triplet at 5 = 1.3 ppm (3H, -COO-CH2-CH3);
multiplet at5 =2.4-2.6 ppm (1 H~ -N-CH CH OH);
multiplet at~ = 3.2-3.5ppm (4 H);
multiplet a_5 =2.6-3.9ppm (2H, ~CH2-OH);
qu~rtet at 6 =4.25 ppm ~2 H, -COO-CH2-CH3).
~xam~le 9 N-~eth~l-1-desoxynojirimycin-1-carboxylic acid eth~lester CH
\ N-CH 3 -.0 ~,~> COOC2 ;~5 ' HO OH
From 1-desoxynojirimycin-1-carboxylic acid ethyl ester according to example 6. r ,~lass spectrum: The most important peaks in the upper mass range are at m/e=218(M-CH20H), m/e= 200, m/e=176, m/e=158 and m/e=126.
Example 10 1-Desoxynojir-mycin-1-carbox~lic acid amide ~OCY.
\r-~'H
HO ~ ~-CO~H
Y~O, OY~
6 g of 1-ciesoxynojirimycin-1-carboxylic acid ethyl ester are refluxed in 90 ml of 25 % strength aqueous a~monia for one hour. After cooling to room-temp-rature the solution --is treated with ethanol and the precipitate (ammonium salt of 1-desoxynojirimycin-1-carboxylic acid) is separated off. Tne Le ~ 13 389 _ 81 -~L2343~7 ~'.
filtrate is concentrated, treated with water and chromato-graphed ~ith a column filled with a strongly basic ion exchange resin (OH -form). The product is eluted with water. The fractions containing the carbonamide are collected and ~ ~ concentrated. The residue is recrystallized from ethanol and 3 g of 1-desoxynojirimycin-1-carboxylic acid amide, m.p.
175-176C, are obtained.
Exam~le 11 ~~
1-Desoxynojirimycin-1-carboxylic acid benzvlamide \--NH
HO~ CO--NH--CH2--~ r HO OH
1~ - 500 mg of 1-desoxynojirimycin-1-carboxylic acid ethyl ester are refIuxed for 5 minutes in 1 ml of benzvlamine. The mixture after cooling is treated several times with ether and the solvent decanted off. The residue is recrystallized fro~ methanol and ~OO mg of 1-desoxynojirimycin-1-carboxylic ZO acid benzYlamide, m.p. 221-222C are obtained.
Exam~le 12 N-Methyl-1-desoxynojirimvcin-1-carboxylic benzyl amide HO--~--CO--~H-CH,-@) HO OH
From 1-desoxvnojirimycin-1-carboxylic acid benzvlamide accor-Le A 18 389 - 82 -~L~3~3~
ding to example 6; m.p. 229-230C (from methanol).
Exz~ple 13 1-Amino~ethyl-1-desoxynojirimycin - r- NH
E~O ~?--CH2--~H2 HO OH
5 g of 1-cyano-1-desoxynojirimycin are hydrogenated in 100 ml of water with 10 g of Raney-Nickel and a ~ressure of 3.5 bar hydrogen. The catalyst is filtered of~ and the solution is dried on the rotary evaporator. The residue is treated with some hot methanol, filtered and evaporated.
The residue is recrystallized from methanol to yield 3.4 g of 1-aminomethyl-1-desoxynojirimycin, m.p. 154-155C.
Exa~,?le 14 1-Acetamidomethyl-1-desoxynojirimycin ;~
\r NH
HO ~ -CH2-NH-C-CH3 ~0 0~1 L
3.S g of 1-aminomethyl-1-desoxynojirimycin in 40 ml methanol/water (1:1) are treated at 0C with 3 ml of acetic acid anhydride and stirred for 15 minutes at 0C and 30 minutes ~.
at roo~ temperature. The solution was evaporated. The residue s treated with 60 ml of water and neutralized with a basic ion exchange resin (OH -form). After removal of the resin Le A 18 389 - 83 -:. : .
:: ,: .. .. . :
lZ3;g~37 the solution is dried and recrystallized twice from ethanol.
3 g~of 1-acetamidomethyl-1-desoxynojirimycin are obtained, ~-?- 169-171C.
, Example 15 - . . _ -~lethyl-1-acetamidomethYl-1-desoxynojirim~cin CHl OEi' _C;~ L
~O~ CH2-~-H-CO-CH
~ iO C~
tO
the compound is prepared from 1-acetamido-methyl-1-desoxy-no~ir~mycin ~nalogously to example 6. i~
~lass spectrum: the most important peaks.in the upper mass range are at m/e = 176 and.m/e = 158. '-l; ~x~m~le 16 ~ . ~
l-Ber.zoylaminomethyl-l-desoxynojir~mycin ~ ~H
HO ~ >-CHz-N-~-CO-?O HO OH
i~
the compound is prepared ~rom 1-aminomethyl-1-desoxynojirimycin and ben~oylchloride according to example 14; m.p. 216C (~rom methanol).
Exam.ple 17 N-Metnyl~ benzoylamino-1-desoxynojirimycin ~ N-C~, ~ ~ _ ~>-CH2-NH-co-~
HO OH
Le A 18 38.9 - 84'-:
, . . .
~Z3~3'7 .
the~compound is prepared from 1-benzoylamino-1-desoxynojiri-` mycin according to example 6; m.p. 135-136C (Lrom butanol).
E~am~le 18 1-Tosylaminomethyl-l-desoxy:nojirimycin \_ NH
H0 - ~ ~ C~2-NH-s02 ~ CH3 _ 960 mg of 1-aminomethyl-1-desoxynojirimycin are refluxed -~ith 1 g of tosylchloride in 10 ml of methanol/water (1:1) ~or 3 hours. The solvent was distilled off in vacuo and .he residue treated with acetone. The solid is filtered off, dissolved in water and neutralized with a basic ion-excnange resin. After removal of the resin tne soluiion is evaporated and residue recrystallized from water. 600 mg 1-tosylaminomethyi-1-desoxyno; rimycin of m.p. 173-175C are obtained.
Exa~le 19 ~-~la ~hyl-1-tosylaminomethyl-1-desoxynojirimycin ;~
HOC~2 \- 2l-CH3 H0 ~ -CH2-NH-S0. ~ ~ CH3 - H~ OH
the compound is prepared from ~he compound of example 18 ac^ording to exam le 6; m.p. 218-~19C (from water).
Le .~ 18 389 _ 85 ~
~Z3~37 Example 20 ~ Phenylureidomethyl)-l-desoxynojirimyCin = . _ .
HOCH~
HO ~ 2 NH -- lCI - Nl~l HO OH
960 mg of l-aminc~ethyl-l-desc~lojirimycin are stirred for 15 minutes with 0,8 ml of phenylisocyanate in 10 ml methanol~water (1:1) at -20C. The mixture is slc~ly warmed to roam temperature and the solvent is distilled off. The residue is discharged onto a column filled with cellulose and the product is eluted with butanol/water (9:1). me fractions containing the prcduct are collected and concentrated. me residue is recrystallized from ethanol and 400 mg of m.p. 161 - 162C are c)btained.
Example 21 N-(l-Desoxynojirimycinyl)-aoetic acid-6-lactone.
.
HO OH
~} OH
5 g of N-(l-desoxynojirimycinyl)-aoetic acid are refluxed in 50 ml of dimethylformamide for 30 minutes. me solvent is rem~ved in high vacuo and the remaining oil crystallized from ethanol. 3.5 g of the cc~pound of m.p. 157 - 159& are obtained.
~."
- r ' - - . .. :, ~ Z3437 Example 22 N-(l-DesQxynojirimycinyl)-acetic acid benzylamide UO ~ - U2 ~ ~ ~ C~l2 HO OH
500 mg of the co~,pound of exampLe 21 are refluxed with 1 ml of benzylanine in 20 ml of dimethylformamide for 6 hours. me solvent is re-moved in high vacuo and the residue recrysta]Llized from ethano V a oe tone (1:2).
400 mg of m.p. 129C are obtained.
N-(l-Desoxynojirimycinyl)-acetic acid n-butylamide is prepared ~n~logously.
Mass spectrum: m e most important peaks in the upper mass range are: m/e =
245, m/e = 203, m/e = 176, m/e = 159 and m/e = 145.
Example 23
filtrate is concentrated, treated with water and chromato-graphed ~ith a column filled with a strongly basic ion exchange resin (OH -form). The product is eluted with water. The fractions containing the carbonamide are collected and ~ ~ concentrated. The residue is recrystallized from ethanol and 3 g of 1-desoxynojirimycin-1-carboxylic acid amide, m.p.
175-176C, are obtained.
Exam~le 11 ~~
1-Desoxynojirimycin-1-carboxylic acid benzvlamide \--NH
HO~ CO--NH--CH2--~ r HO OH
1~ - 500 mg of 1-desoxynojirimycin-1-carboxylic acid ethyl ester are refIuxed for 5 minutes in 1 ml of benzvlamine. The mixture after cooling is treated several times with ether and the solvent decanted off. The residue is recrystallized fro~ methanol and ~OO mg of 1-desoxynojirimycin-1-carboxylic ZO acid benzYlamide, m.p. 221-222C are obtained.
Exam~le 12 N-Methyl-1-desoxynojirimvcin-1-carboxylic benzyl amide HO--~--CO--~H-CH,-@) HO OH
From 1-desoxvnojirimycin-1-carboxylic acid benzvlamide accor-Le A 18 389 - 82 -~L~3~3~
ding to example 6; m.p. 229-230C (from methanol).
Exz~ple 13 1-Amino~ethyl-1-desoxynojirimycin - r- NH
E~O ~?--CH2--~H2 HO OH
5 g of 1-cyano-1-desoxynojirimycin are hydrogenated in 100 ml of water with 10 g of Raney-Nickel and a ~ressure of 3.5 bar hydrogen. The catalyst is filtered of~ and the solution is dried on the rotary evaporator. The residue is treated with some hot methanol, filtered and evaporated.
The residue is recrystallized from methanol to yield 3.4 g of 1-aminomethyl-1-desoxynojirimycin, m.p. 154-155C.
Exa~,?le 14 1-Acetamidomethyl-1-desoxynojirimycin ;~
\r NH
HO ~ -CH2-NH-C-CH3 ~0 0~1 L
3.S g of 1-aminomethyl-1-desoxynojirimycin in 40 ml methanol/water (1:1) are treated at 0C with 3 ml of acetic acid anhydride and stirred for 15 minutes at 0C and 30 minutes ~.
at roo~ temperature. The solution was evaporated. The residue s treated with 60 ml of water and neutralized with a basic ion exchange resin (OH -form). After removal of the resin Le A 18 389 - 83 -:. : .
:: ,: .. .. . :
lZ3;g~37 the solution is dried and recrystallized twice from ethanol.
3 g~of 1-acetamidomethyl-1-desoxynojirimycin are obtained, ~-?- 169-171C.
