CA1265445A - Composition for use in treating inflammation - Google Patents
Composition for use in treating inflammationInfo
- Publication number
- CA1265445A CA1265445A CA000514887A CA514887A CA1265445A CA 1265445 A CA1265445 A CA 1265445A CA 000514887 A CA000514887 A CA 000514887A CA 514887 A CA514887 A CA 514887A CA 1265445 A CA1265445 A CA 1265445A
- Authority
- CA
- Canada
- Prior art keywords
- cif
- composition
- tgf
- cartilage
- leu
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired - Lifetime
Links
Classifications
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/435—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- C07K14/475—Growth factors; Growth regulators
- C07K14/495—Transforming growth factor [TGF]
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
- A61K38/16—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- A61K38/17—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- A61K38/18—Growth factors; Growth regulators
- A61K38/1841—Transforming growth factor [TGF]
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/0012—Galenical forms characterised by the site of application
- A61K9/0019—Injectable compositions; Intramuscular, intravenous, arterial, subcutaneous administration; Compositions to be administered through the skin in an invasive manner
- A61K9/0024—Solid, semi-solid or solidifying implants, which are implanted or injected in body tissue
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P29/00—Non-central analgesic, antipyretic or antiinflammatory agents, e.g. antirheumatic agents; Non-steroidal antiinflammatory drugs [NSAID]
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P37/00—Drugs for immunological or allergic disorders
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P7/00—Drugs for disorders of the blood or the extracellular fluid
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/435—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- C07K14/475—Growth factors; Growth regulators
- C07K14/51—Bone morphogenetic factor; Osteogenins; Osteogenic factor; Bone-inducing factor
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/18—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans
- C07K16/22—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from animals or humans against growth factors ; against growth regulators
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S530/00—Chemistry: natural resins or derivatives; peptides or proteins; lignins or reaction products thereof
- Y10S530/827—Proteins from mammals or birds
- Y10S530/84—Bones; tendons; teeth; cartilage
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S930/00—Peptide or protein sequence
- Y10S930/01—Peptide or protein sequence
- Y10S930/12—Growth hormone, growth factor other than t-cell or b-cell growth factor, and growth hormone releasing factor; related peptides
Abstract
A COMPOSITION FOR USE
IN TREATING INFLAMMATION
Abstract Inflammation, acute and/or chronic, is treated with a CIF (TGF-.beta.). The CIF may be administered locally of systemically, depending upon the indication, and does not require coadministration of activator or cofactor for efficacy.
IN TREATING INFLAMMATION
Abstract Inflammation, acute and/or chronic, is treated with a CIF (TGF-.beta.). The CIF may be administered locally of systemically, depending upon the indication, and does not require coadministration of activator or cofactor for efficacy.
Description
A COMPOSITION FOR USE
IN TRE~TING INFL~MMATION
D scrip~
Technical Field Thi6 invention i5 in the field of anti-inflammatory co~pounds. More particularly it relate6 to using polypeptides called cartilage-inducing f~ctors~ -(CIFs) and functionally related polypeptides as factor~
for inhibiting inflammatory processes in~olving lymphohistiocytic in~lamma~ion, granulomatous inflammation, and acu~e inflammation.
BackqrUnd Commonly owned European Patent ~pplication No.
85304848.6, published 22 January 1986 under No. 0169016, describes two bovine bone-derived CIFs, deçignated CIF-~and CIF-B. ~oth have molecular weights of approximately 26,000 daltons by SDS-PAGE and are dimers. They each exhibit in vitro chondrogenic activity by themselves, as measured by cartilage &pecific proteoglycan (PG~
production in an agarose gel culture model using fetal rat mesenchymal cells. ~either, however, is chondrogenically active in vivo by itself. ~mino acid sequencing of the CIF-A showed that it has a partial (30 amino acids) N-te~minal sequence identical to that reported for a human placenta-derived polypeptide called beta-type transforming growth factor (TGF-~). The partial M-terminal sequence of CIF'-B i6 different from that of TGF-~. Both CIFs exhibit activity in the TGF-~assay (ability to induce anchorage-independent growth of normal rat kidney cell colonies in 60ft agar).
~2~
TGF-~ derived from bovine kidney, human placanta, and human platelets is described in In~ernational Patent ~pplication PCT/US83/01460, published ?9 March 1984 under no. W084/01106, and ~.PA
5 8445001S.5, published 19 December 1984 under no.
0128849. These applications present data showing that such TGF-~, when combined with EGF or TGF-, (1) promotes cell proliferation in the above mentioned soft agar culture assay and (2) promotes cell-proli$er~a~ion and protein depo~ition in a rat soft tissue wound healing model. The applications characterize the ~GF-~s as being dimers having a molecular weight of approximately 26,000 daltons by SDS-PAGE.
Disclosure of the Invention The present invention is based on the finding that the two bone-de~ived CIFs described above exhibit anti-inflammatory activity. Evaluations of implants containing CIF indicate that CIF is active both locally and systemically for inhibiting acute and/or chronic inflammation. Based on the similarity (or perhaps identity in the case of CIF-~) of these polypeptides to TGF-~s, it is believed that TGF-~s also have these newly discovered activities. These activities appear to be independent of the presence of activating agents or cofactors and are distinct from the in vitro chondrogenic activity and cell prolifera~ion activity reported previously. For convenience, the term CIF is used in this 6ection and the claims as a generic term to encompass CIF-A, CIF-B, the TGF-~s and functional equivalents thereof.
Subsequent finding~ that CIF is localized at ~ites of- hematopoiesis and lymphopoie~is and inhibits the response of thymocytes to interleukin-l (IL-l) ~2~5~S
indicate that CIF may also be efficacious in treating dysfunction or malfunction of red blood cell and/or lymphocyte development.
Accordingly, the invention provide~ two new S uses for C~F.
One is a composition for u~e in treating inflammation, which composition comprise6 a cartilage-inducing factor. Both acute and chronic forms of inflammation may be so treated. Further the - -treatment may be systemic or CIF may be admini~tered locally to treat predetermined sites of inflammation.
The other is a composition for use in treating a dysfunction or malfunction of hematopoiesis or lymphopoiesis, which composition comprises a cartilage-inducing factor.
Brief Description of the Drawinqs In the drawings:
Figure 1 is the amino acid sequence of platelet-derived human TGF-B monomer.
Figure 2 is a graph of tha optical densities tabSorbances) (280 nm) of the gel filtration fractions of the axample 1 (~C);
Figure 3 is a graph of the optical densities t2~0 nm) of eluate fractions from the preparative ion exchange chromatography of the example 1 (1~D~; and Figure 4 shows graphically the effec~ of CIF-A
(TGP-B) and CIF-B upon the proliferation of murine thymocytes to stimulation of different amounts of recombinant IL-l (rIL-l) (Example 4, infra).
Figure 5 is a graph showing the dose-dependent inhibition of stimulated murine thymocyte proliferation by TGF-~ and CIF-B (Example 4, infra).
5~
Figure 6 i6 a graph showing ths effect of TGF-~and CIF-B upon thymocyte cultures prestimulated with IL-l for di~ferent lengths of time (Example 4, infra).
Figure 7 ~hows graphically the effect of TGF-~and CIF-B pretreatment upon the responsivenes6 ~o IL-l mediated proliferation (Example 4, infra).
Figure 8 is a g~aph of the results of the T
cell prolifera~ion a~says described in Example 5 (ffB).
Modes for CarrYinq Out the Invention As used herein the term "inflammation" i8 intended to encompass both acu~e responses ~i.e., a response in which the inflamma~ory processes are ac~ive~
and chronic re~ponses (i.e., a response marked by 610w progress and formation of new connective tissue).
Chronic and acute inflammation may be distinguished by the cell types involved. Acute inflammation often involves polymorphonuclear neutrophils; whereas chronic inflammation is normally characterized by a lymphohistiocytic and/or granulomatous response.
Examples of specific types of inflammation are dif~use inflammation~ focal inflammation, croupous inflammation, interstitial inflammation, obliterative inflammation, parenchymatous inflammation, reactive inflammation, specific inflammation, toxic inflammation, and traumatic inflammation.
~ s used herein the term "treat" is intended to mean prophylaxis or attenuation of an existing condition. Accordingly, in the case of inflammation, the invention method may be used to prevent inflammation or alleviate existing inflammation.
The term "functional equivalent" as used to describeia polypeptide ifi intended to mean polypeptide~, whether native or synthetic and regardless of ~pecies or , ~s~
derivation, that have ~he same amino acid sequence as the referenced polypeptide, and polypeptide6 of subs~an~ially homologous (i.e., et least 90% identity in amino acid sequence) but dif~erent amino acid ~equence, which difference~6) does not af~ect an~i-inflammatory activity adver~ely.
CIF-~, CIF-B and T~F-~s exhibit act;vity in the TGF-~ assay described in Methods for PreParation of M~dia~ Su~plements, and Subs~rate for Serum-Fre^e Animal -Cell Culture (1984) pp 181-194, Alan R. Liss, Inc. That assay determines ability to induce anchorage-independent growth in non-neoplastic normal rat kidney (NRK) fibroblasts by measuring the formation of cell colonies in so~t agar. Procedures for obtaining TGF-~s from platelets, placenta and kidney tissues are described in International patent publication W08~/01106 and EPA
publication no 01288~9. Briefly, they involve extracting the source material with acid-ethanol, sizing the extract by gel filtration, and isola~ing the TGF-~
from the filtrate by high performance liquidchromatography (HPLC).
A procedure for isolating CIFs from bovine bone is described in European Patent ~pplication No.
85304848.6. It involves extracting demineralized bone (DMB) witb an extractant (e.g., >4M guanidine hydrochloride, 8M urea) that solubilizes nonfibrous proteins, gel filtering the extract to obtain a < 30 Kd fraction, chromatographing the fraction on carboxymethyl cellulose (C~C~ at pH 4.5-5.5, preferably 4.8, eluting the CMC-adsorbed ~rac~ion with an NaCl gradient, and p~rifying the protein6 from the portion eluting at about 150-250 mM NaCl by RP-HPLC or gel electrophoresis.
CIF-A, CIF-B, and the TGF-~s isolated to date from natural sourca6 are polypeptide dimers of ~65~
approximately 2S to 26 Kd molecular weight as determined by SDS-PA~E. Nature (1985) 316:701-705 reports a cDNA
nucleotide sequence and deduced amino acid sequence fo~
platelet-derived human TGF-~. Mature platelet-derived human TGF-~ is characterized ag a homodimer of a 112 amino acid-long monomer.
Platelet/placenta/kidney-derived TGF-~ and CIF-A and CIF-B are non-species specific as regards TGF-B activi~y. It i8 believed, therefore, that tne~e polypeptides have been highly conserved among animal species ~i.e., a given polypeptide from different mammalian species has an amino acid sequence that varies, if at all, in one or more amino acid residue additives, deletions, or substitutions ~hat do not affect the non-species specific activity of the molecule adversely) and have cross-species functionality.