, Example 15 - . . _ -~lethyl-1-acetamidomethYl-1-desoxynojirim~cin CHl OEi' _C;~ L
~O~ CH2-~-H-CO-CH
~ iO C~
tO
the compound is prepared from 1-acetamido-methyl-1-desoxy-no~ir~mycin ~nalogously to example 6. i~
~lass spectrum: the most important peaks.in the upper mass range are at m/e = 176 and.m/e = 158. '-l; ~x~m~le 16 ~ . ~
l-Ber.zoylaminomethyl-l-desoxynojir~mycin ~ ~H
HO ~ >-CHz-N-~-CO-?O HO OH
i~
the compound is prepared ~rom 1-aminomethyl-1-desoxynojirimycin and ben~oylchloride according to example 14; m.p. 216C (~rom methanol).
Exam.ple 17 N-Metnyl~ benzoylamino-1-desoxynojirimycin ~ N-C~, ~ ~ _ ~>-CH2-NH-co-~
HO OH
Le A 18 38.9 - 84'-:
, . . .
~Z3~3'7 .
the~compound is prepared from 1-benzoylamino-1-desoxynojiri-` mycin according to example 6; m.p. 135-136C (Lrom butanol).
E~am~le 18 1-Tosylaminomethyl-l-desoxy:nojirimycin \_ NH
H0 - ~ ~ C~2-NH-s02 ~ CH3 _ 960 mg of 1-aminomethyl-1-desoxynojirimycin are refluxed -~ith 1 g of tosylchloride in 10 ml of methanol/water (1:1) ~or 3 hours. The solvent was distilled off in vacuo and .he residue treated with acetone. The solid is filtered off, dissolved in water and neutralized with a basic ion-excnange resin. After removal of the resin tne soluiion is evaporated and residue recrystallized from water. 600 mg 1-tosylaminomethyi-1-desoxyno; rimycin of m.p. 173-175C are obtained.
Exa~le 19 ~-~la ~hyl-1-tosylaminomethyl-1-desoxynojirimycin ;~
HOC~2 \- 2l-CH3 H0 ~ -CH2-NH-S0. ~ ~ CH3 - H~ OH
the compound is prepared from ~he compound of example 18 ac^ording to exam le 6; m.p. 218-~19C (from water).
Le .~ 18 389 _ 85 ~
~Z3~37 Example 20 ~ Phenylureidomethyl)-l-desoxynojirimyCin = . _ .
HOCH~
HO ~ 2 NH -- lCI - Nl~l HO OH
960 mg of l-aminc~ethyl-l-desc~lojirimycin are stirred for 15 minutes with 0,8 ml of phenylisocyanate in 10 ml methanol~water (1:1) at -20C. The mixture is slc~ly warmed to roam temperature and the solvent is distilled off. The residue is discharged onto a column filled with cellulose and the product is eluted with butanol/water (9:1). me fractions containing the prcduct are collected and concentrated. me residue is recrystallized from ethanol and 400 mg of m.p. 161 - 162C are c)btained.
Example 21 N-(l-Desoxynojirimycinyl)-aoetic acid-6-lactone.
.
HO OH
~} OH
5 g of N-(l-desoxynojirimycinyl)-aoetic acid are refluxed in 50 ml of dimethylformamide for 30 minutes. me solvent is rem~ved in high vacuo and the remaining oil crystallized from ethanol. 3.5 g of the cc~pound of m.p. 157 - 159& are obtained.
~."
- r ' - - . .. :, ~ Z3437 Example 22 N-(l-DesQxynojirimycinyl)-acetic acid benzylamide UO ~ - U2 ~ ~ ~ C~l2 HO OH
500 mg of the co~,pound of exampLe 21 are refluxed with 1 ml of benzylanine in 20 ml of dimethylformamide for 6 hours. me solvent is re-moved in high vacuo and the residue recrysta]Llized from ethano V a oe tone (1:2).
400 mg of m.p. 129C are obtained.
N-(l-Desoxynojirimycinyl)-acetic acid n-butylamide is prepared ~n~logously.
Mass spectrum: m e most important peaks in the upper mass range are: m/e =
245, m/e = 203, m/e = 176, m/e = 159 and m/e = 145.
Example 23
7 ~ _ _ _ _ . _ _ _ l-Hydroxymethyl-l-desQxynojirimycin N - H
HO ~ CH2H
HO OH
A suspension of 2.3 g of l-desoxynojirimycin-l-carboxylic acid ethyl ester in 50 mL of abs. tetrahydrofuran (THF) are added to 1.9 g of IiPiLH4 in 50 ml of abs. ~ . m e mixture is stirred for one hour and then refluxed for 5 hours. 20 mL of ethyl a oe tate, 2 mL of water and 4 n~L of 15%
strength XOH are added dropwise. m e precipitate is filtered off and extracted by a water-methanol mixture. m e solvent is distilled off and the residue extracted with methanol. The methanol solution is con oentrated and the residue discharged with water onto a colu~n filled with a strongly acidic ,,~. ;`, : ~
1~3437 ion exchange resin (H~3- form). m e column is eluted first with water and then with 0,25% strength aqueous ammonia. The fractions containing the pro-duct are collected and freed from the solvent. 500 mg of the compound are obtained.
Mass spectrum: m e most important peak in the upper mass range is at m/e 162. Smaller peaks are m/e = 144 and m/e 102.
Example 24 6-O-Benzoyl-l-desoxynojirimycin HO ~
HO OH
3.5 g of pulverized K2C03 and 2.0 g of benzoylchloride are added to 2.1 g of l-desoxynorjirimycin in 40 ml of a oe tone and 15 ml of water. m e mixture is stirred for 3 hours at 40C and for 12 hours at room temperature.
The salts are filtered off and the solvent is removed in vacuo. m e residue is chromatographed on a silica gel column and eluted first with ethylacetate/
methanol (10:4) and then with ethylacetate/methanol/water/ammonia (10:4:0.
5:0.02). Each 10 ml of eluate were obtained separately and fractions 51 to 57 contained the desired product (350 mg of m.p. 160 &).
Example 25 N-(~-Methoxyethyl)-l-desoxynojirimycin HOCH~2 ~ N - CH2 - CH2 - OCH3 ~\ >
HO OH
.~ ' ' : `' ` ;, 1 ~343~
5.2 g of ~-methoxyaoetaldehyd-dimethylaoetal in 15 ml of water and 5 ml of methanol are treated with 0.6 ml of HCl for 48 hours at room tempera-ture and 6 hours at 60C. men 1.6 g of l-desoxynojirimycin and 0.7 g oE
NaCNBH3 are added at room temperature. me mixture is kept for 12 hours at 50 C. m e solvent is removed in vacuo, the residue together with water is discharged onto a column which is filled with a strongly acidic ion exchange resin. me solumn is eluted first with water and then wi~h 2% strength amnonia. me fractions containing the product are collected and conoentrated.
m e residue is chromatographed on a cellulose-column with butanol/water (9:1).
1.2 g of the compound are obtained with a Rf-value: 0.57 (on thin layer chr~natography ready-to-use silica gel 60 plates from Messrs. Merck; running -~
agent: ethyl acetate/methanol/H2O/ 25% strength ammonia 100:60:40:2). For ccmparison Rf-value of l-desoxynojirimycin: 0.3.
Analogously are obtained N-(~-methylmercaptoethyl)-l-desoxy-nojirimycin (MS: Mbst important peaks in the upper mass range are at m/e =
220, m/e = 206 and m/e = 176), N-(~-ethylmercapto-ethyl)-l-desoxynojirimycin (MS: Most importc~nt peaks in the upper mass range are at m/e = 220 and m/e =
176) and N-~ -methoxy)-ethoxyethyl]-l-desoxynojirimycin (MS: Most impor-tant peaks in the upper mass range are at m/e = 234 and m/e = 176.
Example 26 N-n-Nonyl-l-acetaminomethyl-l-desoxynojirimycin .
~2 HO ~ CH2 - NH - CO - CH
HO OH
the ccmpound is obtained from l-acetamino-l-desoxynojirimycin according to example 3.
MS: Most important peaks in the upper mass range are at m/e 329, m/e = 288, m/e = 270 and m/e 258.
.. , ~
~.~,3~37 Example 27 l-n-Nonylamlnomethyl-l-desoxynojirimycin HO - CH
t--NH
HO ~ CH2 - NH - (C~I2)g - CH8 HO OH
1.2 ml of acetic acid, 1.56 ml of nonylaldehyd and 0.7 g of NaCNBH
are added to 1.9 g OL l-amQnomethyl-l-desoxynojiri~ycin in 40 ml methanol at 0C. The mLxture is stirred for 1 hour at o& and 12 hours at rocm tempera-ture. The solvent is distilled off in vacuo and the residue is slurried in water, discharged onto a column filled with a strongly acidic ion exchange resin (~- form~ and eluted first with ethanol/water (1:1), then with 0.3%
strength aqueous ammonia and finally with ethanol/0.6% strength aqueous a ammonia (1:1). me fractions containing the product are collected and con-centrated. 1 g of the compound with Rf-value 0.52 tplate and running agent i as in ex. 25) are obtained.
Exa~ple 28 N-Methylnojirimycin hydrochloride .
(a) Preparation of the starting materials 57 ml of chloroformic acid ethylester dissolved in 360 ml of absolute THF are added dropwise to a solution of 294 g of 3-O-benzyl-6-O-tri-phenylmethyl-1.2-isopropylidene-5-am~no-5-desoxy-~-D-glucofuranose in 800 ml of absolute THF and 83.6 ml of triethylamine at 0C. The mixture is stirred for 2 hours at 20&, filtered to remove precipitated salt and concentrated.
m e product is put into ethyl acetate, twice extracted with water, dried and concentrated. 318.6 g of crude 3-O-benzyl-6-O-triphenylmethyl-1.2-O-iso- -propylidene-5-ethoxycclrbonylamino-5-desoxy-~-D-glucofuranose are obtained as a yellGw oil.
174.7 g of this oil are dissolved in 340 ml of absolute ether and ~' .
3~:~7 added drcpwise illtO a suspension of 39 g LiAlH4 in 690 ml of abs. ether at 10 to 15C. The mixture is refluxed for 5 hours and while cooled with ice treated with 520 ml of ethyl acetate, 40 ml of water and 78.5 15~ strength aqueous KQH. The mixture is filtered to be freed from solids, washed with ether and evaporated in vacuo. 144.2 g of 3-O-benzyl-6-O-triphenylmethyl-1.2-iso-propylidene-5-methylamino-5-desoxy-Y-D-glucofuranose are obtained as a yellcw oil.
This crude product is dissolved in 165 ml of abs. THF and added dropwise at -70 & into a mixture of 24.6 g of metallic sodium in 820 ml liquid ammonia. Further 2.5 g of sodium is added and the mixture is stirred for 2 hours. Still at -70 & 91 g of ammonium chloride is added in portions.
The mixture is allcwed to warm to room temperature within 12 hours. m e sus-pension is stirred into 500 ml of methanol. The solids æ e filtered off and the filtrate is concentrated. m e residue is treated with water/chloroform and the phases æ e separated. m e aqueous phase is concentrated and the crude product is purified by means of a cation exchange resin. After recry-stallization from ethyl a oe tate 14.8 g of 5 methylamino-5-desoxy-1.2-O-iso-propylidene, m.p. 124 - 126 & are abtained.
~b) Prep æ ation of the final product.
A solution of 470 mg of the product obtained according to example 28 (a) in 2 ml of hydrochloric acid is kept at 0C for 16 hours. The mixture is can oe ntrated at 20C in vacuo and twi oe dissolved in water and evaporated in vacuo.
m e amorphous N-methylnojirimycin-hydrochloride shcws a three times stronger effect in the saccharose inhibition test than l-desoxy-nojirimycin.
Example 29 N-Phenyl-l-desoxynojirimycin (a) Prep æ ation of the starting material 20 g of l-~-a oe tyl-2.3-O-isopropylidene-6-p-toluenesulfonyl-~-lr sorbofuranose æ e heated together with 30 ml of aniline for 5 hours to llo&.
,,, ~
After cooling, 200 ml of ethyl acetate are added and the solids are filtered off. me solution is concentrated in vacuo and excess aniline is removed in high vacuo. The residue is purified by chromatography with a cation exchange resin. After recrystallisation from ethyl acetate/petroleum ether 3.0 g of 6-phenylamino-2.3-O-isopropylidene-6-desoxy-~-L-sorbofuranose, m.p. 156&, are obtained.
(b) Preparation of the final product 1.0 g of the product obtained according to example 29 (a) are dis-solved in 4 ml 6 n HCl and kept for 24 hours at o&. men 6 ml water are added and the pH is adjusted to 6-7 with 3 ml triethylamine. 1 g Raney-nickel is added and the product is hydrogenated under a H2-pressure of 3.5 bar. me catalyst is filtered off and the solvent is removed. The product is purified by means of column filled with a Qtion exchange resin. 470 mg of a slightly yellcw oil are obtained.
MS: most important peaks in the upper mass range are at m~e = 239, m/e = 208 and m/e = 148.
Example 30 N-Cyclohexyl-l-descxynojirimycin lMethod A
2 g of l-desoxynojirimycin are dissolved in 40 ml of abs. methanol and 1.8 ml glacial acetic acid and treated first with 5.2 ml cyclohexanone and then with 3.4 g of NaCNBH3. This mixture is refluxed for 96 hours, ~ ~-oooled and concentrated in vacuo. The residue is treated with methanol/water (1:1) and purified by a column filled with a cation exchange resin (H - form).
1.9 g pure product are obtained with a Rf-value of 0.58 (thin layer chromato-graphy 60/F 254 plates of ~Iessrs. ~Ierck, running agent: ethyl acetate/
methanol/water/25% stxength aqueous ammonia 120:70:10:1); for comparison:
Rf-value of l-desoxynojirimycin is 0.13.
Method B
1 g of 6-cyclohexylamino-2.3-O-isopropylidene-6-desoxy-~-L,sorbc-- ~ - .
3~37 furanose (prepared according to example 29 (a)) is kept for 40 hours in a mixture of 6 ml of methanol/6 n HCl (1:1) at 0C, treated with 10 ml of water and 3.0 ml of triethylamine and hydrogenated for 2 hours with 3.5 bar H2 and PtO2 as the catalyst. The catalyst is filtered off, the solution evaporated in vacuo and purified by a column filled with cation exchange resin. 610 mg of the co~pound are obtained, identical with the compound prepared according to method A.
N-Isopropyl-l-desoxynojirimycin (Rf-value = 0.45) is prepared analogDus to method A.
N-(l-Methyldecyl)-l-desoxynojirimycin (mixture of diastereomers, Rf-value 0.79 and 0.86) is prepared analogous to method A.
Example 31 1.6-Didesoxynojirimycin (a) 5-Azido-3-O-benzyl-5.6-didesoxy-1.2-O-isopropylidene-~-D-glucofuranose 3 ~ ~ CH
~0 ":~
t 3 186 g of 3-O-benzyl-6-desoxy-1.2-O-isopropylidene-5-O-methylsulfonyl-~-L
idofuranose, 500 ml of dimethylsulfoxide and 65 of NaN3 are heated 5 hours under nitrogen at 120 - 125 &. After cooling the mixture is poured into ice- -water, extracted three times with petroleum ether, the organic phase washed with water, dried and evaporated. 156 g of crude product is obtained as an oil. 1 H-NMR(100 Mhz, C6D6): ~ = 7.15 (m, 5H), 5-72 (d, J = 4Hz, lH), 1.32 (s, 3H), 1.17 (d, J = 6Hz, 3H), 1.06 ppm (s, 3H).
(b) 5-Amino-3-O-benzyl-5.6-didesoxy-1.2-O-isopropylidene-~-D-glucofuranose .
~23~3~
2 ~ ~ ~H2 `llo ~, ~
t 3 C~3 100 g of the crude product of example 31 (a) in 200 ml of anhydrous THF are added dropwise to 6 g of LiAlH4 in 250 ml of anhydrous T~F. me mix-ture is stirred for 15 hours and refluxed for 1 hour. While cooling 6 ml of water and 18 ml of 15% strength aqueous XOH are added dropwise. me mixture is stirred for further 15 hours, the precipitate is filtered off and the solvent is removed. I~.e residue is treated with 500 ml of ether and twice ex*racted with 100 ml of 2 n HCl. me aqueous phase is rendered alkaline by means of 45% strength aqueous NaOH and extracted three times with 200 ml ether. After drying the organic phase the solvent is distilled off and ~;
62.5 g of the compound are obtained as a yellow oilO lH-NMR (100 MHz, CDC13): ~ = 7.3 (m, 5H), 5.8 (d, J = 4Hz, lH), 5.70 (d, J = 12Hz, 14), ~ ;~
5.58 (d, J = 4Hz, lH), 5.42 (d, J = 12Hz, 14), 3.98 (d, J = 4Hz, lH), 1.45 (s, 3H), 1.30 (s, 3H) 1.15 ppm (d, J = 6Hz, 3H). -(c) 5-AmLno-5.6-didesoxy-1.2-O-isopropylidene-~-D-glucofuranose ~' ;' CIH3 i ~ O
~0 ,'` ' '~;`
t 3 ~
3 ; ~;
50 g of the compound obtained according to example 31 (b) are hydrogenated in 1 1 m~thanol in the pres nce of 10 g of Pd on charcoal (5%
. , ~ .
. ~,,".
.
~I~LZ;3437 strength) at 60C for 5 hours with a pressure of 70 bar hydrogen. me catalyst is filtered off and the solvent removed in vacuo. 25.7 g of ~e com-pound are obtained.
lH-NMR (100 MHz, ccmpound disso]ved in CDC13 and extracted with D2O): ~ = 5.97 (d, J = 4Hz, lH), 4.50 (d, J = 4Hz, lH), 4.34 (d, J = 4Hz, lH), 1.49 (s, 3H), 1.32 (s, 3H), 1.28 ppm (d, J = 6Hz, 3H).
(d) 5-Amino-5.6-didesoxy-D-glueose-l-sulfonie acid HO CH H
~ N - ~H
HO ~ so3~3 HO OH
10 g of the compound obt~-ned according to e.~ample 31 (c) are suspended in 50 ml of water.
Sulfurdioxide is passed in for 15 hours. A clear solution originates which is war~ed up to 60C. After about 4 hours the co~pound starts to crystallize. 100 ml of methanol are added and the precipitated produet is filtered off after 15 hours. 8.5 g of the compound are obtained, m.p. 180C (dec.) (e) 1.6-Didesoxynojirimycin 10 g of the com~ound of example 31 (d) are hydrogenated in 120 ml of water in the presen oe of 13.3 g of Ba (OH)2 .8 H2O and 10 g of Raney-Nickel for approximately 7 hours. The solids are filtered off and the sol-vent removed in vacuo. me remaining oil crystallizes after a short time andthe compound is reerystallized from methanol to yield 5.3 g with m.p. 163 -164C.
Example 32 N-(l-Desoxyglueityl)-l-desox~nojirimycin ~ -.~ .
' ' ` ' . ' ~lZ3437 OH OH OH
)--N CH2 - CH - CH - CH - CH - CH2CH
OH
OH
0.8 g of l-deso~ynojirimycin, 7.2 g of glucose, 40 ml of methanol, 10 ml of water, 1.5 ml glacial acetic acid and 1.3 g NaCNBH3 are stirred to-gether for 15 hours at rocm temperature. men the mixture is refluxed for 6 hours, evaporated, treated with 10 ml 2 n HCl, warmed up to 40& until the generating of hydrogen ceases, discharged onto a column filled with an acidific ion exchange resin and washed with water. The pmduct is eluted with 0.3 n am~onia, the solvent distillea off in vacuo and the residue chromatographed on 100 g of silica gel (70-230 mesh) with methano Vconc.
amnonia (10:5). 1 g of the compound is obtained.
Mass spectrum: m/e = 296 (20%), 278 (15%) 176 (100%), 158 (30%), 132 (30%).
Example 33 ~`
l-Desc~y-6-O-methylnojirimycin ., ,~
a) 3-O-Benzyl-1.2-O-isopropylidene-6-O-methyl-~-L-idofuranose ;
, 2 3 2 ~ ~ -OtCH3 440 g of 5.6-anhydrc-:3-0-benzyl-1.2-0-isopropylidene-~-L-idofuranose are refluxed in 1.5 1 of methanol with 92 g of sodium methylate for 1 hour. After cooling the mixture i9 neutralized with glacial acetic acid, methanol is dis-tilled off, the residue is discharged on to 300 ml of water and extracted - 96 - `
~3~ 3~
with chloroform. After drying and evaporating 388 g of an oil are obtained.
b) 3-o-senzyl-1.2-o-isopropylidene-6-O-methyl-5-o-methylsulfonyl-~-Lr idofuranose 384 g of the product of example 33 a) in 300 ml of pyridine and 760 ml of chloroform are treated dropwise with 148 ml of m~esylchloride at o&, and the mLxture is stirred for 15 hours at room temperature. 200 ml of ice-water are added. The mixture is stirred for 20 minutes and extracted three times with 200 ml of chloroform. me organic phase is washed twice with deluted hydro-chloric acid, with water and with 10% strength NaHCO3-solution and dried.
m e solvent is removed in vacuo and the residue recrystallized from ethyl-aoetate to yield 347 g to which further 26 g obtained from the mother liquors by filtratian over 200 g of silica gel are added. 79% of theory;
m.p. 133&~
c) 5-Azido-3-O-benzyl-5-desoxy-1.2-O-isopro~ylidene-6-O-methyl-~-D-gluco-furanose t 2 3 N3 ~ CH
~0 : ' o t CH3 201 g of the pr~duct of example 33 b), 500 ml of hexamethylphosphoric acid triamide and 65 g of sodium azide are heated for 15 hours to 100 to 110C
under a nitrogen current. After cooling the mixture is poured on to ice-water, extracted four times with ethylether, the ethyl ether phases washedwith diluted hydrochloric acid, water and NaHCO3-solution, dried and evapor-ated in vacuo. 159 g (91% of theory) are obtained as an oil.
d) 5-Amino-3-O-benzyl-5-desaxy-1.2-O-isopropylidene-6-O-methyl-l-D-gluco-furanose . - ' . '~
. ..
~,.".- , .