~ccordingly, CIF-~, CIF-B, and the TGF-~s may be derived from cells or tissue of diverse animal origin or may be obtained by recombinant DNA technology. Correlatively, CIF (TGF-R) from one vertebrate species may be used to treat another vertebrate species. The most common usage of CIF (TGF~~) as an anti-inflammatory agent will be in the treatment of humans, domestic animals such as cattle, fiheep, and pigs, and sports or pet animals such as dogs, cats, and horses. CIF-A and CIF-B are preferred for use in the invention method.
ExamPlas The following examples are intended to illustratè specific embodiments of the invention. They are not intended to limit the invention in any manner.
1. Preparation of CIFs from Bone A. PrePara~ion of Demineraliz~d ~one Bo~ine metatarsal bone was obtai~ed ~re~h from.
t~e slaughte~hou~e and ~ransported o~ dry ice. ~he bones were cleaned of marrow and ~on-bone tissue~.
b~oken in fragment6 smaller than 1 cm diamet2r, and pulverized in a mill at 4C. The pulverized bone wa~
washed ~wice wi~h 9,4 liters of double di~ d ~.te~
per kg of ~one foc about 15 min eac~. and then washed overnig~t in 0.~1 N HCl at 4C. ~ashed bone wa~
defatted using 3 ~ 3 ~olume6 ethanol. fsllowea by 3 ~ 3 ~olumes diethylet~er, each washed for 20 min. and all at room temperature. The resulting defatted bone powder was t~en de~ineralized in 0.5 N HCl (25 l/kg defatted bone) at 4C. The acid was decanted and ~he resulting D~ washed until ~he wash pH was greater tha~ 4, and t~e DMB dried on a suction filter.
B. Extraction of Noncollaqenous Proteins Tha DMB as prepared in ~A was extracted wi~h 3.3 1 of 4 ~ guanidine-~Cl, 10 mM
ethylenediaminetetraacetic acid ~DTA), pH 6.8, 1 ~M
PMSF, 10 mM NEM per kg fo~ 16 hr, t~e suspension suction fi}tered and the non-soluble material extracted agai~
for 4 hr. The soluble fractio~s were combined and concentrated at least 5-fold by ultrafiltration using an Amicon*ultra~iltration ~lOK) unit, and the concentrate dialyzed again~t 6 ~hanges of 35 volumes cold deionized water over a period of 4 days, and then lyophilized.
All of the procedures of this ~aragraph ~ere condu~ted at 4C excep~ the lyophilization which was conducted under standard lyophilizatio~ conditions.
(*) Tradema~k . ..
~5~
C. Gel Filtration The extract from 1~B, redi6solved in 4 M
guanidine-HCl, wa~ fractionated on a Sephac~yl S-200 column equilibrated in 4 M guanidine-HC1, 0.02% sodium azide, 10 mM EDTA, pH 6.8. Fractions were as~ayed by ~heir absorbance at 280 nm and the fractions were combined as shown in Figure 2. Fraction F2 of Figure 2, constituting a low molecular weight (LMW, 10,000-30,000 dal~ons~ protein fraction was dialyzed against ~ changes of 180 volumes of deionized water and lyophilized. All operations except lyophilization and dialysifi (4C) were conducted at room temperature.
D. Ion Exchanqe C _ matoqraphY
Fraction F2 from 1~C was dissolved in 6 M urea 10 mM NaCl, 1 ~M NEM, 50 mM sodium acetate, p~ ~.8 and centrifuged at 10,000 rpm for 5 min. The supernatant was fractionated on a CM52 (a commercially available CMC) column e~uilibrated in the same buffer. Bound proteins were eluted from the column using a 10 mM to 400 mM NaCl gradient in the same buffer, and a total volume of 350 ml at a flow rate of 27 ml/hr. Three major fractions, designated CM-l, CM-2 and CM-3, were collected as shown in Figure 3. CM-2 and CM-3 eluted at ~5 approximately 150-250 mM NaCl. Each fraction was dialyzed against 6 changes of 110 volumes of deionized water for 4 days and lyophilized. All of the foregoing operations were conducted at room temperature except dialysis (4C).
E. RP-HPLC
The combined lyophilized fractions CM-2 and CM-3 from UD were each dissolved in 0.1% trifluoroacetic acid (TFA) and aliquots of the solutions loaded onto a :12~5~S
Vydac C18 RP-HPLC columns (~.6 mm ID X 25 cm) and washed with 0.1% TFA for 5 min at 1 ml/min. ~he eluting solven~ was a 0%~60% acetonitrile gradien~ in 0.1% TFA
at a rate of 2~/min.
Two peaks were obtained from the RP-HPLC of combined CM-~ and CM-3--peak A at about 29.5 min and peak ~ at about 31.2 min. The proteins of these peaks are the subject of said U.S. patent application serial no. 630,93B. They are designated CIF-A and CI~-B.-respec~ively~
Tbe proteins were stored in 0.1%
TFA~acetonitrile eluting solution at -20C until u~ed.
F. Characterization of CIF-A and CIF-B
Table 1 below gi~es the partial amino acid compositions of CIF-A and CIF-B.
~L2~i4A~
--10-- _ Table 1 ~mt (mols/100 mols recovered) Amino ~cid CIF-A CIF-B
~sp 9~2 12.0 Glu 9.2 8.5 Ser 7.0 10.6 ~is 2.7 0.9 Gly 16.5 22.0 Thr 2.7 0.0 Arg 5.9 4-~
~la 6.6 6.7 Tyr 3.2 1.9 Met O.o o.o ~al 7.5 2.4 Phe 3.0 3.0 Ile 3.9 2.2 Leu 8.6 8.2 Lys 13.9 17.3 Pro ND ND
Cys ND ND
Trp ND ND
SDS-PAGE analysis of CIF-A and CIF-B indicate that both have a molecular weight of approximately 26,000 daltons. Both proteins exhibited activity in the TGF-B assay refarred to above comparable to that reported for T&F-~s derived from human platelets, human placenta, or bovine kidney.
N-terminal amino acid sequencing of the first 30 amino acids of CIF-A and CIF-B wa~ carried out and found to be as follows:
--ll--CIF-~
Ala-Leu-~se-Thr-Asn-Tyr-Cy6-Phe-Ser-Ser-Thr-Glu-Lys-Asn--Cys-Cys-Val-Arg-Gln-Leu-Tyr-Ile-~sp-Phe Arg-Lys-~sp-Leu-.
~. :
10 -Gly-Trp-, CIF-B
Ala-Leu-Asp-Ala-Ala-Tyr-Cys-Phe-Arg-~sn-Val-Glu-Asp-Asn--(Cys-Cys)-Leu-~rg~Pro-Leu-Tyr-Ile-Asp-Phe-Lys-Arg-Asp---Leu-&ly-Trp-.
The N-terminal amino acid sequence of CIF-A is identical to ~hat reported for pla~elet-derived human TGF-~ (see Nature, in~ra).
IN TRE~TING INFL~MMATION
D scrip~
Technical Field Thi6 invention i5 in the field of anti-inflammatory co~pounds. More particularly it relate6 to using polypeptides called cartilage-inducing f~ctors~ -(CIFs) and functionally related polypeptides as factor~
for inhibiting inflammatory processes in~olving lymphohistiocytic in~lamma~ion, granulomatous inflammation, and acu~e inflammation.
BackqrUnd Commonly owned European Patent ~pplication No.
85304848.6, published 22 January 1986 under No. 0169016, describes two bovine bone-derived CIFs, deçignated CIF-~and CIF-B. ~oth have molecular weights of approximately 26,000 daltons by SDS-PAGE and are dimers. They each exhibit in vitro chondrogenic activity by themselves, as measured by cartilage &pecific proteoglycan (PG~
production in an agarose gel culture model using fetal rat mesenchymal cells. ~either, however, is chondrogenically active in vivo by itself. ~mino acid sequencing of the CIF-A showed that it has a partial (30 amino acids) N-te~minal sequence identical to that reported for a human placenta-derived polypeptide called beta-type transforming growth factor (TGF-~). The partial M-terminal sequence of CIF'-B i6 different from that of TGF-~. Both CIFs exhibit activity in the TGF-~assay (ability to induce anchorage-independent growth of normal rat kidney cell colonies in 60ft agar).
~2~
TGF-~ derived from bovine kidney, human placanta, and human platelets is described in In~ernational Patent ~pplication PCT/US83/01460, published ?9 March 1984 under no. W084/01106, and ~.PA
5 8445001S.5, published 19 December 1984 under no.
0128849. These applications present data showing that such TGF-~, when combined with EGF or TGF-, (1) promotes cell proliferation in the above mentioned soft agar culture assay and (2) promotes cell-proli$er~a~ion and protein depo~ition in a rat soft tissue wound healing model. The applications characterize the ~GF-~s as being dimers having a molecular weight of approximately 26,000 daltons by SDS-PAGE.
Disclosure of the Invention The present invention is based on the finding that the two bone-de~ived CIFs described above exhibit anti-inflammatory activity. Evaluations of implants containing CIF indicate that CIF is active both locally and systemically for inhibiting acute and/or chronic inflammation. Based on the similarity (or perhaps identity in the case of CIF-~) of these polypeptides to TGF-~s, it is believed that TGF-~s also have these newly discovered activities. These activities appear to be independent of the presence of activating agents or cofactors and are distinct from the in vitro chondrogenic activity and cell prolifera~ion activity reported previously. For convenience, the term CIF is used in this 6ection and the claims as a generic term to encompass CIF-A, CIF-B, the TGF-~s and functional equivalents thereof.
Subsequent finding~ that CIF is localized at ~ites of- hematopoiesis and lymphopoie~is and inhibits the response of thymocytes to interleukin-l (IL-l) ~2~5~S
indicate that CIF may also be efficacious in treating dysfunction or malfunction of red blood cell and/or lymphocyte development.
Accordingly, the invention provide~ two new S uses for C~F.
One is a composition for u~e in treating inflammation, which composition comprise6 a cartilage-inducing factor. Both acute and chronic forms of inflammation may be so treated. Further the - -treatment may be systemic or CIF may be admini~tered locally to treat predetermined sites of inflammation.
The other is a composition for use in treating a dysfunction or malfunction of hematopoiesis or lymphopoiesis, which composition comprises a cartilage-inducing factor.
Brief Description of the Drawinqs In the drawings:
Figure 1 is the amino acid sequence of platelet-derived human TGF-B monomer.
Figure 2 is a graph of tha optical densities tabSorbances) (280 nm) of the gel filtration fractions of the axample 1 (~C);
Figure 3 is a graph of the optical densities t2~0 nm) of eluate fractions from the preparative ion exchange chromatography of the example 1 (1~D~; and Figure 4 shows graphically the effec~ of CIF-A
(TGP-B) and CIF-B upon the proliferation of murine thymocytes to stimulation of different amounts of recombinant IL-l (rIL-l) (Example 4, infra).
Figure 5 is a graph showing the dose-dependent inhibition of stimulated murine thymocyte proliferation by TGF-~ and CIF-B (Example 4, infra).
5~
Figure 6 i6 a graph showing ths effect of TGF-~and CIF-B upon thymocyte cultures prestimulated with IL-l for di~ferent lengths of time (Example 4, infra).
Figure 7 ~hows graphically the effect of TGF-~and CIF-B pretreatment upon the responsivenes6 ~o IL-l mediated proliferation (Example 4, infra).
Figure 8 is a g~aph of the results of the T
cell prolifera~ion a~says described in Example 5 (ffB).
Modes for CarrYinq Out the Invention As used herein the term "inflammation" i8 intended to encompass both acu~e responses ~i.e., a response in which the inflamma~ory processes are ac~ive~
and chronic re~ponses (i.e., a response marked by 610w progress and formation of new connective tissue).
Chronic and acute inflammation may be distinguished by the cell types involved. Acute inflammation often involves polymorphonuclear neutrophils; whereas chronic inflammation is normally characterized by a lymphohistiocytic and/or granulomatous response.
Examples of specific types of inflammation are dif~use inflammation~ focal inflammation, croupous inflammation, interstitial inflammation, obliterative inflammation, parenchymatous inflammation, reactive inflammation, specific inflammation, toxic inflammation, and traumatic inflammation.
~ s used herein the term "treat" is intended to mean prophylaxis or attenuation of an existing condition. Accordingly, in the case of inflammation, the invention method may be used to prevent inflammation or alleviate existing inflammation.
The term "functional equivalent" as used to describeia polypeptide ifi intended to mean polypeptide~, whether native or synthetic and regardless of ~pecies or , ~s~
derivation, that have ~he same amino acid sequence as the referenced polypeptide, and polypeptide6 of subs~an~ially homologous (i.e., et least 90% identity in amino acid sequence) but dif~erent amino acid ~equence, which difference~6) does not af~ect an~i-inflammatory activity adver~ely.
CIF-~, CIF-B and T~F-~s exhibit act;vity in the TGF-~ assay described in Methods for PreParation of M~dia~ Su~plements, and Subs~rate for Serum-Fre^e Animal -Cell Culture (1984) pp 181-194, Alan R. Liss, Inc. That assay determines ability to induce anchorage-independent growth in non-neoplastic normal rat kidney (NRK) fibroblasts by measuring the formation of cell colonies in so~t agar. Procedures for obtaining TGF-~s from platelets, placenta and kidney tissues are described in International patent publication W08~/01106 and EPA
publication no 01288~9. Briefly, they involve extracting the source material with acid-ethanol, sizing the extract by gel filtration, and isola~ing the TGF-~
from the filtrate by high performance liquidchromatography (HPLC).
A procedure for isolating CIFs from bovine bone is described in European Patent ~pplication No.
85304848.6. It involves extracting demineralized bone (DMB) witb an extractant (e.g., >4M guanidine hydrochloride, 8M urea) that solubilizes nonfibrous proteins, gel filtering the extract to obtain a < 30 Kd fraction, chromatographing the fraction on carboxymethyl cellulose (C~C~ at pH 4.5-5.5, preferably 4.8, eluting the CMC-adsorbed ~rac~ion with an NaCl gradient, and p~rifying the protein6 from the portion eluting at about 150-250 mM NaCl by RP-HPLC or gel electrophoresis.
CIF-A, CIF-B, and the TGF-~s isolated to date from natural sourca6 are polypeptide dimers of ~65~
approximately 2S to 26 Kd molecular weight as determined by SDS-PA~E. Nature (1985) 316:701-705 reports a cDNA
nucleotide sequence and deduced amino acid sequence fo~
platelet-derived human TGF-~. Mature platelet-derived human TGF-~ is characterized ag a homodimer of a 112 amino acid-long monomer.
Platelet/placenta/kidney-derived TGF-~ and CIF-A and CIF-B are non-species specific as regards TGF-B activi~y. It i8 believed, therefore, that tne~e polypeptides have been highly conserved among animal species ~i.e., a given polypeptide from different mammalian species has an amino acid sequence that varies, if at all, in one or more amino acid residue additives, deletions, or substitutions ~hat do not affect the non-species specific activity of the molecule adversely) and have cross-species functionality.
~ccordingly, CIF-~, CIF-B, and the TGF-~s may be derived from cells or tissue of diverse animal origin or may be obtained by recombinant DNA technology. Correlatively, CIF (TGF-R) from one vertebrate species may be used to treat another vertebrate species. The most common usage of CIF (TGF~~) as an anti-inflammatory agent will be in the treatment of humans, domestic animals such as cattle, fiheep, and pigs, and sports or pet animals such as dogs, cats, and horses. CIF-A and CIF-B are preferred for use in the invention method.
ExamPlas The following examples are intended to illustratè specific embodiments of the invention. They are not intended to limit the invention in any manner.
1. Preparation of CIFs from Bone A. PrePara~ion of Demineraliz~d ~one Bo~ine metatarsal bone was obtai~ed ~re~h from.
t~e slaughte~hou~e and ~ransported o~ dry ice. ~he bones were cleaned of marrow and ~on-bone tissue~.
b~oken in fragment6 smaller than 1 cm diamet2r, and pulverized in a mill at 4C. The pulverized bone wa~
washed ~wice wi~h 9,4 liters of double di~ d ~.te~
per kg of ~one foc about 15 min eac~. and then washed overnig~t in 0.~1 N HCl at 4C. ~ashed bone wa~
defatted using 3 ~ 3 ~olume6 ethanol. fsllowea by 3 ~ 3 ~olumes diethylet~er, each washed for 20 min. and all at room temperature. The resulting defatted bone powder was t~en de~ineralized in 0.5 N HCl (25 l/kg defatted bone) at 4C. The acid was decanted and ~he resulting D~ washed until ~he wash pH was greater tha~ 4, and t~e DMB dried on a suction filter.
B. Extraction of Noncollaqenous Proteins Tha DMB as prepared in ~A was extracted wi~h 3.3 1 of 4 ~ guanidine-~Cl, 10 mM
ethylenediaminetetraacetic acid ~DTA), pH 6.8, 1 ~M
PMSF, 10 mM NEM per kg fo~ 16 hr, t~e suspension suction fi}tered and the non-soluble material extracted agai~
for 4 hr. The soluble fractio~s were combined and concentrated at least 5-fold by ultrafiltration using an Amicon*ultra~iltration ~lOK) unit, and the concentrate dialyzed again~t 6 ~hanges of 35 volumes cold deionized water over a period of 4 days, and then lyophilized.
All of the procedures of this ~aragraph ~ere condu~ted at 4C excep~ the lyophilization which was conducted under standard lyophilizatio~ conditions.
(*) Tradema~k . ..
~5~
C. Gel Filtration The extract from 1~B, redi6solved in 4 M
guanidine-HCl, wa~ fractionated on a Sephac~yl S-200 column equilibrated in 4 M guanidine-HC1, 0.02% sodium azide, 10 mM EDTA, pH 6.8. Fractions were as~ayed by ~heir absorbance at 280 nm and the fractions were combined as shown in Figure 2. Fraction F2 of Figure 2, constituting a low molecular weight (LMW, 10,000-30,000 dal~ons~ protein fraction was dialyzed against ~ changes of 180 volumes of deionized water and lyophilized. All operations except lyophilization and dialysifi (4C) were conducted at room temperature.
D. Ion Exchanqe C _ matoqraphY
Fraction F2 from 1~C was dissolved in 6 M urea 10 mM NaCl, 1 ~M NEM, 50 mM sodium acetate, p~ ~.8 and centrifuged at 10,000 rpm for 5 min. The supernatant was fractionated on a CM52 (a commercially available CMC) column e~uilibrated in the same buffer. Bound proteins were eluted from the column using a 10 mM to 400 mM NaCl gradient in the same buffer, and a total volume of 350 ml at a flow rate of 27 ml/hr. Three major fractions, designated CM-l, CM-2 and CM-3, were collected as shown in Figure 3. CM-2 and CM-3 eluted at ~5 approximately 150-250 mM NaCl. Each fraction was dialyzed against 6 changes of 110 volumes of deionized water for 4 days and lyophilized. All of the foregoing operations were conducted at room temperature except dialysis (4C).
E. RP-HPLC
The combined lyophilized fractions CM-2 and CM-3 from UD were each dissolved in 0.1% trifluoroacetic acid (TFA) and aliquots of the solutions loaded onto a :12~5~S
Vydac C18 RP-HPLC columns (~.6 mm ID X 25 cm) and washed with 0.1% TFA for 5 min at 1 ml/min. ~he eluting solven~ was a 0%~60% acetonitrile gradien~ in 0.1% TFA
at a rate of 2~/min.
Two peaks were obtained from the RP-HPLC of combined CM-~ and CM-3--peak A at about 29.5 min and peak ~ at about 31.2 min. The proteins of these peaks are the subject of said U.S. patent application serial no. 630,93B. They are designated CIF-A and CI~-B.-respec~ively~
Tbe proteins were stored in 0.1%
TFA~acetonitrile eluting solution at -20C until u~ed.
F. Characterization of CIF-A and CIF-B
Table 1 below gi~es the partial amino acid compositions of CIF-A and CIF-B.
~L2~i4A~
--10-- _ Table 1 ~mt (mols/100 mols recovered) Amino ~cid CIF-A CIF-B
~sp 9~2 12.0 Glu 9.2 8.5 Ser 7.0 10.6 ~is 2.7 0.9 Gly 16.5 22.0 Thr 2.7 0.0 Arg 5.9 4-~
~la 6.6 6.7 Tyr 3.2 1.9 Met O.o o.o ~al 7.5 2.4 Phe 3.0 3.0 Ile 3.9 2.2 Leu 8.6 8.2 Lys 13.9 17.3 Pro ND ND
Cys ND ND
Trp ND ND
SDS-PAGE analysis of CIF-A and CIF-B indicate that both have a molecular weight of approximately 26,000 daltons. Both proteins exhibited activity in the TGF-B assay refarred to above comparable to that reported for T&F-~s derived from human platelets, human placenta, or bovine kidney.
N-terminal amino acid sequencing of the first 30 amino acids of CIF-A and CIF-B wa~ carried out and found to be as follows:
--ll--CIF-~
Ala-Leu-~se-Thr-Asn-Tyr-Cy6-Phe-Ser-Ser-Thr-Glu-Lys-Asn--Cys-Cys-Val-Arg-Gln-Leu-Tyr-Ile-~sp-Phe Arg-Lys-~sp-Leu-.