134.5 g of the product of example 33 c) in 200 ml anhydrous l~ are added dropwise to 7.3 g of LiAlH4 Ln 500 ml of anhydrous THF at room temperature.
The mixture is stirred for 4 hours and kept over night. men 7.3 ml of water are added dropwise, 22 ml 15% strength KOH are added and the mixture is stirred for 8 hours. me precipitate is filtered off, washed with T~ and the filtrate is evaporated in vacuo.
me obtaIned oil is covered with a layer of 300 ml of ethylether and treated under cooling at 0 - 10C with 150 ml of 5 N hydrochloric acid.
The organic phase is separated and washed with hydrochloric acid. m e aqueous phases are washed with ethyl ether. The aqueous phase is treated with 100 ml of 40% strength NaOH and extracted three times with 150 ml of ethyl ether. The collected ethyl ether extracts are dried and the solvent is removed in vacuo. 92 g (74% of theory) are obtained as an oil.
e) 5-Amino-5-desoxy-1.2-O-isopropylidene-6-O-methyl-D-glucofuranose ; ,-' O ~.
o t CH3 `~ ~
85 g of the product of example 33 d) in 500 ml of anhydrous THF are added at ~`~
-70C to 1.5 1 of liquid ammonia. 30.5 g of sodium in small pieces are added.
After 4 hours the mixture is treated with a total of 106 g of NH4Cl in 20 portions and kept over night whereby the ammonia evaporates. me residue is treated with methanol, the precipitate filtered of and the solvent removed in varuo. m e residue is treated with ethyl ether~hydrochloric acid, the ether phase extracted three times with a total of 300 ml of diluted hydrcchloric acid and the hydrochloric acid phases collected, treated with 200 ml of con-centrated NaOH and extracted three times with a total of 600 ml of chloroform.
' , . - . :
~;~3~3~
The solution is dried and the solvent removed. me residue is recrystallized from ethyl acetate to yield 47 g (77% of theory) of the product; m.p. 95 -96C.
f) 5-Amino-5-deso~y-6-O-methyl-D-glucose-l-sulfonic acid OH
I ~ OH
H3C - O - CH2 - CH - CH - CH - CH - CH ~ SO3 ~ H3 OH OH
10 g of the product of exa~ple 33 e) are ~issolved in 50 ml of water. S02 is introd~ced for 2 hours at room temperature and for 15 hours at 60C. The slurry is treated with methanol, kept for one day, filtered off ana dried.
11.8 g (99% of theory) are obtained; m.p~ 154C (dec.) g) 1-~esoxy-6-O-methylnojirimycin CH20CH3 .
; ,", H
~OH >
;. HO ~
OH
11 g of the product of exa~ple 33 f) in 90 ml of water are treated with 13.3 g of Ba(OH)2 8 H20. 3 g of Raney-nickel are added and the mixture is hydrogenated for 10 hours. The mixture is filtered and the solvent is re-mDved in vacuo. The residue is treated with 30 ml of 2 N hydrochloric acid, discharged onto a column filled with an acidic ion exchange resin and washed with water. m e product is eluted with 0.3 N ammonia and obtained after evaporating in vacuo. After recrystallization from ethanol 5.5 g (78~ of ~ ~
theory) of m.p. 145 to 146 C are obtained. ~ -_ 99 _ ' ~
HO ~ CH2H
HO OH
A suspension of 2.3 g of l-desoxynojirimycin-l-carboxylic acid ethyl ester in 50 mL of abs. tetrahydrofuran (THF) are added to 1.9 g of IiPiLH4 in 50 ml of abs. ~ . m e mixture is stirred for one hour and then refluxed for 5 hours. 20 mL of ethyl a oe tate, 2 mL of water and 4 n~L of 15%
strength XOH are added dropwise. m e precipitate is filtered off and extracted by a water-methanol mixture. m e solvent is distilled off and the residue extracted with methanol. The methanol solution is con oentrated and the residue discharged with water onto a colu~n filled with a strongly acidic ,,~. ;`, : ~
1~3437 ion exchange resin (H~3- form). m e column is eluted first with water and then with 0,25% strength aqueous ammonia. The fractions containing the pro-duct are collected and freed from the solvent. 500 mg of the compound are obtained.
Mass spectrum: m e most important peak in the upper mass range is at m/e 162. Smaller peaks are m/e = 144 and m/e 102.
Example 24 6-O-Benzoyl-l-desoxynojirimycin HO ~
HO OH
3.5 g of pulverized K2C03 and 2.0 g of benzoylchloride are added to 2.1 g of l-desoxynorjirimycin in 40 ml of a oe tone and 15 ml of water. m e mixture is stirred for 3 hours at 40C and for 12 hours at room temperature.
The salts are filtered off and the solvent is removed in vacuo. m e residue is chromatographed on a silica gel column and eluted first with ethylacetate/
methanol (10:4) and then with ethylacetate/methanol/water/ammonia (10:4:0.
5:0.02). Each 10 ml of eluate were obtained separately and fractions 51 to 57 contained the desired product (350 mg of m.p. 160 &).
Example 25 N-(~-Methoxyethyl)-l-desoxynojirimycin HOCH~2 ~ N - CH2 - CH2 - OCH3 ~\ >
HO OH
.~ ' ' : `' ` ;, 1 ~343~
5.2 g of ~-methoxyaoetaldehyd-dimethylaoetal in 15 ml of water and 5 ml of methanol are treated with 0.6 ml of HCl for 48 hours at room tempera-ture and 6 hours at 60C. men 1.6 g of l-desoxynojirimycin and 0.7 g oE
NaCNBH3 are added at room temperature. me mixture is kept for 12 hours at 50 C. m e solvent is removed in vacuo, the residue together with water is discharged onto a column which is filled with a strongly acidic ion exchange resin. me solumn is eluted first with water and then wi~h 2% strength amnonia. me fractions containing the product are collected and conoentrated.
m e residue is chromatographed on a cellulose-column with butanol/water (9:1).
1.2 g of the compound are obtained with a Rf-value: 0.57 (on thin layer chr~natography ready-to-use silica gel 60 plates from Messrs. Merck; running -~
agent: ethyl acetate/methanol/H2O/ 25% strength ammonia 100:60:40:2). For ccmparison Rf-value of l-desoxynojirimycin: 0.3.
Analogously are obtained N-(~-methylmercaptoethyl)-l-desoxy-nojirimycin (MS: Mbst important peaks in the upper mass range are at m/e =
220, m/e = 206 and m/e = 176), N-(~-ethylmercapto-ethyl)-l-desoxynojirimycin (MS: Most importc~nt peaks in the upper mass range are at m/e = 220 and m/e =
176) and N-~ -methoxy)-ethoxyethyl]-l-desoxynojirimycin (MS: Most impor-tant peaks in the upper mass range are at m/e = 234 and m/e = 176.
Example 26 N-n-Nonyl-l-acetaminomethyl-l-desoxynojirimycin .
~2 HO ~ CH2 - NH - CO - CH
HO OH
the ccmpound is obtained from l-acetamino-l-desoxynojirimycin according to example 3.
MS: Most important peaks in the upper mass range are at m/e 329, m/e = 288, m/e = 270 and m/e 258.
.. , ~
~.~,3~37 Example 27 l-n-Nonylamlnomethyl-l-desoxynojirimycin HO - CH
t--NH
HO ~ CH2 - NH - (C~I2)g - CH8 HO OH
1.2 ml of acetic acid, 1.56 ml of nonylaldehyd and 0.7 g of NaCNBH
are added to 1.9 g OL l-amQnomethyl-l-desoxynojiri~ycin in 40 ml methanol at 0C. The mLxture is stirred for 1 hour at o& and 12 hours at rocm tempera-ture. The solvent is distilled off in vacuo and the residue is slurried in water, discharged onto a column filled with a strongly acidic ion exchange resin (~- form~ and eluted first with ethanol/water (1:1), then with 0.3%
strength aqueous ammonia and finally with ethanol/0.6% strength aqueous a ammonia (1:1). me fractions containing the product are collected and con-centrated. 1 g of the compound with Rf-value 0.52 tplate and running agent i as in ex. 25) are obtained.
Exa~ple 28 N-Methylnojirimycin hydrochloride .
(a) Preparation of the starting materials 57 ml of chloroformic acid ethylester dissolved in 360 ml of absolute THF are added dropwise to a solution of 294 g of 3-O-benzyl-6-O-tri-phenylmethyl-1.2-isopropylidene-5-am~no-5-desoxy-~-D-glucofuranose in 800 ml of absolute THF and 83.6 ml of triethylamine at 0C. The mixture is stirred for 2 hours at 20&, filtered to remove precipitated salt and concentrated.
m e product is put into ethyl acetate, twice extracted with water, dried and concentrated. 318.6 g of crude 3-O-benzyl-6-O-triphenylmethyl-1.2-O-iso- -propylidene-5-ethoxycclrbonylamino-5-desoxy-~-D-glucofuranose are obtained as a yellGw oil.
174.7 g of this oil are dissolved in 340 ml of absolute ether and ~' .
3~:~7 added drcpwise illtO a suspension of 39 g LiAlH4 in 690 ml of abs. ether at 10 to 15C. The mixture is refluxed for 5 hours and while cooled with ice treated with 520 ml of ethyl acetate, 40 ml of water and 78.5 15~ strength aqueous KQH. The mixture is filtered to be freed from solids, washed with ether and evaporated in vacuo. 144.2 g of 3-O-benzyl-6-O-triphenylmethyl-1.2-iso-propylidene-5-methylamino-5-desoxy-Y-D-glucofuranose are obtained as a yellcw oil.
This crude product is dissolved in 165 ml of abs. THF and added dropwise at -70 & into a mixture of 24.6 g of metallic sodium in 820 ml liquid ammonia. Further 2.5 g of sodium is added and the mixture is stirred for 2 hours. Still at -70 & 91 g of ammonium chloride is added in portions.
The mixture is allcwed to warm to room temperature within 12 hours. m e sus-pension is stirred into 500 ml of methanol. The solids æ e filtered off and the filtrate is concentrated. m e residue is treated with water/chloroform and the phases æ e separated. m e aqueous phase is concentrated and the crude product is purified by means of a cation exchange resin. After recry-stallization from ethyl a oe tate 14.8 g of 5 methylamino-5-desoxy-1.2-O-iso-propylidene, m.p. 124 - 126 & are abtained.
~b) Prep æ ation of the final product.
A solution of 470 mg of the product obtained according to example 28 (a) in 2 ml of hydrochloric acid is kept at 0C for 16 hours. The mixture is can oe ntrated at 20C in vacuo and twi oe dissolved in water and evaporated in vacuo.
m e amorphous N-methylnojirimycin-hydrochloride shcws a three times stronger effect in the saccharose inhibition test than l-desoxy-nojirimycin.
Example 29 N-Phenyl-l-desoxynojirimycin (a) Prep æ ation of the starting material 20 g of l-~-a oe tyl-2.3-O-isopropylidene-6-p-toluenesulfonyl-~-lr sorbofuranose æ e heated together with 30 ml of aniline for 5 hours to llo&.