~. :
10 -Gly-Trp-, CIF-B
Ala-Leu-Asp-Ala-Ala-Tyr-Cys-Phe-Arg-~sn-Val-Glu-Asp-Asn--(Cys-Cys)-Leu-~rg~Pro-Leu-Tyr-Ile-Asp-Phe-Lys-Arg-Asp---Leu-&ly-Trp-.
The N-terminal amino acid sequence of CIF-A is identical to ~hat reported for pla~elet-derived human TGF-~ (see Nature, in~ra).
2. ~nti-InflammatorY ~cti _tY of CIFs A. Formulation of CIF-~/CIF-B-Containinq ImPlants A collagenous carrier was prepared by mixing collagen in solution (CIS, 1-3mg ~rotein/ml; sold by Collagen Corporation under the trademark VITROGEN
lOQ~) wi-t.h bone collagen powder (BCP, lyophilized solids from bone collagen) to give a minimal final ~26S~as5 concentr~tion of 10% collagen from CIS. A 2:1 weight ratio mixture of CIF-A and CIF-B (in 0.1% TFA) was added to carrier in weig~t ratios of 1:1200, 1:4500, 1:6000.
1:8000, and 1:2Q000. The formulations were stirred for 1-2 hr at 4C and either directly lyophilized or dialyzed agains~ water and lyophilized. Carrier alone was used as a comparative control.
B. Histoloqical Evaluation of ImPlant Formula~ionE o-f 1. ImPlantation The lyophilized formulations were rehydrated with two paLts by weight of cold sterile water and mixed to form a homogeneous paste. The rehydrated material was formed into compact pellets (80-100 mg wet weight).
The pellets were implanted subcutaneously in the ventral thoracic region of young male rats. Each rat received bilateral implan~s. The explants were recovered at 3, 10, and 14 days post implantation and evaluated histologically 2. Histoloqical Evaluation Explants were fixed in 10% neutral f ormalin and paraffin embedded by routine method6. Sections were subsequently stained with either hematoxylin-eosin or with Gomori trichome.
lOQ~) wi-t.h bone collagen powder (BCP, lyophilized solids from bone collagen) to give a minimal final ~26S~as5 concentr~tion of 10% collagen from CIS. A 2:1 weight ratio mixture of CIF-A and CIF-B (in 0.1% TFA) was added to carrier in weig~t ratios of 1:1200, 1:4500, 1:6000.
1:8000, and 1:2Q000. The formulations were stirred for 1-2 hr at 4C and either directly lyophilized or dialyzed agains~ water and lyophilized. Carrier alone was used as a comparative control.
B. Histoloqical Evaluation of ImPlant Formula~ionE o-f 1. ImPlantation The lyophilized formulations were rehydrated with two paLts by weight of cold sterile water and mixed to form a homogeneous paste. The rehydrated material was formed into compact pellets (80-100 mg wet weight).
The pellets were implanted subcutaneously in the ventral thoracic region of young male rats. Each rat received bilateral implan~s. The explants were recovered at 3, 10, and 14 days post implantation and evaluated histologically 2. Histoloqical Evaluation Explants were fixed in 10% neutral f ormalin and paraffin embedded by routine method6. Sections were subsequently stained with either hematoxylin-eosin or with Gomori trichome.
3. Results The results of the histological evaluations are summarized below.
3-Days Post Implantation 1. Carrier alone At three days post implantation, the implant was, for the mo6t part, acellular. Sparse neutrophils were the most apparent cell type.
2. CIF-Carrier The implant was also relatively acellular at three days. However, t~her~ was -an apparent act.ivation of fibroblasts from adjacentmuficle and the surLounding subcutaneous tissues. These fibroblasts contained abundant cytoplasm and were, Eor the most part, euchromatic suggesting the ce~ls were highly activated. Fibroblast infiltration was beginning at the margins of the implant.
10-Days Post Implantation 1 Carcier alone The inflammatory profile was .
markedly changed by 10 days following implantation. The implant con~ained a diffuse mixed inflammatory cell infiltrate dominated by lymphocy~es and histiocytes.
Focal areas of granulocytes (neutrophils and eosinophils) and giant cells were evident around some of 2~ the bone collagen particles.
2. CIF-Carrier There were few inflammatory cells a~sociated with the implant at this time poin~
Numerous hyperplastic fibroblasts were present throughout the implant. A collagenous connec~ive tissue matrix was evident around and 6urrounding the bone collagen powder pacticles.
-i5~
l~-Days Post Implantation 1. Carrier alone By 14-days post implantation, most bone collagen particles were sequestered by granulomas consis~ing of lymphocy~es, histiocytes and giant cells. Implant-aszociated fibrosis was evident as well as multifocal areas of eosinophils.
2. CIF-C_ rier Implant-associated inflammation was negligible compared with the control implants. A dense collagenous connective tissue matrix was e~ident throughout the implant. Morphologically, the fibrobla6~s appeared to be me~abolically less active than at earlie~ time points.
These histological obse~vations demonstrate that CIF inhibits inflammatory cell function in vivo.
The lack of polymorphonuclear neutrophils, lymphocytes, and histiocytes at the CIF-containing implant si~es suggests that CIF may function as a potent anti-inflammatory agent.
In the implants having CIF to carrier weight ratios of 1:8000 and 1:20000 there was a maLked reduction in implant-associated inflammation compared with carrier alone implants. The implan~s containing higher CIF to cacrier weight ratios developed a dense eollagenous eonneetive tissue matrix throughout the implant. ~t all CIF levels, implant-associated inflammation was negligible compared to no CIF.
In similar in vivo studies in which the rats reeeived bilateral implan~s with and without CIF-containing extracts, it was noted that inflamma~ion was redueed or absent in the implant ~emote from the CIF-containing implant. The6e ob6ervations indicate that CIF acts ~ystemically as well as locally.
When u~ed a6 a local an~i-inflammatory agent the CIF (and/or TGF-~) will usually be formula~ed in effective amount6 wi~h pharmaceutically acceptable carriers in weight ratios to carrier in the range of 1:1000 ~o 1:20000. If ti~sue deposition at the site i~
not desired, the level of CIF to carrier may be lowered to below that (e.g., a~ weight ratios ~elow abQ~t~ 6000-in the case of collagen carrier) which promote~ ~issuedeposition. In addition to being formulated as an in3ectable, the CIF may be incorporated (dispersed) into solid peLmeable implants such as collagenous soft and hard tissue implants, prostheses, sponges, wound dressings and sutures to modulate local inflammatory responses to such solid bodies. Since such implants are made from permeable materials the CIF can diffuse from the implant and exert its anti-inflammatory properties.
If it is de~ired to minimize other activities of CIF
lcell proliferation, tissue deposition) the CIF will be incorporated free of activating agents or coactor, ~referably at level6 below that which promote tissue deposition.
When used ~o treat inflammation at internal body sites locally, the CIF- or TGF-~-containing formulation is injected, inhaled, placed surgically, or otherwi~e administered locally, depending on the particular formulation, and the site where inflammation control is desired.
For systemic administration CIF may be formulated with conventional carriers used with water-soluble proteins for injection into circulation.
Alternat;vèly, it may be formulated as a sustairled ~2~ 5 release implant formulation if the indication being treated requires.
The amount o~ CIF (TGF-~) administered to treat inflammation will depend upon the pa~ient, ~he in~lammatory condition being treated, and the mode of administration. In general, the amounts administered to adul~ humans will be in the range of about 0.1 to 1000 ~g. When CIF i8 administered locally, amounts in the lower por~ion oE this range will normally-be us*d~ -typically 0.1 to 10 ~g. Correspondingly, sy~temic administra~ion will typically involve amounts in the 10-1000 ~g range.
CIF may be particularly effective in the treatment of inflammation involving the respiratory system. In this application, the CIFs may be administered by inhala~ion with a suitable aerosol. In this form, these factors would be useful for the treatment of diffuse interstitial diseases of the lung such as asbestosis, silicosis, or coal~miner's pneumoconiosis; the treatment of immunological diseases that involve the respiratory tract such as rheumatoid arthritis, lupus erythematosus, or GoodpastuLe's syndrome; and the treatment of granulomatous inflammation of the lungs and pulmonary tract ~uch as Wegener's granulomatosus and eosinophilic granulomatosus.
These anti-inflammatory peptides may be combined with carriers in the form of a salve, ointment, or other topical formulation and thereby by useful in the control of dermal inflammation by topical application. Such formulation~ would be particularly useful in the local treatment of p~oriasis vulgaris, contact dermatitis, dermal ulcers, and acute or chronic eczematous dermatitis.
~ ~S'~4~;
-17- , _ CIF may be either used alone or combined with a slow release carrier and injec~ed into or around joints.
bone, or muscle for the con~rol of in1ammatio~
associated with various diseases. Some examples include myositis (viral, bacterial, parasitic, fungal o~
autoimmune pcocesses) myasthenia gravis: osteomyelitis:
osteoarthritis and rheumatoid arthritis.
Since ~he CIF molecules have been shown ~o be stable at low pH and resistent to enzyme digest~ion, ~- -~hese factors may be delivered systemically byingestion. These properties make these factors particularly useful for controlling inflammation in the gas~rointes~inal tract. This would be particularly useful for the treatment of gastric and duodenal ulcers, granulomatous gastritis, esophagitis (numerous causes):
enteristis (numerous causes) and colitis (numerous causes).
3. Immunohistochemical Localization of CIF-~ (TGF-~) 2~
Materials and Methods . Synthetic Polv~ep~ide SYnthesi~
~ synthetic polypeptide, referred to as Al/30, was constructed to be identical to the N-terminal amino acid sequence (residues 1-30) of CIF-A and TGF-~. The peptide Al/30 was synthesized by a solid-phase method.
The peptide was assembled on p-me~hylbenzhydrylamine resin, cleaved from the resin, deprotected via a 2-step hydrogen fluoride procedure, and purified by reverse-phase liquid chromatography on octadeaylsilica.
Peptide Al/30 was determined to be homogeneous by RP-HPLC and thin layer chromatography and the amino acid sequence was verified by gas-phase se~uence analysis.
5~
B. Radioiodination Purified CIF-~ and CIF-B were radioiodinated with Na I using a lactoperoxidase method. The specific activity was 0.8 to 1.0 x 107 cpm/~g protein.
C. Immunization A New Zealand white rabbit was immunized wi~h peptide ~1/30 at multiple intramuscular sites biweekly for 6-10 weeks using 250 to 500 ~g of peptide ~1/30 per injec~ion. The primary immunization was in Freund' 6 compleie adjuvant and the subsequent boosts were in Freund`s incomplete adjuvant. Ten days following the final boos~, the rabbit was bled by cardiac puncture.
The blood was clot~ed at 22C for 4 hr and overnight at 4C, and the serum was collected and stored at -70C.