,,, ~
After cooling, 200 ml of ethyl acetate are added and the solids are filtered off. me solution is concentrated in vacuo and excess aniline is removed in high vacuo. The residue is purified by chromatography with a cation exchange resin. After recrystallisation from ethyl acetate/petroleum ether 3.0 g of 6-phenylamino-2.3-O-isopropylidene-6-desoxy-~-L-sorbofuranose, m.p. 156&, are obtained.
(b) Preparation of the final product 1.0 g of the product obtained according to example 29 (a) are dis-solved in 4 ml 6 n HCl and kept for 24 hours at o&. men 6 ml water are added and the pH is adjusted to 6-7 with 3 ml triethylamine. 1 g Raney-nickel is added and the product is hydrogenated under a H2-pressure of 3.5 bar. me catalyst is filtered off and the solvent is removed. The product is purified by means of column filled with a Qtion exchange resin. 470 mg of a slightly yellcw oil are obtained.
MS: most important peaks in the upper mass range are at m~e = 239, m/e = 208 and m/e = 148.
Example 30 N-Cyclohexyl-l-descxynojirimycin lMethod A
2 g of l-desoxynojirimycin are dissolved in 40 ml of abs. methanol and 1.8 ml glacial acetic acid and treated first with 5.2 ml cyclohexanone and then with 3.4 g of NaCNBH3. This mixture is refluxed for 96 hours, ~ ~-oooled and concentrated in vacuo. The residue is treated with methanol/water (1:1) and purified by a column filled with a cation exchange resin (H - form).
1.9 g pure product are obtained with a Rf-value of 0.58 (thin layer chromato-graphy 60/F 254 plates of ~Iessrs. ~Ierck, running agent: ethyl acetate/
methanol/water/25% stxength aqueous ammonia 120:70:10:1); for comparison:
Rf-value of l-desoxynojirimycin is 0.13.
Method B
1 g of 6-cyclohexylamino-2.3-O-isopropylidene-6-desoxy-~-L,sorbc-- ~ - .
3~37 furanose (prepared according to example 29 (a)) is kept for 40 hours in a mixture of 6 ml of methanol/6 n HCl (1:1) at 0C, treated with 10 ml of water and 3.0 ml of triethylamine and hydrogenated for 2 hours with 3.5 bar H2 and PtO2 as the catalyst. The catalyst is filtered off, the solution evaporated in vacuo and purified by a column filled with cation exchange resin. 610 mg of the co~pound are obtained, identical with the compound prepared according to method A.
N-Isopropyl-l-desoxynojirimycin (Rf-value = 0.45) is prepared analogDus to method A.
N-(l-Methyldecyl)-l-desoxynojirimycin (mixture of diastereomers, Rf-value 0.79 and 0.86) is prepared analogous to method A.
Example 31 1.6-Didesoxynojirimycin (a) 5-Azido-3-O-benzyl-5.6-didesoxy-1.2-O-isopropylidene-~-D-glucofuranose 3 ~ ~ CH
~0 ":~
t 3 186 g of 3-O-benzyl-6-desoxy-1.2-O-isopropylidene-5-O-methylsulfonyl-~-L
idofuranose, 500 ml of dimethylsulfoxide and 65 of NaN3 are heated 5 hours under nitrogen at 120 - 125 &. After cooling the mixture is poured into ice- -water, extracted three times with petroleum ether, the organic phase washed with water, dried and evaporated. 156 g of crude product is obtained as an oil. 1 H-NMR(100 Mhz, C6D6): ~ = 7.15 (m, 5H), 5-72 (d, J = 4Hz, lH), 1.32 (s, 3H), 1.17 (d, J = 6Hz, 3H), 1.06 ppm (s, 3H).
(b) 5-Amino-3-O-benzyl-5.6-didesoxy-1.2-O-isopropylidene-~-D-glucofuranose .
~23~3~
2 ~ ~ ~H2 `llo ~, ~
t 3 C~3 100 g of the crude product of example 31 (a) in 200 ml of anhydrous THF are added dropwise to 6 g of LiAlH4 in 250 ml of anhydrous T~F. me mix-ture is stirred for 15 hours and refluxed for 1 hour. While cooling 6 ml of water and 18 ml of 15% strength aqueous XOH are added dropwise. me mixture is stirred for further 15 hours, the precipitate is filtered off and the solvent is removed. I~.e residue is treated with 500 ml of ether and twice ex*racted with 100 ml of 2 n HCl. me aqueous phase is rendered alkaline by means of 45% strength aqueous NaOH and extracted three times with 200 ml ether. After drying the organic phase the solvent is distilled off and ~;
62.5 g of the compound are obtained as a yellow oilO lH-NMR (100 MHz, CDC13): ~ = 7.3 (m, 5H), 5.8 (d, J = 4Hz, lH), 5.70 (d, J = 12Hz, 14), ~ ;~
5.58 (d, J = 4Hz, lH), 5.42 (d, J = 12Hz, 14), 3.98 (d, J = 4Hz, lH), 1.45 (s, 3H), 1.30 (s, 3H) 1.15 ppm (d, J = 6Hz, 3H). -(c) 5-AmLno-5.6-didesoxy-1.2-O-isopropylidene-~-D-glucofuranose ~' ;' CIH3 i ~ O
~0 ,'` ' '~;`
t 3 ~
3 ; ~;
50 g of the compound obtained according to example 31 (b) are hydrogenated in 1 1 m~thanol in the pres nce of 10 g of Pd on charcoal (5%
. , ~ .
. ~,,".
.
~I~LZ;3437 strength) at 60C for 5 hours with a pressure of 70 bar hydrogen. me catalyst is filtered off and the solvent removed in vacuo. 25.7 g of ~e com-pound are obtained.
lH-NMR (100 MHz, ccmpound disso]ved in CDC13 and extracted with D2O): ~ = 5.97 (d, J = 4Hz, lH), 4.50 (d, J = 4Hz, lH), 4.34 (d, J = 4Hz, lH), 1.49 (s, 3H), 1.32 (s, 3H), 1.28 ppm (d, J = 6Hz, 3H).
(d) 5-Amino-5.6-didesoxy-D-glueose-l-sulfonie acid HO CH H
~ N - ~H
HO ~ so3~3 HO OH
10 g of the compound obt~-ned according to e.~ample 31 (c) are suspended in 50 ml of water.
Sulfurdioxide is passed in for 15 hours. A clear solution originates which is war~ed up to 60C. After about 4 hours the co~pound starts to crystallize. 100 ml of methanol are added and the precipitated produet is filtered off after 15 hours. 8.5 g of the compound are obtained, m.p. 180C (dec.) (e) 1.6-Didesoxynojirimycin 10 g of the com~ound of example 31 (d) are hydrogenated in 120 ml of water in the presen oe of 13.3 g of Ba (OH)2 .8 H2O and 10 g of Raney-Nickel for approximately 7 hours. The solids are filtered off and the sol-vent removed in vacuo. me remaining oil crystallizes after a short time andthe compound is reerystallized from methanol to yield 5.3 g with m.p. 163 -164C.
Example 32 N-(l-Desoxyglueityl)-l-desox~nojirimycin ~ -.~ .
' ' ` ' . ' ~lZ3437 OH OH OH
)--N CH2 - CH - CH - CH - CH - CH2CH
OH
OH
0.8 g of l-deso~ynojirimycin, 7.2 g of glucose, 40 ml of methanol, 10 ml of water, 1.5 ml glacial acetic acid and 1.3 g NaCNBH3 are stirred to-gether for 15 hours at rocm temperature. men the mixture is refluxed for 6 hours, evaporated, treated with 10 ml 2 n HCl, warmed up to 40& until the generating of hydrogen ceases, discharged onto a column filled with an acidific ion exchange resin and washed with water. The pmduct is eluted with 0.3 n am~onia, the solvent distillea off in vacuo and the residue chromatographed on 100 g of silica gel (70-230 mesh) with methano Vconc.
amnonia (10:5). 1 g of the compound is obtained.
Mass spectrum: m/e = 296 (20%), 278 (15%) 176 (100%), 158 (30%), 132 (30%).
Example 33 ~`
l-Desc~y-6-O-methylnojirimycin ., ,~
a) 3-O-Benzyl-1.2-O-isopropylidene-6-O-methyl-~-L-idofuranose ;
, 2 3 2 ~ ~ -OtCH3 440 g of 5.6-anhydrc-:3-0-benzyl-1.2-0-isopropylidene-~-L-idofuranose are refluxed in 1.5 1 of methanol with 92 g of sodium methylate for 1 hour. After cooling the mixture i9 neutralized with glacial acetic acid, methanol is dis-tilled off, the residue is discharged on to 300 ml of water and extracted - 96 - `
~3~ 3~
with chloroform. After drying and evaporating 388 g of an oil are obtained.
b) 3-o-senzyl-1.2-o-isopropylidene-6-O-methyl-5-o-methylsulfonyl-~-Lr idofuranose 384 g of the product of example 33 a) in 300 ml of pyridine and 760 ml of chloroform are treated dropwise with 148 ml of m~esylchloride at o&, and the mLxture is stirred for 15 hours at room temperature. 200 ml of ice-water are added. The mixture is stirred for 20 minutes and extracted three times with 200 ml of chloroform. me organic phase is washed twice with deluted hydro-chloric acid, with water and with 10% strength NaHCO3-solution and dried.
m e solvent is removed in vacuo and the residue recrystallized from ethyl-aoetate to yield 347 g to which further 26 g obtained from the mother liquors by filtratian over 200 g of silica gel are added. 79% of theory;
m.p. 133&~
c) 5-Azido-3-O-benzyl-5-desoxy-1.2-O-isopro~ylidene-6-O-methyl-~-D-gluco-furanose t 2 3 N3 ~ CH
~0 : ' o t CH3 201 g of the pr~duct of example 33 b), 500 ml of hexamethylphosphoric acid triamide and 65 g of sodium azide are heated for 15 hours to 100 to 110C
under a nitrogen current. After cooling the mixture is poured on to ice-water, extracted four times with ethylether, the ethyl ether phases washedwith diluted hydrochloric acid, water and NaHCO3-solution, dried and evapor-ated in vacuo. 159 g (91% of theory) are obtained as an oil.
d) 5-Amino-3-O-benzyl-5-desaxy-1.2-O-isopropylidene-6-O-methyl-l-D-gluco-furanose . - ' . '~
. ..
~,.".- , .
134.5 g of the product of example 33 c) in 200 ml anhydrous l~ are added dropwise to 7.3 g of LiAlH4 Ln 500 ml of anhydrous THF at room temperature.
The mixture is stirred for 4 hours and kept over night. men 7.3 ml of water are added dropwise, 22 ml 15% strength KOH are added and the mixture is stirred for 8 hours. me precipitate is filtered off, washed with T~ and the filtrate is evaporated in vacuo.
me obtaIned oil is covered with a layer of 300 ml of ethylether and treated under cooling at 0 - 10C with 150 ml of 5 N hydrochloric acid.
The organic phase is separated and washed with hydrochloric acid. m e aqueous phases are washed with ethyl ether. The aqueous phase is treated with 100 ml of 40% strength NaOH and extracted three times with 150 ml of ethyl ether. The collected ethyl ether extracts are dried and the solvent is removed in vacuo. 92 g (74% of theory) are obtained as an oil.
e) 5-Amino-5-desoxy-1.2-O-isopropylidene-6-O-methyl-D-glucofuranose ; ,-' O ~.
o t CH3 `~ ~
85 g of the product of example 33 d) in 500 ml of anhydrous THF are added at ~`~
-70C to 1.5 1 of liquid ammonia. 30.5 g of sodium in small pieces are added.
After 4 hours the mixture is treated with a total of 106 g of NH4Cl in 20 portions and kept over night whereby the ammonia evaporates. me residue is treated with methanol, the precipitate filtered of and the solvent removed in varuo. m e residue is treated with ethyl ether~hydrochloric acid, the ether phase extracted three times with a total of 300 ml of diluted hydrcchloric acid and the hydrochloric acid phases collected, treated with 200 ml of con-centrated NaOH and extracted three times with a total of 600 ml of chloroform.
' , . - . :
~;~3~3~
The solution is dried and the solvent removed. me residue is recrystallized from ethyl acetate to yield 47 g (77% of theory) of the product; m.p. 95 -96C.
f) 5-Amino-5-deso~y-6-O-methyl-D-glucose-l-sulfonic acid OH
I ~ OH
H3C - O - CH2 - CH - CH - CH - CH - CH ~ SO3 ~ H3 OH OH
10 g of the product of exa~ple 33 e) are ~issolved in 50 ml of water. S02 is introd~ced for 2 hours at room temperature and for 15 hours at 60C. The slurry is treated with methanol, kept for one day, filtered off ana dried.
11.8 g (99% of theory) are obtained; m.p~ 154C (dec.) g) 1-~esoxy-6-O-methylnojirimycin CH20CH3 .
; ,", H
~OH >
;. HO ~
OH
11 g of the product of exa~ple 33 f) in 90 ml of water are treated with 13.3 g of Ba(OH)2 8 H20. 3 g of Raney-nickel are added and the mixture is hydrogenated for 10 hours. The mixture is filtered and the solvent is re-mDved in vacuo. The residue is treated with 30 ml of 2 N hydrochloric acid, discharged onto a column filled with an acidic ion exchange resin and washed with water. m e product is eluted with 0.3 N ammonia and obtained after evaporating in vacuo. After recrystallization from ethanol 5.5 g (78~ of ~ ~
theory) of m.p. 145 to 146 C are obtained. ~ -_ 99 _ ' ~
Claims (44)
PROPERTY OR PRIVILEGE IS CLAIMED ARE DEFINED AS FOLLOWS:
1. A process for preparing a compound which is a 3,4,5-trihydroxypiperidine of the following general formula I
in which R1 and R3 are the same or different and each is H or alkyl having from 1 to 30 C atoms, alkenyl or alkinyl having from 2 to 18 C atoms, a monocyclic, bicyclic or tricyclic radical having from 3 to 10 C atoms, which is saturated, mono-unsaturated or di-unsaturated, aryl having 6 or 10 C atoms, or a heterocyclic radical having from 3 to 8 ring members which contains 1, 2, 3 or 4 heteroatoms and to which a benzene ring or a further said heterocyclic radical can be fused, each of the above groups being optionally substituted by from 1 to 5 substituents selected from the group consisting of hydroxyl; alkoxy having from 1 to 4 carbon atoms; acyloxy, the acyl radical being derived from i) an aliphatic carboxylic acid having from 1 to 7 atoms or ii) an aromatic carboxylic acid which optionally may be substituted in the aromatic moiety by OH, halogen, nitro and/or amino or iii) a heterocyclic carboxylic acid whose heterocyclic radical is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally being substituted in the heterocyclic moiety by C1 to C4-alkyl, chlorine, bromine or amino;
amino, mono- or dialkyl amino with 1 to 4 C-atoms in the alkyl radicals, monoacylamino, the acyl moiety being derived from i) an aliphatic C1 to C7-carboxylic acid or ii) an aromatic carboxylic acid optionally being substituted by OH, halogen, C1 to C4-alkyl, C1 to C4-alkoxy, nitro and/or amino or iii) a heterocyclic carboxylic acid optionally being substituted by C1 to C4-alkyl, chlorine, bromine or amino; mercapto or alkylthio having from 1 to 4 carbon atoms; halogen; alkylcarbonyl having from 1 to 4 carbon atoms in the alkyl moiety; carboxyl; nitro;
cyano; an aldehyde group or a sulphonic acid group; a heterocyclic radical which is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally substituted in the heterocyclic moiety by C1 to C4 alkyl, chlorine, bromine or amino; a heterocyclic radical which is derived from a hexose or pentose, which is bonded to the alkyl moiety directly via a ring atom or via an -O-, -S- or -NH- bridge; naphthyl or phenyl, optionally having from 1 to 3, identical or different substituents each of which is -OH, -NH2, C1 to C4-alkyl-NH-, C1 to C4-dialkyl-N-, C1 to C4-alkoxy, -NO2, -CN, -COOH, -COO-alkyl (C1 to C4), C1 to C6-alkyl, halogen, C1 to C4-alkylthio, -SH, C1 to C4-alkylsulphonyl, -SO3H, -SO2-NH2 and -SO2-NH-alkyl (C1 to C4); a monocyclic, bicyclic or tricyclic aliphatic substituent having from 3 to 10 carbon atoms, which in turn can be substituted by hydroxyl, amino, halogen or -COOH, and R2 is -H, -OH, -OR', -SH, -SR', -NH2, -NHR', , NH2CH2-, NHR'-CH2-. NR'R"-CH2-, -COOH, -COOR', HO-CH2-, R'CO-NHCH2-, R'CO-NR"CH2-, R'SO2NHCH2-, R'SO2 -NR"CH2-,, ,, -SO3H, -CN, -CONH2, -CONHR' or -CONR'R", wherein R'- and R" are the same or different and each has any of the meanings given above for R1, provided that when R3 is -CH2OH and R2 is H or OH; R3 is H and R2 is H, OH, SO3H, -CN or CH2-NH2; or R3 is -CH2-NH2 and R2 is OH, then R1 is other than hydrogen, or a pharmaceutically acceptable salt thereof which process comprises:
(a) subjecting to acid hydrolysis a compound of formula II or IIa II IIa wherein R1 and R3 are as defined above, to remove the isopropyl-idene or cyclohexylidene group to obtain a compound in which R2 is OH;
(b) reacting a compound of formula II or IIa above with trifluoroacetic anhydride to produce a compound of formula III
or IIIa III IIIa wherein R4 is trifluoroacetyl and R5 is trifluoroacetyl or hydrogen, subjecting the compound of formula III or IIIa to acid hydrolysis to remove the isopropylidene or cyclohexylidene group and obtain a compound of formula IV
IV
and subsequently removing the trifluoroacetyl compound in a neutral or alkaline medium to obtain the compound of formula I
in which R2 is OH;
(c) reducing an amide of formula VII
VII
or a derivative thereof in which hydroxyl groups are protected, in which R3 is as defined above and R8 plus a -CH2- radical form R1, or a compound of formula VIII
VIII
or a derivative thereof in which hydroxyl groups are protected, to the corresponding amine with an amide reducing agent, (d) reacting a compound of formula V
V
with a reactive alkylating agent of formula IX
wherein R1 is as defined above and Z is an easily eliminated leaving group, (e) reacting a compound of formula V
V
with a carbonyl compound of formula VI
VI
in the presence of a hydrogen donor reducing agent, whereby R6, R7, the carbon atom to which they are attached and a hydrogen atom form R1, as defined above, in the obtained compound of formula I, (f) to obtain a compound in which R3 is a methyl group, reacting a compound of formula I in which R3 is -CH2OH with p-toluenesulphonic acid to form the corresponding p-toluene-sulphonic ester and subjecting the ester to reduction to obtain the compound in which R3 is a methyl group, (g) to obtain a compound in which R3 is an aminomethyl group, reacting a compound of formula I in which R3 is -CH2OH
with p-toluenesulphonic acid to form the corresponding p-toluenesulphonic ester, converting the ester group to a -CH2-N3 group and subjecting the compound to reduction to obtain the compound of formula I in which R3 is a -CH2NH2 group, (h) reacting a compound of formula I in which R3 is -CH2NH2 with an aldehyde or ketone in the presence of a hydrogen donor, with a carboxylic acid chloride or a sulphonic acid chloride, with a chlorocarbonic acid ester, isocyanate, isothiocyanate or alkyl halide, (i) hydrolyzing a compound of formula XXI
XXI
with strong mineral acid at a pH of 1 or less at a temperature between -20 and +20°C and then hydrogenating the hydrolyzed product at a pH of 4 to 6 with H2/Raney nickel, H2/Pt O2 or sodium borohydride;
and, if required, converting a product of formula I into a pharmaceutically acceptable salt.