D. ~ntibody Purification Serum IgG was purified using Sepharose protein-A. Briefly, serum was diluted with an equal volume of 0.01 M Tris (pH 7.2) con~aining 0.15 M NaCl.
Antibodies were precipitated with an equal volume of saturated ammonium sulfate adjusted to pH 8.0 (4C) and collected by centrifugation at 100,000 x g (30 min).
The protein pellet was resuspended in a minimal volume of pH 7.2 PBS and dialyzed against PBS. The retentate was clarified by centrifugation and the supernatant applied to a 10 ml column of Sepharose protein-~. Bound IgG was eluted with 0.1 M glycine-HCl (pH 2.0). The antibodies were immediately neutralized (4.0 M Tri~), dialyzed against PBS, and lyophilized.
~L2~5~
E. ~nzyme-Linked Immuno~orbent ~s~ay (EkIS~) ~ ntiserum ~as evaluated for reactivi~y with pept;de A1~30, CIF-~, or the low ~olecular weigh~ bone extract by an ELISA. Peptide Al/30 was solubilized in PBS, while purified CIF-A or t~e partially purified bone ~xtracts were solubilized in 0.01 ~ HCl. ~ntige~6 ~ere diluted in 0.01 M carbonate bufer ~pH 9.63 and 400 ng of p~o~ein in 100 ~1 volume were added to ~he well6 of a ~icrotitar ~late. Peptides ~1/30 and ~IF-A ~ere~
dried onto ~e wells overnight. Pla~e~ con~aining the partially purified e~ract were ~ealed and ~tored overnight at 4C. Prio~ to u6e. nonspecific protein binding to the ~LISA pla~e was blocked by incubating with PBS containing 1~ (w/v) BSA for 1 hr. Anti~erum wa8 6e~ially twoold diluted and 100 ~1 ~ere added to each well for 1 hr. The plates ~er0 was~ed wi~h PBS
containing 0.05% (v~v) Tween*20 and 1% (w/v) ~SA, and peroxidase-con~ugated goa~ F(ab')2 anti-rabbit IgG was added for 2 hr. The Rlates were wa6hed ~-8 times and the peroxidase substrate wa6 added. The 6ubstrate con~isted of 2,2'-azino-di-(3-ethylbenz~hiazoline) sulfonic acid (~BTS, 0.03% w/v) and 0.03~ (v/v) H202 in 0.1 M citrate buffer (pH 4.0)~ color wa6 allowed to develop for 30 min and the optical den6ity dete~mined at 414 nm.
F. AntibodY ComPetition ELISA
~ n antibody com~etition ELIS~ was used to determine if antibodie~ detected by ~he ELISA were an~igen 6pecific. ~arious concentration~ (1 to 100 ng) of ~oluble competing antigen peptide IAl/30) were added to the wells ~o com~ete the binding of ~n~ibody eo pla6tic adsorbed ~yntheti~ polype~ti~e: for the~e studie6 the antiserum ~as diluted 1:5000 and the ( * ? Trademark -2~
antibodies were washed away and the bound anti~odies detected by the ELISA.
G. Sodium Dodecyl Sulate - PolYacrYlamide Gel Electro-Phoresis Purified and partially purified proteins were separated by SDS-PAGE. The stacking gels were 4~ and ~he separating gels were 15~ polyacrylamide. The gels were ei~her silver stained or electrophoretically :
transferred to nitrocellulose. In some instances, the gels were "spiked~ with 125I-labeled CIF-A as an internal standard to identify CIF-A in the gel or the protein to blot.
H- Two-Dimensional Acetic ~cid-Urea PAGE
Partially purified low molecular weight bone ex~racts were evaluated by two-dimensional polyacrylamide gel electrophoresis. Proteins (20 to ~0 ~g) were separated ~by mass and charge) in the first dimension in 15% polyacrylamide containing 2.5 M urea and acetic acid in glass tubes (2 x 4 x 125 mm) for 5-6 hr at 160 V (constant voltage), and the second dimension in a 15% SDS-polyacrylamide slab gel. The gels were either silver stained or the proteins were transferred to nitrocellulose (below). `In some instances, the gels were '`spiked" with I-labeled CIF-A and CIF-B and subsequently autoradiographed to identify the factors on the silver stained gel.
I~ Immunoblottinq Samples were fir~t electrophoretically separated ~n one or ~wo dimensions. After separation, the proteins were transferred to nitrocellulo~e using a trans blot apparatus filled with 25 mM Tri6 ~pH 8.3) and ~%6~
192 ~M glycine (pH ~.33 contai~ing ~0~ ~v/v~ ~ethanol.
T~e p~oteins were transferred for lB hr at 170 mA
(con6tant current). Following transfer, nonspeci~ic protein bindi~g wa~ blocked with P~S buffer containing 0.05% ~v~v) Tween-20 and 1% (w/v) BSA f or ~-2 hr. The protein blot~ were t~en incubated for 2 hr in a 1:100 d~lution~ of rabbit anti-Al~30 6erum. The ~lot wa~
was~ed for 30 min ~ith the ~ame buffer and the~
incubated for 1 hr wi~ 200,000 cpm,~ml ~- I]
protein-A. The immunoblo~ were washed~ air dried. and autoradiographed with Kodax*XAR-5 film at -80C for 1 to lB hr.
J. I~munohistochemical Staininq The cell association and di6tribution of CIF-~
was determined by immunohistochemical ~taining ~ethods.
Fetal bovine ti6sues were collected from a ~ingle ~nimal at 6 mont~ gestation. The ti~sue~ were fixed in 10~
neutral fo~malin. Hard ~i~sue~ were demineralized in lOS formic acid. The ti6~ues were dehydrated and paraffin embedded ~ith a Fi~her Histomatic Tisaue Proce~sor model 1~6A (15 hr ~ycle). The sections were deparaffinized with xylene and endogenous peroxidase blocked with 0.1% hydrogen peroxide in 0.01 M Tris containing 0.15 M NaCl (15 min). The sections were then treated with 1 mg~ml testicular hyaluronidase in 0~1 M
60dium acetate ~pH 5.5) in saline (30 min at 37C).
Non6pecific p~otein binding wa6 blocked with 005% (w/v) BSA in Tris-saline (15 min). The 6ection~ were incubated ~ith optimally diluted (1:50) rabbit (IgG~
anti-Al/30 or ~onimmune rabbit IgG ~or 1 ~, wa~hed with Tris-~aline, and incubated for 1 hr with peroxidase conjugated goat P(ab')2 anti-rabbit IgG. The slides were treated ~ith diaminobenzidine ~ub~trate buffer.
(*? Trademark ~6S~
The substrate buffer consisted of 0.5 mg/ml diaminobenzidine in 0.05 ~ Tris (pH) ~aline containing 0.1~ hyd~ogen perogide. The sections were counters~ained with ~ayer's hematoxylin.
Results A. n~ibodY Reactivity The antiserum had a titer of l:lO,OOO~on ~1-/30 -and CIF-A, and a titer of 1:1,000 on a partially purified CIF-~ containing bone extract. The antibodies also reacted with T~F-~ from platelets, as expected, since the N-terminal sequence is identical.
The competitive ~LISA method was used to determine if the antibodies detected by the ELISA were antigen-specific antibodies. In this experiment, the binding of an optimal dilution of antiserum (1:5,000~ to 400 ng of peptide Al/30 bound to plastic was competed with variable amounts (1 to 100 ng) of soluble synthetic polypeptide. Antibody binding was competed in a linear dose-response type fashion and 100 ng of the soluble competitor competed binding by more than 80%. The linear titrations characteristics of the antibodies and linear and near complete competitions of binding suggest that the antibodies were antigen specific. The antibody specificity was also confirmed by immunoblotting methods in which the antibodies were immunoreactive with nonreduced CIF-A and with B-mecaptoethanol-reduced CIF-A, a~ well as peptide Al/30. Having dete~mined that the antibodie~ to peptide ~1~30 were immunoreactive with CIF-A, they were used to determine if other molecular weight species of CIF-A were contained in crude bone extracts. High and low molecular weight bone extract~
s were prepa~ed and the congtituen~ proteins 6eparated by gel electrQphoresis. ~ silver stained gel and a duplicate immunoblot were pLepared. The te~t6 showed that antibodies to peptide ~lt30 detected only a protein of the same molecular weigh~ as CIF-~ in bo~h the high and low molecular weight bone extracts.
B. Cell ~ssociation and Tissue Distribution Osteocytes within the cancellous boneto~ the femur were specifically labeled by staining. In addition, there was intense staining of articula~
chondrocytes, particula~ly those cells in close association with the cartilage canals. Chondrocytes within the epiphyseal plate were not labeled by the lS antibodies, Kidney tissue and platelets were examined.
There was specific staining of the epithelial cells lining the calyces, while surrounding fitromal and parenchymal cells were not labeled by the anti-Al/30 antibodias. Bone marrow was also examined, and the platelet-p~oducing megakaryocytes were specifically labeled by the antibodies. Some mononuclear bone marrow cells were also stained by ~he antibodies.
Staining was also carried out to determine if CIF-~ might also be associated with centers of hematopoiesis and lymphopoiesis. There was intense cytoplasmic staining of clusters of hematopoie~ic stem cells in the fetal liver, while hepatocytes and stromal cells were not labeled. Hematopoie~ic stem cells in the bone marrow were specifically stained with the antibodie6. The thymus was examined and specific staining of Hassall' 8 corpuscle and some of the medullary thymocytes wa~ observed. There wa~ no specific staining of the less dif~erentiated co~tical ~2~
-24- . _ thymocytes. Further staining studie6 were carried out to confirm the thymic localization of CIF-A. The antibodies to CIF-A speci~ically stained the ret~culo-~pithelial cells in the medullary portion of the thymu6 and the epithelial cells comprising the Hassall's corpuscles. Epithelial cells in the cortical region and the surrounding capsule were not stained by the antibodies. There was no detectable staining of the subcapsular, cortical, or medullary thymocytes~
Other tissues were examined, including the thyroid, adrenal, and the submaxillary salivary gland, as well as the aorta. CIF-~ was not detected in any of these tissue by the staining technique.
The localization of CIF-~/TGF-~ in centers of hematopoiesis (bone marrow and liver) and lymphopoiesis (thymus) suggest that the molecule may regulate red blood cell and~or lymphocyte differentiation in vivo.
~cco~dingly, CIF may find use in therapy for indications as60ciated with dysfunction or malfunction of 2~0 hematopoiesis and~or lymphopoiesis such as congenital thymic aplasia, severe combined immunodeficiency, hereditary hemolytic anemia, and acquired hemolytic anemia.
3-Days Post Implantation 1. Carrier alone At three days post implantation, the implant was, for the mo6t part, acellular. Sparse neutrophils were the most apparent cell type.
2. CIF-Carrier The implant was also relatively acellular at three days. However, t~her~ was -an apparent act.ivation of fibroblasts from adjacentmuficle and the surLounding subcutaneous tissues. These fibroblasts contained abundant cytoplasm and were, Eor the most part, euchromatic suggesting the ce~ls were highly activated. Fibroblast infiltration was beginning at the margins of the implant.
10-Days Post Implantation 1 Carcier alone The inflammatory profile was .
markedly changed by 10 days following implantation. The implant con~ained a diffuse mixed inflammatory cell infiltrate dominated by lymphocy~es and histiocytes.
Focal areas of granulocytes (neutrophils and eosinophils) and giant cells were evident around some of 2~ the bone collagen particles.
2. CIF-Carrier There were few inflammatory cells a~sociated with the implant at this time poin~
Numerous hyperplastic fibroblasts were present throughout the implant. A collagenous connec~ive tissue matrix was evident around and 6urrounding the bone collagen powder pacticles.
-i5~
l~-Days Post Implantation 1. Carrier alone By 14-days post implantation, most bone collagen particles were sequestered by granulomas consis~ing of lymphocy~es, histiocytes and giant cells. Implant-aszociated fibrosis was evident as well as multifocal areas of eosinophils.
2. CIF-C_ rier Implant-associated inflammation was negligible compared with the control implants. A dense collagenous connective tissue matrix was e~ident throughout the implant. Morphologically, the fibrobla6~s appeared to be me~abolically less active than at earlie~ time points.
These histological obse~vations demonstrate that CIF inhibits inflammatory cell function in vivo.
The lack of polymorphonuclear neutrophils, lymphocytes, and histiocytes at the CIF-containing implant si~es suggests that CIF may function as a potent anti-inflammatory agent.
In the implants having CIF to carrier weight ratios of 1:8000 and 1:20000 there was a maLked reduction in implant-associated inflammation compared with carrier alone implants. The implan~s containing higher CIF to cacrier weight ratios developed a dense eollagenous eonneetive tissue matrix throughout the implant. ~t all CIF levels, implant-associated inflammation was negligible compared to no CIF.
In similar in vivo studies in which the rats reeeived bilateral implan~s with and without CIF-containing extracts, it was noted that inflamma~ion was redueed or absent in the implant ~emote from the CIF-containing implant. The6e ob6ervations indicate that CIF acts ~ystemically as well as locally.
When u~ed a6 a local an~i-inflammatory agent the CIF (and/or TGF-~) will usually be formula~ed in effective amount6 wi~h pharmaceutically acceptable carriers in weight ratios to carrier in the range of 1:1000 ~o 1:20000. If ti~sue deposition at the site i~
not desired, the level of CIF to carrier may be lowered to below that (e.g., a~ weight ratios ~elow abQ~t~ 6000-in the case of collagen carrier) which promote~ ~issuedeposition. In addition to being formulated as an in3ectable, the CIF may be incorporated (dispersed) into solid peLmeable implants such as collagenous soft and hard tissue implants, prostheses, sponges, wound dressings and sutures to modulate local inflammatory responses to such solid bodies. Since such implants are made from permeable materials the CIF can diffuse from the implant and exert its anti-inflammatory properties.
If it is de~ired to minimize other activities of CIF
lcell proliferation, tissue deposition) the CIF will be incorporated free of activating agents or coactor, ~referably at level6 below that which promote tissue deposition.
When used ~o treat inflammation at internal body sites locally, the CIF- or TGF-~-containing formulation is injected, inhaled, placed surgically, or otherwi~e administered locally, depending on the particular formulation, and the site where inflammation control is desired.
For systemic administration CIF may be formulated with conventional carriers used with water-soluble proteins for injection into circulation.
Alternat;vèly, it may be formulated as a sustairled ~2~ 5 release implant formulation if the indication being treated requires.
The amount o~ CIF (TGF-~) administered to treat inflammation will depend upon the pa~ient, ~he in~lammatory condition being treated, and the mode of administration. In general, the amounts administered to adul~ humans will be in the range of about 0.1 to 1000 ~g. When CIF i8 administered locally, amounts in the lower por~ion oE this range will normally-be us*d~ -typically 0.1 to 10 ~g. Correspondingly, sy~temic administra~ion will typically involve amounts in the 10-1000 ~g range.
CIF may be particularly effective in the treatment of inflammation involving the respiratory system. In this application, the CIFs may be administered by inhala~ion with a suitable aerosol. In this form, these factors would be useful for the treatment of diffuse interstitial diseases of the lung such as asbestosis, silicosis, or coal~miner's pneumoconiosis; the treatment of immunological diseases that involve the respiratory tract such as rheumatoid arthritis, lupus erythematosus, or GoodpastuLe's syndrome; and the treatment of granulomatous inflammation of the lungs and pulmonary tract ~uch as Wegener's granulomatosus and eosinophilic granulomatosus.
These anti-inflammatory peptides may be combined with carriers in the form of a salve, ointment, or other topical formulation and thereby by useful in the control of dermal inflammation by topical application. Such formulation~ would be particularly useful in the local treatment of p~oriasis vulgaris, contact dermatitis, dermal ulcers, and acute or chronic eczematous dermatitis.
~ ~S'~4~;
-17- , _ CIF may be either used alone or combined with a slow release carrier and injec~ed into or around joints.
bone, or muscle for the con~rol of in1ammatio~
associated with various diseases. Some examples include myositis (viral, bacterial, parasitic, fungal o~
autoimmune pcocesses) myasthenia gravis: osteomyelitis:
osteoarthritis and rheumatoid arthritis.
Since ~he CIF molecules have been shown ~o be stable at low pH and resistent to enzyme digest~ion, ~- -~hese factors may be delivered systemically byingestion. These properties make these factors particularly useful for controlling inflammation in the gas~rointes~inal tract. This would be particularly useful for the treatment of gastric and duodenal ulcers, granulomatous gastritis, esophagitis (numerous causes):
enteristis (numerous causes) and colitis (numerous causes).
3. Immunohistochemical Localization of CIF-~ (TGF-~) 2~
Materials and Methods . Synthetic Polv~ep~ide SYnthesi~
~ synthetic polypeptide, referred to as Al/30, was constructed to be identical to the N-terminal amino acid sequence (residues 1-30) of CIF-A and TGF-~. The peptide Al/30 was synthesized by a solid-phase method.
The peptide was assembled on p-me~hylbenzhydrylamine resin, cleaved from the resin, deprotected via a 2-step hydrogen fluoride procedure, and purified by reverse-phase liquid chromatography on octadeaylsilica.
Peptide Al/30 was determined to be homogeneous by RP-HPLC and thin layer chromatography and the amino acid sequence was verified by gas-phase se~uence analysis.
5~
B. Radioiodination Purified CIF-~ and CIF-B were radioiodinated with Na I using a lactoperoxidase method. The specific activity was 0.8 to 1.0 x 107 cpm/~g protein.
C. Immunization A New Zealand white rabbit was immunized wi~h peptide ~1/30 at multiple intramuscular sites biweekly for 6-10 weeks using 250 to 500 ~g of peptide ~1/30 per injec~ion. The primary immunization was in Freund' 6 compleie adjuvant and the subsequent boosts were in Freund`s incomplete adjuvant. Ten days following the final boos~, the rabbit was bled by cardiac puncture.
The blood was clot~ed at 22C for 4 hr and overnight at 4C, and the serum was collected and stored at -70C.
D. ~ntibody Purification Serum IgG was purified using Sepharose protein-A. Briefly, serum was diluted with an equal volume of 0.01 M Tris (pH 7.2) con~aining 0.15 M NaCl.
Antibodies were precipitated with an equal volume of saturated ammonium sulfate adjusted to pH 8.0 (4C) and collected by centrifugation at 100,000 x g (30 min).
The protein pellet was resuspended in a minimal volume of pH 7.2 PBS and dialyzed against PBS. The retentate was clarified by centrifugation and the supernatant applied to a 10 ml column of Sepharose protein-~. Bound IgG was eluted with 0.1 M glycine-HCl (pH 2.0). The antibodies were immediately neutralized (4.0 M Tri~), dialyzed against PBS, and lyophilized.
~L2~5~
E. ~nzyme-Linked Immuno~orbent ~s~ay (EkIS~) ~ ntiserum ~as evaluated for reactivi~y with pept;de A1~30, CIF-~, or the low ~olecular weigh~ bone extract by an ELISA. Peptide Al/30 was solubilized in PBS, while purified CIF-A or t~e partially purified bone ~xtracts were solubilized in 0.01 ~ HCl. ~ntige~6 ~ere diluted in 0.01 M carbonate bufer ~pH 9.63 and 400 ng of p~o~ein in 100 ~1 volume were added to ~he well6 of a ~icrotitar ~late. Peptides ~1/30 and ~IF-A ~ere~
dried onto ~e wells overnight. Pla~e~ con~aining the partially purified e~ract were ~ealed and ~tored overnight at 4C. Prio~ to u6e. nonspecific protein binding to the ~LISA pla~e was blocked by incubating with PBS containing 1~ (w/v) BSA for 1 hr. Anti~erum wa8 6e~ially twoold diluted and 100 ~1 ~ere added to each well for 1 hr. The plates ~er0 was~ed wi~h PBS
containing 0.05% (v~v) Tween*20 and 1% (w/v) ~SA, and peroxidase-con~ugated goa~ F(ab')2 anti-rabbit IgG was added for 2 hr. The Rlates were wa6hed ~-8 times and the peroxidase substrate wa6 added. The 6ubstrate con~isted of 2,2'-azino-di-(3-ethylbenz~hiazoline) sulfonic acid (~BTS, 0.03% w/v) and 0.03~ (v/v) H202 in 0.1 M citrate buffer (pH 4.0)~ color wa6 allowed to develop for 30 min and the optical den6ity dete~mined at 414 nm.
F. AntibodY ComPetition ELISA
~ n antibody com~etition ELIS~ was used to determine if antibodie~ detected by ~he ELISA were an~igen 6pecific. ~arious concentration~ (1 to 100 ng) of ~oluble competing antigen peptide IAl/30) were added to the wells ~o com~ete the binding of ~n~ibody eo pla6tic adsorbed ~yntheti~ polype~ti~e: for the~e studie6 the antiserum ~as diluted 1:5000 and the ( * ? Trademark -2~
antibodies were washed away and the bound anti~odies detected by the ELISA.
G. Sodium Dodecyl Sulate - PolYacrYlamide Gel Electro-Phoresis Purified and partially purified proteins were separated by SDS-PAGE. The stacking gels were 4~ and ~he separating gels were 15~ polyacrylamide. The gels were ei~her silver stained or electrophoretically :
transferred to nitrocellulose. In some instances, the gels were "spiked~ with 125I-labeled CIF-A as an internal standard to identify CIF-A in the gel or the protein to blot.