in which R1 and R3 are the same or different and each is H or alkyl having from 1 to 30 C atoms, alkenyl or alkinyl having from 2 to 18 C atoms, a monocyclic, bicyclic or tricyclic radical having from 3 to 10 C atoms, which is saturated, mono-unsaturated or di-unsaturated, aryl having 6 or 10 C atoms, or a heterocyclic radical having from 3 to 8 ring members which contains 1, 2, 3 or 4 heteroatoms and to which a benzene ring or a further said heterocyclic radical can be fused, each of the above groups being optionally substituted by from 1 to 5 substituents selected from the group consisting of hydroxyl; alkoxy having from 1 to 4 carbon atoms; acyloxy, the acyl radical being derived from i) an aliphatic carboxylic acid having from 1 to 7 atoms or ii) an aromatic carboxylic acid which optionally may be substituted in the aromatic moiety by OH, halogen, nitro and/or amino or iii) a heterocyclic carboxylic acid whose heterocyclic radical is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally being substituted in the heterocyclic moiety by C1 to C4-alkyl, chlorine, bromine or amino;
amino, mono- or dialkyl amino with 1 to 4 C-atoms in the alkyl radicals, monoacylamino, the acyl moiety being derived from i) an aliphatic C1 to C7-carboxylic acid or ii) an aromatic carboxylic acid optionally being substituted by OH, halogen, C1 to C4-alkyl, C1 to C4-alkoxy, nitro and/or amino or iii) a heterocyclic carboxylic acid optionally being substituted by C1 to C4-alkyl, chlorine, bromine or amino; mercapto or alkylthio having from 1 to 4 carbon atoms; halogen; alkylcarbonyl having from 1 to 4 carbon atoms in the alkyl moiety; carboxyl; nitro;
cyano; an aldehyde group or a sulphonic acid group; a heterocyclic radical which is a 5- or 6-membered ring containing 1 to 3 heteroatoms N, O, S and optionally substituted in the heterocyclic moiety by C1 to C4 alkyl, chlorine, bromine or amino; a heterocyclic radical which is derived from a hexose or pentose, which is bonded to the alkyl moiety directly via a ring atom or via an -O-, -S- or -NH- bridge; naphthyl or phenyl, optionally having from 1 to 3, identical or different substituents each of which is -OH, -NH2, C1 to C4-alkyl-NH-, C1 to C4-dialkyl-N-, C1 to C4-alkoxy, -NO2, -CN, -COOH, -COO-alkyl (C1 to C4), C1 to C6-alkyl, halogen, C1 to C4-alkylthio, -SH, C1 to C4-alkylsulphonyl, -SO3H, -SO2-NH2 and -SO2-NH-alkyl (C1 to C4); a monocyclic, bicyclic or tricyclic aliphatic substituent having from 3 to 10 carbon atoms, which in turn can be substituted by hydroxyl, amino, halogen or -COOH, and R2 is -H, -OH, -OR', -SH, -SR', -NH2, -NHR', , NH2CH2-, NHR'-CH2-. NR'R"-CH2-, -COOH, -COOR', HO-CH2-, R'CO-NHCH2-, R'CO-NR"CH2-, R'SO2NHCH2-, R'SO2 -NR"CH2-,, ,, -SO3H, -CN, -CONH2, -CONHR' or -CONR'R", wherein R'- and R" are the same or different and each has any of the meanings given above for R1, provided that when R3 is -CH2OH and R2 is H or OH; R3 is H and R2 is H, OH, SO3H, -CN or CH2-NH2; or R3 is -CH2-NH2 and R2 is OH, then R1 is other than hydrogen, or a pharmaceutically acceptable salt thereof which process comprises:
(a) subjecting to acid hydrolysis a compound of formula II or IIa II IIa wherein R1 and R3 are as defined above, to remove the isopropyl-idene or cyclohexylidene group to obtain a compound in which R2 is OH;
(b) reacting a compound of formula II or IIa above with trifluoroacetic anhydride to produce a compound of formula III
or IIIa III IIIa wherein R4 is trifluoroacetyl and R5 is trifluoroacetyl or hydrogen, subjecting the compound of formula III or IIIa to acid hydrolysis to remove the isopropylidene or cyclohexylidene group and obtain a compound of formula IV
IV
and subsequently removing the trifluoroacetyl compound in a neutral or alkaline medium to obtain the compound of formula I
in which R2 is OH;
(c) reducing an amide of formula VII
VII
or a derivative thereof in which hydroxyl groups are protected, in which R3 is as defined above and R8 plus a -CH2- radical form R1, or a compound of formula VIII
VIII
or a derivative thereof in which hydroxyl groups are protected, to the corresponding amine with an amide reducing agent, (d) reacting a compound of formula V
V
with a reactive alkylating agent of formula IX
wherein R1 is as defined above and Z is an easily eliminated leaving group, (e) reacting a compound of formula V
V
with a carbonyl compound of formula VI
VI
in the presence of a hydrogen donor reducing agent, whereby R6, R7, the carbon atom to which they are attached and a hydrogen atom form R1, as defined above, in the obtained compound of formula I, (f) to obtain a compound in which R3 is a methyl group, reacting a compound of formula I in which R3 is -CH2OH with p-toluenesulphonic acid to form the corresponding p-toluene-sulphonic ester and subjecting the ester to reduction to obtain the compound in which R3 is a methyl group, (g) to obtain a compound in which R3 is an aminomethyl group, reacting a compound of formula I in which R3 is -CH2OH
with p-toluenesulphonic acid to form the corresponding p-toluenesulphonic ester, converting the ester group to a -CH2-N3 group and subjecting the compound to reduction to obtain the compound of formula I in which R3 is a -CH2NH2 group, (h) reacting a compound of formula I in which R3 is -CH2NH2 with an aldehyde or ketone in the presence of a hydrogen donor, with a carboxylic acid chloride or a sulphonic acid chloride, with a chlorocarbonic acid ester, isocyanate, isothiocyanate or alkyl halide, (i) hydrolyzing a compound of formula XXI
XXI
with strong mineral acid at a pH of 1 or less at a temperature between -20 and +20°C and then hydrogenating the hydrolyzed product at a pH of 4 to 6 with H2/Raney nickel, H2/Pt O2 or sodium borohydride;
and, if required, converting a product of formula I into a pharmaceutically acceptable salt.
2. A process according to claim 1 wherein process (a) is used and the compound of formula I is isolated as an adduct with sulphurous acid or hydrocyanic acid to obtain a compound in which R2 is SO3H or CN, respectively
3. A process according to claim 2 which comprises the further step of treating a compound in which R2 is SO3H with a base to obtain a compound in which R2 is OH.
4. A process according to claim 3 which comprises the further step of reducing the compound in which R2 is OH with a hydrogen donor reducing agent to obtain a compound in which R2 is H.
5. A process according to claim 2 which comprises the further step of subjecting a compound in which R2 is CN to catalytic hydrogenation to obtain a compound in which R2 is CH2NH2.
6. A process according to claim 5 which comprises subjecting the com-pound in which R2 is CH2NH2 to acylation, alkylation or sulphonylation or to reaction with an isocyanate or an isothiocyanate to obtain a compound in which R2 is R'CONHCH2-, R'CONR"CH2-, NHR'-CH2-, NR'R"CH2- or R'SO2NHCH2-, R'-NH-CO-NH-CH2-, R'-NH-CS-NH-CH2- or R'-O-CO-NH-CH2-, wherein R' and R" are as defined in claim 1.
7. A process according to claim 1 in which R3 is -H, -CH3, -CH2OH, -CH2-NH2, NHR'-CH2-, NR'R"-CH2-, R'CONH-CH2-, R'CO-NR"CH2-, Hal-CH2-, R'O-CH2-, R'COOCH2-, R'SO2O-CH2-, R'SO2NHCH2-, R'SO2-NR"CH2-, R'NH-CO-NH-CH2-, R'NHCS-NH-CH2-, R'O-CO-NH-CH2-, -CN, -COOH, -COOR', -CONH2, -CONHR' or -CONR'R" wherein R' and R" are the same or different and each has any of the meanings given above for R1.
8. A process according to claim 1 in which R2 is -H, -OH, -SO3H, -CN, -CH2NH2, -CH2NH-[C1 to C14-alkyl], -CH2NH-?-[C1 to C14-alkyl], -CH2-NH-SO2-[C1 to C14]-alkyl, -CH2-NH-SO2-phenyl, -CH2-NH-?-phenyl, -CH2-NH-C-NH[C1 to C14-alkyl], -CH2-NH-?-NH-phenyl, -CH2-NH-?-NH[C1 to C14-alkyl], -CH2-NH-?-NH-phenyl, -CH2-NH-?-O-[C1 to C14-alkyl] or -CH2-NH-?-O-phenyl wherein phenyl is unsubstituted or substituted by methyl, ethyl, methoxy, chlorine, bromine or nitro.
9. A process according to claim 8, in which R2 is -H, -SO3H or -CN.
10. A process according to claim 9 in which R2 is -H.
11. A process according to claim 1, in which R3 is -H, -CH2OH, -CH3, -CH2NH2, -CH2-NH-[C1 to C6-alkyl], -CH2NH-CO-[C1 to C6-alkyl] or CH2-O-(C1-C6-alkyl).
12. A process according to claim 1 in which R3 is -CH2OH.
13. A process according to claim 1 in which R2 is hydrogen and R3 is -CH2OH.
14. A process according to claim 1 other than said bioprecursors in which R1 is an optionally substituted straight-chain, branched or cyclic saturated or unsaturated aliphatic hydrocarbon radical or an optionally sub-stituted aromatic or heterocyclic radical and R2 is H, OH, alkoxy, amino, monoalkylamino or dialkylamino, -SO3H or -CN, and R3 is CH2OH.
15. A process according to claim 1 other than said bioprecursors which has the steric formula I
wherein R1, R2 and R3 have the same meaning as defined hereinbefore in claim 1.
wherein R1, R2 and R3 have the same meaning as defined hereinbefore in claim 1.
16. A process according to claim 1 wherein R1 is selected from hydrogen, CH3, C2H5, n C3H7, n C4H9, iso C4H9, n C5H11, n C6H13, C8H17, C9H19, CH2=CH-CH?, CH?C-, CH3OCH2CH2- and CH3SCH2CH2-, R2 is H, OH, -SO3H, -CH2NHSO3C6H4CH3, -CH2NHCOCH3 or -CH2NHCOC6H5 and R3 is -CH2OH.
17. A compound of formula I as defined in claim 1 or a pharmaceutically acceptable salt thereof when prepared by a process according to claim 1 or an obvious chemical equivalent thereof.
18. A process according to claim 1 wherein R1 is n-heptyl, R2 is hydro-gen and R3 is -CH2OH.
19. A process for preparing N-(n-heptyl)-1-desoxynojirimycin which com-prises reacting n-heptaldehyde with 1-desoxynojirimycin in the presence of sodium cyanoborohydride.
20. The compound N-(n-heptyl)-1-desoxynojirimycin when prepared by a process according to claim 18 or an obvious chemical equivalent thereof.
21. A process according to claim 1 wherein R1 is methyl, R2 is hydrogen and R3 is -CH2OH.
22. A process for preparing N-methyl-1-desoxynojirimycin which comprises reacting 1-desoxynojirimycin with formaldehyde in the presence of formic acid.
23. The compound N-methyl-1-desoxynojirimycin when prepared by a process according to claim 22 or an obvious chemical equivalent thereof.
24. A process according to claim 1 wherein R1 is ethyl, R2 is hydrogen and R3 is -CH2OH.
25. A process for preparing N-ethyl-1-desoxynojirimycin which comprises reacting acetaldehyde with 1-desoxynojirimycin in the presence of sodium cyanoborohydride.
26. The compound N-ethyl-1-desoxynojirimycin when prepared by a process according to claim 25 or an obvious chemical equivalent thereof.
27. A process according to claim 1 wherein R1 is benzyl, R2 is hydrogen and R3 is -CH2OH.
28. A process for preparing N-benzyl-1-desoxynojirimycin which comprises reacting benzaldehyde with 1-desoxynojirimycin in the presence of sodium cyanoborohydride.
29. The compound N-benzyl-1-desoxynojirimycin when prepared by a process according to claim 28 or an obvious chemical equivalent thereof.
30. A process according to claim 1 wherein R1 is n-butyl, R2 is hydrogen and R3 is -CH2OH.
31. A process for preparing N-(n-butyl)-1-desoxynojirimycin which com-prises reacting n-butyraldehyde with 1-desoxynojirimycin in the presence of sodium cyanoborohydride.
32. The compound N-(n-butyl)-1-desoxynojirimycin when prepared by a pro-cess according to claim 31 or an obvious chemical equivalent thereof.
33. A process according to claim 1 wherein R1 is .beta.-hydroxy-ethyl, R2 is hydrogen and R3 is -CH2OH.
34. A process for preparing N-(.beta.-hydroxy-ethyl)-1-desoxynojirimycin which comprises reacting .beta.-hydroxy-acetaldehyde with 1-desoxynojirimycin in the presence of sodium cyanoborohydride.
35. The compound N-(.beta.-hydroxy-ethyl)-1-desoxynojirimycin when prepared by a process according to claim 34 or an obvious chemical equivalent thereof.