H- Two-Dimensional Acetic ~cid-Urea PAGE
Partially purified low molecular weight bone ex~racts were evaluated by two-dimensional polyacrylamide gel electrophoresis. Proteins (20 to ~0 ~g) were separated ~by mass and charge) in the first dimension in 15% polyacrylamide containing 2.5 M urea and acetic acid in glass tubes (2 x 4 x 125 mm) for 5-6 hr at 160 V (constant voltage), and the second dimension in a 15% SDS-polyacrylamide slab gel. The gels were either silver stained or the proteins were transferred to nitrocellulose (below). `In some instances, the gels were '`spiked" with I-labeled CIF-A and CIF-B and subsequently autoradiographed to identify the factors on the silver stained gel.
I~ Immunoblottinq Samples were fir~t electrophoretically separated ~n one or ~wo dimensions. After separation, the proteins were transferred to nitrocellulo~e using a trans blot apparatus filled with 25 mM Tri6 ~pH 8.3) and ~%6~
192 ~M glycine (pH ~.33 contai~ing ~0~ ~v/v~ ~ethanol.
T~e p~oteins were transferred for lB hr at 170 mA
(con6tant current). Following transfer, nonspeci~ic protein bindi~g wa~ blocked with P~S buffer containing 0.05% ~v~v) Tween-20 and 1% (w/v) BSA f or ~-2 hr. The protein blot~ were t~en incubated for 2 hr in a 1:100 d~lution~ of rabbit anti-Al~30 6erum. The ~lot wa~
was~ed for 30 min ~ith the ~ame buffer and the~
incubated for 1 hr wi~ 200,000 cpm,~ml ~- I]
protein-A. The immunoblo~ were washed~ air dried. and autoradiographed with Kodax*XAR-5 film at -80C for 1 to lB hr.
J. I~munohistochemical Staininq The cell association and di6tribution of CIF-~
was determined by immunohistochemical ~taining ~ethods.
Fetal bovine ti6sues were collected from a ~ingle ~nimal at 6 mont~ gestation. The ti~sue~ were fixed in 10~
neutral fo~malin. Hard ~i~sue~ were demineralized in lOS formic acid. The ti6~ues were dehydrated and paraffin embedded ~ith a Fi~her Histomatic Tisaue Proce~sor model 1~6A (15 hr ~ycle). The sections were deparaffinized with xylene and endogenous peroxidase blocked with 0.1% hydrogen peroxide in 0.01 M Tris containing 0.15 M NaCl (15 min). The sections were then treated with 1 mg~ml testicular hyaluronidase in 0~1 M
60dium acetate ~pH 5.5) in saline (30 min at 37C).
Non6pecific p~otein binding wa6 blocked with 005% (w/v) BSA in Tris-saline (15 min). The 6ection~ were incubated ~ith optimally diluted (1:50) rabbit (IgG~
anti-Al/30 or ~onimmune rabbit IgG ~or 1 ~, wa~hed with Tris-~aline, and incubated for 1 hr with peroxidase conjugated goat P(ab')2 anti-rabbit IgG. The slides were treated ~ith diaminobenzidine ~ub~trate buffer.
(*? Trademark ~6S~
The substrate buffer consisted of 0.5 mg/ml diaminobenzidine in 0.05 ~ Tris (pH) ~aline containing 0.1~ hyd~ogen perogide. The sections were counters~ained with ~ayer's hematoxylin.
Results A. n~ibodY Reactivity The antiserum had a titer of l:lO,OOO~on ~1-/30 -and CIF-A, and a titer of 1:1,000 on a partially purified CIF-~ containing bone extract. The antibodies also reacted with T~F-~ from platelets, as expected, since the N-terminal sequence is identical.
The competitive ~LISA method was used to determine if the antibodies detected by the ELISA were antigen-specific antibodies. In this experiment, the binding of an optimal dilution of antiserum (1:5,000~ to 400 ng of peptide Al/30 bound to plastic was competed with variable amounts (1 to 100 ng) of soluble synthetic polypeptide. Antibody binding was competed in a linear dose-response type fashion and 100 ng of the soluble competitor competed binding by more than 80%. The linear titrations characteristics of the antibodies and linear and near complete competitions of binding suggest that the antibodies were antigen specific. The antibody specificity was also confirmed by immunoblotting methods in which the antibodies were immunoreactive with nonreduced CIF-A and with B-mecaptoethanol-reduced CIF-A, a~ well as peptide Al/30. Having dete~mined that the antibodie~ to peptide ~1~30 were immunoreactive with CIF-A, they were used to determine if other molecular weight species of CIF-A were contained in crude bone extracts. High and low molecular weight bone extract~
s were prepa~ed and the congtituen~ proteins 6eparated by gel electrQphoresis. ~ silver stained gel and a duplicate immunoblot were pLepared. The te~t6 showed that antibodies to peptide ~lt30 detected only a protein of the same molecular weigh~ as CIF-~ in bo~h the high and low molecular weight bone extracts.
B. Cell ~ssociation and Tissue Distribution Osteocytes within the cancellous boneto~ the femur were specifically labeled by staining. In addition, there was intense staining of articula~
chondrocytes, particula~ly those cells in close association with the cartilage canals. Chondrocytes within the epiphyseal plate were not labeled by the lS antibodies, Kidney tissue and platelets were examined.
There was specific staining of the epithelial cells lining the calyces, while surrounding fitromal and parenchymal cells were not labeled by the anti-Al/30 antibodias. Bone marrow was also examined, and the platelet-p~oducing megakaryocytes were specifically labeled by the antibodies. Some mononuclear bone marrow cells were also stained by ~he antibodies.
Staining was also carried out to determine if CIF-~ might also be associated with centers of hematopoiesis and lymphopoiesis. There was intense cytoplasmic staining of clusters of hematopoie~ic stem cells in the fetal liver, while hepatocytes and stromal cells were not labeled. Hematopoie~ic stem cells in the bone marrow were specifically stained with the antibodie6. The thymus was examined and specific staining of Hassall' 8 corpuscle and some of the medullary thymocytes wa~ observed. There wa~ no specific staining of the less dif~erentiated co~tical ~2~
-24- . _ thymocytes. Further staining studie6 were carried out to confirm the thymic localization of CIF-A. The antibodies to CIF-A speci~ically stained the ret~culo-~pithelial cells in the medullary portion of the thymu6 and the epithelial cells comprising the Hassall's corpuscles. Epithelial cells in the cortical region and the surrounding capsule were not stained by the antibodies. There was no detectable staining of the subcapsular, cortical, or medullary thymocytes~
Other tissues were examined, including the thyroid, adrenal, and the submaxillary salivary gland, as well as the aorta. CIF-~ was not detected in any of these tissue by the staining technique.
The localization of CIF-~/TGF-~ in centers of hematopoiesis (bone marrow and liver) and lymphopoiesis (thymus) suggest that the molecule may regulate red blood cell and~or lymphocyte differentiation in vivo.
~cco~dingly, CIF may find use in therapy for indications as60ciated with dysfunction or malfunction of 2~0 hematopoiesis and~or lymphopoiesis such as congenital thymic aplasia, severe combined immunodeficiency, hereditary hemolytic anemia, and acquired hemolytic anemia.
4. ~CtiVitY of CIF on DeveloPinq T LYmphocytes Having established ~hat CIF is associa~ed in situ with developing T lymphocytes, tests wera carried out as follows to determine the effect of CIF upon the mitogenic response of thymocytes.
~0 . Cell Culture PreParation Single cell suspensions of murine (C3H/He~
thymocytes were prepared and the cells suspended i~
Eagle's minimal essential medium supplemented with 5%
fetal calf 6erum, 100 Utml penicillin, 100 ~g~ml strepeomycin, 2 mM L-glutamine, and 5 x 10 M
2-mercaptoethanol. Cell viability was determined by cell morphology and trypan blue exclusion.
B. IL-l ~ssa~
Thymocytes (1 x 10 ) were plated into flatbottom 96 well microtiter plates. The cells were co-stimulated with optimal concentrations-of ~ -phytohemag~lutinin (PHA) and IL-l (2 U IL-l and PX~).
Purified, endotoxin-free human blood monocyte derived IL-l or recombinant IL-l (rIL-l) were used. One unit of specific activity was de~ined as ~he amount of IL-l which results in a half maximal thymocyte proliferative res~onse. Different amounts of CIF-A (TGF-~) and CIF-B
were added to the thymocyte cultures (see Figures 4-7).
The cells were cultured for 72 hr in a humidified incubator in 5% CO2 at 37C. Prior to harvesting ~24 hr), the cultures were pulsed with 0.5 ~Ci of H-thymidine. The cultures were harvested with a semi-automated cell harvester and the amount of H-thymidine incorpora~ion was determined by standard liquid scintillation methods.
Results The re~ul~s of the tests are reported graphically in Figures 4-7. As seen in Figure 4A, 1.9 x M and 1.5 x 10 M concentrations of TGF-B
inhibited (86% to 92% of control) H-thymidine incorporation by thymocyte culture6 treated with 2 U to 40 U of rIL-l. TGF-B at a culture concentration of 1.9 x 10 M inhibited the proli~erative Lesponse by 49%
to 59% at each concentration of rIL-l tested.
Similarly, 1.9 x 10 M CIF-B inhibited (90% of ~65~
control) thymocyte proliferation ~o all concentrations of rIL-l tested. Thymocyte cultures with 1.5 x 10 M CIF-B were inhibited by 50~ to 60~; while cultures treated with 1.9 x 10 12 M CIF-B were inhibited by 17%
to 26% compared wi~h nontreated control cultures. The cell viability of the TGF-~ and CIF-B ~reated cultures was comparable to nontreated cultures as judged by cell mo~phology and trypan blue exclusion.
, The effective dose range for TGF-~ and~CIF B is illustrated in Figure 5. The effective do~e cange was between 10 M and 10 M for both ~actor~. Both factors exhibited maximal inhibition (90~ of control) at a culture concentration of approximately 2 x 10 M;
half-maximal inhibition for TGF-~ and CIF-B was 6 x 1~ 10 12 M and 4 x 10 12 M, respectively.
The results depicted in Figures 4 and 5 show that when TGF-~ or CIF-B was simultaneously added to the cultures with IL-l and PHA there was a dose-dependent inhibition of the proliferative response. Figure 6 shows the effect of these factors upon thymocytes prestimulated by the mitogens. In that experi~ent, thymocyte cultures were stimulated with 2 U IL-l and PHA
for 1 hr to 48 hr prior to the addition of TGF-~ oe CIF-B (1.9 x 10 M). The results of Figure 6 show that cultures prestimulated for 1 hr to 6 hr by the mitogens were significantly inhibi~ed (86% of control) by the addition of exogenous TGF-~ or CIF-B. Thymocytes prestimulated ~or 24 hr were partially inhibited (47% to 63~ of control) by treatment with TGF-~ or CIF-B.
Thymocytes prestimulated for 48 hr were not affected, or were only slightly (27~ of control) inhibited, by treatement with T&F-~ or CIF-B.