36. A process according to claim 1 wherein R1 is allyl or crotyl, R2 is hydrogen and R3 is -CH2OH.
37. A process for preparing N-ally-1-desoxynojirimycin which comprises reacting 1-desoxynojirimycin with allyl bromide.
38. The compound N-allyl-1-desoxynojirimycin when prepared by a process according to claim 37 or an obvious chemical equivalent thereof.
39. A process according to claim 1 wherein R1 is phenylpropyl or cinnamyl, R2 is hydrogen and R3 is -CH2OH.
40. A process for preparing N-phenylpropyl-1-desoxynojiri-mycin which comprises reacting 1-desoxynojirimycin with phenylacetaldehyde in the presence of sodium cyanoborohydride.
41. The compound N-phenylpropyl-1-desoxynojirimycin when prepared by a process according to claim 40 or an obvious chemical equivalent thereof.
42. A process according to claim 1 wherein R1 is 2-hydroxyethyl, R2 is hydrogen and R3 is -CH2OH.
43. A process for preparing N-(2-hydroxyethyl)-desoxyno-jirimycin which comprises reacting 1-desoxynojirimycin with .alpha.-hydroxyacetaldehyde in the presence of sodium cyanoborohydride.
44. The compound N-(2-hydroxyethyl)-desoxynojirimycin when prepared by a process according to claim 43 or an obvious chemical equivalent thereof.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| DE19772738717 DE2738717A1 (en) | 1977-08-27 | 1977-08-27 | Tri:hydroxy-piperidine derivs. - useful as glucosidase inhibitors for treating diabetes etc. and as animal feed additives |
| DEP2738717.3 | 1977-08-27 | ||
| DE19772758025 DE2758025A1 (en) | 1977-12-24 | 1977-12-24 | Tri:hydroxy-piperidine derivs. - useful as glucosidase inhibitors for treating diabetes etc. and as animal feed additives |
| DEP2758025.2 | 1977-12-24 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1123437A true CA1123437A (en) | 1982-05-11 |
Family
ID=25772626
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA310,084A Expired CA1123437A (en) | 1977-08-27 | 1978-08-25 | 3,4,5-trihydroxypiperidine compound, their production and their medicinal use |
Country Status (19)
| Country | Link |
|---|---|
| US (2) | US4639436A (en) |
| EP (1) | EP0000947B2 (en) |
| JP (1) | JPS5446786A (en) |
| AT (1) | AT373239B (en) |
| AU (2) | AU3921478A (en) |
| CA (1) | CA1123437A (en) |
| DE (1) | DE2860330D1 (en) |
| DK (1) | DK152753C (en) |
| ES (1) | ES472838A1 (en) |
| FI (1) | FI72715C (en) |
| GR (1) | GR73065B (en) |
| HU (1) | HU182449B (en) |
| IE (1) | IE47070B1 (en) |
| IL (1) | IL55423A (en) |
| IT (1) | IT1111197B (en) |
| LU (1) | LU90211I2 (en) |
| NL (1) | NL960027I2 (en) |
| NO (1) | NO154918C (en) |
| PT (1) | PT68474A (en) |
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| GB2020278B (en) * | 1978-05-03 | 1983-02-23 | Nippon Shinyaku Co Ltd | Moranoline dervitives |
| JPS5943948B2 (en) * | 1978-07-06 | 1984-10-25 | 日本新薬株式会社 | Substituted moranoline derivatives |
| DE2830469A1 (en) * | 1978-07-11 | 1980-01-24 | Bayer Ag | PRODUCTION OF L-DESOXY-NOJIRIMYCIN AND N-SUBSTITUTED DERIVATIVES |
| JPS5943948A (en) * | 1982-09-03 | 1984-03-12 | Toyota Motor Corp | Variable venturi type carburetor |
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1978
- 1978-08-09 NO NO782713A patent/NO154918C/en unknown
- 1978-08-23 US US05/936,280 patent/US4639436A/en not_active Expired - Lifetime
- 1978-08-24 AU AU39214/78A patent/AU3921478A/en active Pending
- 1978-08-24 GR GR57073A patent/GR73065B/el unknown
- 1978-08-24 PT PT68474A patent/PT68474A/en unknown
- 1978-08-24 IL IL55423A patent/IL55423A/en active IP Right Grant
- 1978-08-25 DK DK377678A patent/DK152753C/en not_active IP Right Cessation
- 1978-08-25 AT AT0621778A patent/AT373239B/en not_active IP Right Cessation
- 1978-08-25 IT IT27067/78A patent/IT1111197B/en active
- 1978-08-25 JP JP10297478A patent/JPS5446786A/en active Granted
- 1978-08-25 HU HU78BA3696A patent/HU182449B/en unknown
- 1978-08-25 CA CA310,084A patent/CA1123437A/en not_active Expired
- 1978-08-25 ES ES472838A patent/ES472838A1/en not_active Expired
- 1978-08-25 IE IE1716/78A patent/IE47070B1/en not_active IP Right Cessation
- 1978-08-25 FI FI782607A patent/FI72715C/en not_active IP Right Cessation
- 1978-08-25 EP EP78100750A patent/EP0000947B2/en not_active Expired
- 1978-08-25 DE DE7878100750T patent/DE2860330D1/en not_active Expired
- 1978-08-28 AU AU39304/78A patent/AU520686B2/en not_active Expired
-
1979
- 1979-09-20 US US06/077,507 patent/US4260622A/en not_active Expired - Lifetime
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1996
- 1996-10-21 NL NL960027C patent/NL960027I2/en unknown
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1998
- 1998-02-04 LU LU90211C patent/LU90211I2/en unknown
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| US10202383B2 (en) | 2002-08-21 | 2019-02-12 | Boehringer Ingelheim International Gmbh | 8-[3-amino-piperidin-1-yl]-xanthines, the preparation thereof and their use as pharmaceutical compositions |
| US10023574B2 (en) | 2002-08-21 | 2018-07-17 | Boehringer Ingelheim International Gmbh | 8-[3-amino-piperidin-1-yl]-xanthines, the preparation thereof and their use as pharmaceutical compositions |
| US9751855B2 (en) | 2004-11-05 | 2017-09-05 | Boehringer Ingelheim International Gmbh | Process for the preparation of chiral 8-(3-aminopiperidin-1-yl)-xanthines |
| US11919903B2 (en) | 2006-05-04 | 2024-03-05 | Boehringer Ingelheim International Gmbh | Polymorphs |
| US9815837B2 (en) | 2006-05-04 | 2017-11-14 | Boehringer Ingelheim International Gmbh | Polymorphs |
| US11291668B2 (en) | 2006-05-04 | 2022-04-05 | Boehringer Ingelheim International Gmbh | Uses of DPP IV inhibitors |
| US11084819B2 (en) | 2006-05-04 | 2021-08-10 | Boehringer Ingelheim International Gmbh | Polymorphs |
| US11033552B2 (en) | 2006-05-04 | 2021-06-15 | Boehringer Ingelheim International Gmbh | DPP IV inhibitor formulations |
| US10080754B2 (en) | 2006-05-04 | 2018-09-25 | Boehringer Ingelheim International Gmbh | Uses of DPP IV inhibitors |
| US10301313B2 (en) | 2006-05-04 | 2019-05-28 | Boehringer Ingelheim International Gmbh | Polymorphs |
| US10022379B2 (en) | 2008-04-03 | 2018-07-17 | Boehringer Ingelheim International Gmbh | DPP-IV inhibitor combined with a further antidiabetic agent, tablets comprising such formulations, their use and process for their preparation |
| US10973827B2 (en) | 2008-04-03 | 2021-04-13 | Boehringer Ingelheim International Gmbh | DPP-IV inhibitor combined with a further antidiabetic agent, tablets comprising such formulations, their use and process for their preparation |
| US10034877B2 (en) | 2008-08-06 | 2018-07-31 | Boehringer Ingelheim International Gmbh | Treatment for diabetes in patients inappropriate for metformin therapy |
| US11911388B2 (en) | 2008-10-16 | 2024-02-27 | Boehringer Ingelheim International Gmbh | Treatment for diabetes in patients with insufficient glycemic control despite therapy with an oral or non-oral antidiabetic drug |
| US10092571B2 (en) | 2009-11-27 | 2018-10-09 | Boehringer Ingelheim International Gmbh | Treatment of genotyped diabetic patients with DPP-IV inhibitors such as linagliptin |
| US9603851B2 (en) | 2010-05-05 | 2017-03-28 | Boehringer Ingelheim International Gmbh | Combination therapy |
| US10004747B2 (en) | 2010-05-05 | 2018-06-26 | Boehringer Ingelheim International Gmbh | Combination therapy |
| US11911387B2 (en) | 2010-11-15 | 2024-02-27 | Boehringer Ingelheim International Gmbh | Vasoprotective and cardioprotective antidiabetic therapy |
| US10195203B2 (en) | 2012-05-14 | 2019-02-05 | Boehringr Ingelheim International GmbH | Use of a DPP-4 inhibitor in podocytes related disorders and/or nephrotic syndrome |
| US9713618B2 (en) | 2012-05-24 | 2017-07-25 | Boehringer Ingelheim International Gmbh | Method for modifying food intake and regulating food preference with a DPP-4 inhibitor |
| US10155000B2 (en) | 2016-06-10 | 2018-12-18 | Boehringer Ingelheim International Gmbh | Medical use of pharmaceutical combination or composition |
Also Published As
| Publication number | Publication date |
|---|---|
| EP0000947B1 (en) | 1981-01-14 |
| AU520686B2 (en) | 1982-02-18 |
| DE2860330D1 (en) | 1981-03-12 |
| NO782713L (en) | 1979-02-28 |
| US4260622A (en) | 1981-04-07 |
| FI72715B (en) | 1987-03-31 |
| DK152753B (en) | 1988-05-09 |
| DK152753C (en) | 1988-10-31 |
| LU90211I2 (en) | 1998-04-08 |
| NO154918C (en) | 1987-01-14 |
| US4639436A (en) | 1987-01-27 |
| IE781716L (en) | 1979-02-27 |
| JPS5446786A (en) | 1979-04-12 |
| ATA621778A (en) | 1983-05-15 |
| NO154918B (en) | 1986-10-06 |
| NL960027I2 (en) | 1997-07-01 |
| PT68474A (en) | 1978-09-01 |
| FI782607A (en) | 1979-02-28 |
| AU3921478A (en) | 1980-02-28 |
| AU3930478A (en) | 1980-03-06 |
| IE47070B1 (en) | 1983-12-14 |
| GR73065B (en) | 1984-01-30 |
| IT7827067A0 (en) | 1978-08-25 |
| NL960027I1 (en) | 1997-01-06 |
| DK377678A (en) | 1979-02-28 |
| IT1111197B (en) | 1986-01-13 |
| IL55423A (en) | 1982-09-30 |
| HU182449B (en) | 1984-01-30 |
| IL55423A0 (en) | 1978-10-31 |
| AT373239B (en) | 1983-12-27 |
| EP0000947A1 (en) | 1979-03-07 |
| EP0000947B2 (en) | 1984-10-10 |
| JPS6231703B2 (en) | 1987-07-09 |
| ES472838A1 (en) | 1979-03-16 |
| FI72715C (en) | 1987-07-10 |
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