-As indicated in Figure 6 TGF-~ and CIF-B were mo~t effective at suppressing the mitogenic response ~2~14~
-27- .
when ~he cells were exposed to ~hese factors during the initial inductive phase. The question of whether continuou6 exposure to these factor6 was required to maintain the inhibitory effect is addressed by the results of Figure 7. In these experiments, thymocytes were pretreated (1 hr to 4 hr) in culture tubes with differen~ concentrations o~ TGF-~ or CIF-B. The pretreated cells were washed extensively ~o remove the exogenous factor and then transferred to micro~ultures with 2 U IL-l and PH~ for an additional 72 hr. Control culturas were treated identical to the pretreated cultures, except TGF-B or CIY-B was added directly to the microculture wells. The results show that cells pretreated for 4 hr with TGF-~ or CI~-B (10 1 M) were less responsi~e (50~ of control) to subsequent stimulation by the mitogens compared with the nontreated control cultures. ~ells pretreated for 1 hr to 2 hr with 10 M TGF-B or CIF-B were only slightly less responsive (20% to 30% respectively) to mitogen stimulation. Cells pretreated for 1 hr to 2 hr with low concentrations (10 M and 10 11 M) of the factors were not inhibited from responding to IL-l induction.
The results of Example 4, in conjunction with the immunolocalization results, suggest that TGF-~ (and perhaps CIF-B) may function physiologically by regulating clonal expansion of the developing T-lymphocyte: and, further, the cells comprising the Hassall`s cor~uscles are likely the cell-types responsible for producing TGF-B in the thymus. This concept ifi supported, in part, by whole animal radiolabelling studies which show that the majority of thymocy~e proliferation is restricted to the subcapsular and cortical regions of the t ffl mu~ and that tffl mocyte ~26S~5 -28- . -maturation i~ compartmentalized within the medullary portion of the thymus.
While the mechanism whereby TGF-~ and CIF-B
inhibits the proliferative respon~e of thymocytes is not understood, a likely explanation is that these factors pertucb IL-2 production and IL-2 receptor e~pression by the IL-l treated ~hymocytes. Failure of the cell to produce either the grow~h factor or the receptor will result in the failure of the T lym~hocyte to b~come--10 aCtivated~
~0 . Cell Culture PreParation Single cell suspensions of murine (C3H/He~
thymocytes were prepared and the cells suspended i~
Eagle's minimal essential medium supplemented with 5%
fetal calf 6erum, 100 Utml penicillin, 100 ~g~ml strepeomycin, 2 mM L-glutamine, and 5 x 10 M
2-mercaptoethanol. Cell viability was determined by cell morphology and trypan blue exclusion.
B. IL-l ~ssa~
Thymocytes (1 x 10 ) were plated into flatbottom 96 well microtiter plates. The cells were co-stimulated with optimal concentrations-of ~ -phytohemag~lutinin (PHA) and IL-l (2 U IL-l and PX~).
Purified, endotoxin-free human blood monocyte derived IL-l or recombinant IL-l (rIL-l) were used. One unit of specific activity was de~ined as ~he amount of IL-l which results in a half maximal thymocyte proliferative res~onse. Different amounts of CIF-A (TGF-~) and CIF-B
were added to the thymocyte cultures (see Figures 4-7).
The cells were cultured for 72 hr in a humidified incubator in 5% CO2 at 37C. Prior to harvesting ~24 hr), the cultures were pulsed with 0.5 ~Ci of H-thymidine. The cultures were harvested with a semi-automated cell harvester and the amount of H-thymidine incorpora~ion was determined by standard liquid scintillation methods.
Results The re~ul~s of the tests are reported graphically in Figures 4-7. As seen in Figure 4A, 1.9 x M and 1.5 x 10 M concentrations of TGF-B
inhibited (86% to 92% of control) H-thymidine incorporation by thymocyte culture6 treated with 2 U to 40 U of rIL-l. TGF-B at a culture concentration of 1.9 x 10 M inhibited the proli~erative Lesponse by 49%
to 59% at each concentration of rIL-l tested.
Similarly, 1.9 x 10 M CIF-B inhibited (90% of ~65~
control) thymocyte proliferation ~o all concentrations of rIL-l tested. Thymocyte cultures with 1.5 x 10 M CIF-B were inhibited by 50~ to 60~; while cultures treated with 1.9 x 10 12 M CIF-B were inhibited by 17%
to 26% compared wi~h nontreated control cultures. The cell viability of the TGF-~ and CIF-B ~reated cultures was comparable to nontreated cultures as judged by cell mo~phology and trypan blue exclusion.
, The effective dose range for TGF-~ and~CIF B is illustrated in Figure 5. The effective do~e cange was between 10 M and 10 M for both ~actor~. Both factors exhibited maximal inhibition (90~ of control) at a culture concentration of approximately 2 x 10 M;
half-maximal inhibition for TGF-~ and CIF-B was 6 x 1~ 10 12 M and 4 x 10 12 M, respectively.
The results depicted in Figures 4 and 5 show that when TGF-~ or CIF-B was simultaneously added to the cultures with IL-l and PHA there was a dose-dependent inhibition of the proliferative response. Figure 6 shows the effect of these factors upon thymocytes prestimulated by the mitogens. In that experi~ent, thymocyte cultures were stimulated with 2 U IL-l and PHA
for 1 hr to 48 hr prior to the addition of TGF-~ oe CIF-B (1.9 x 10 M). The results of Figure 6 show that cultures prestimulated for 1 hr to 6 hr by the mitogens were significantly inhibi~ed (86% of control) by the addition of exogenous TGF-~ or CIF-B. Thymocytes prestimulated ~or 24 hr were partially inhibited (47% to 63~ of control) by treatment with TGF-~ or CIF-B.
Thymocytes prestimulated for 48 hr were not affected, or were only slightly (27~ of control) inhibited, by treatement with T&F-~ or CIF-B.
-As indicated in Figure 6 TGF-~ and CIF-B were mo~t effective at suppressing the mitogenic response ~2~14~
-27- .
when ~he cells were exposed to ~hese factors during the initial inductive phase. The question of whether continuou6 exposure to these factor6 was required to maintain the inhibitory effect is addressed by the results of Figure 7. In these experiments, thymocytes were pretreated (1 hr to 4 hr) in culture tubes with differen~ concentrations o~ TGF-~ or CIF-B. The pretreated cells were washed extensively ~o remove the exogenous factor and then transferred to micro~ultures with 2 U IL-l and PH~ for an additional 72 hr. Control culturas were treated identical to the pretreated cultures, except TGF-B or CIY-B was added directly to the microculture wells. The results show that cells pretreated for 4 hr with TGF-~ or CI~-B (10 1 M) were less responsi~e (50~ of control) to subsequent stimulation by the mitogens compared with the nontreated control cultures. ~ells pretreated for 1 hr to 2 hr with 10 M TGF-B or CIF-B were only slightly less responsive (20% to 30% respectively) to mitogen stimulation. Cells pretreated for 1 hr to 2 hr with low concentrations (10 M and 10 11 M) of the factors were not inhibited from responding to IL-l induction.
The results of Example 4, in conjunction with the immunolocalization results, suggest that TGF-~ (and perhaps CIF-B) may function physiologically by regulating clonal expansion of the developing T-lymphocyte: and, further, the cells comprising the Hassall`s cor~uscles are likely the cell-types responsible for producing TGF-B in the thymus. This concept ifi supported, in part, by whole animal radiolabelling studies which show that the majority of thymocy~e proliferation is restricted to the subcapsular and cortical regions of the t ffl mu~ and that tffl mocyte ~26S~5 -28- . -maturation i~ compartmentalized within the medullary portion of the thymus.
While the mechanism whereby TGF-~ and CIF-B
inhibits the proliferative respon~e of thymocytes is not understood, a likely explanation is that these factors pertucb IL-2 production and IL-2 receptor e~pression by the IL-l treated ~hymocytes. Failure of the cell to produce either the grow~h factor or the receptor will result in the failure of the T lym~hocyte to b~come--10 aCtivated~
5. ~CtiVitY of CIF on Mature Lymphocytes Materials and Methods A. Purification of Peripheral Blood LYmphocytes Peripheral blood mononuclear cells weceisolated from heparinized blood of healthy adult human donors in Ficoll-Hypaque density gradients. The red blood cell-free buffy coat was collected from the aqueous-ficoll interface. The monocytes were removed by incubating at 37C for 1 hr on tissue culture plastic in RPMI 1640 medium containing 10~ fetal calf serum (FCS).
The T lymphocytes were isolated from the nonadherent cells by rosetting with 0.25% sheep red blood cells (E-ro~ettes) for 2 hr at 37C. ~he E-rosetted T
lymphocy~es were separated from the nonrosetted B
lymphocytes by centrifugation through Ficoll-Hypaque for 30 to 40 min at 500 x g. The pellet was >95% E-rosetted cells. The sheep red blood cells were lysed with 0.83%
ammonium chloride.
The nonrosetted B lymphocytes were collected from the ficoll-aqueQus interface.
~i5~
--2g--B. T Cell Mitoqen ~ssaY
T lymphocyte proliferation was evaluated using a mitogen microassay. The assay consisted of plating 0.2 x 10 T cells into s6-well microassay plates. The cells were cultured in RPMI 1~40 medium supplemented with L-glutamine, penicillinstreptomycin, and 10% FCS.
The cul~ures were mitogen stimulated with Concanavalin-A
~6.2 to 24 ~g/ml). CIF-~ or CIF-B was added to the microcultures between 0.01 to 40 ng/ml. The f~nal-culture volumes were adjusted to 250 ~1, and themixture was incubated for 5 days at 37C in a humidified incubator in a 5~ C0~ atmosphere. The cultures were pulsed with 1.0 ~Ci of 3H-thymidine (specific activity ~5 Ci/mmole) 18 hr prior to harvesting with an automated cell harvester. Inhibition of H-thymidîne incorporation by various concentrations of CIF-A or CIF-B was determined from triplicate cultures by the following formula:
mitogen treated with CIF (cpm) % inhibition = 1 - x 100 mitogen-treated control without CIF (cpm) C. B Cell ~ctivation AssaY
A lymphocyte culture was made by mixing 10 T
lymphocytes with 2.5 x 10 fresh autologous B
lymphocytes. The cells were cultured at 37C in 5 C2 in 1 ml RPMI 16~0 medium supplemented with L-glutamine, penicillin-streptomycin, and 10% FCS. The cultures were set up in 12 x 75 mm culture tubes.
Pokeweed mitogen was added to cultures at a 1/100 dilution.--To these cultures various concentrations (1.9 -12 -10 1 5 10-9 M) f either CIF-A or CIF-B were added to the cultures. The cells were cultured for 7 days.
At the end of the culture period, the cell-free culture supernatants were assayed ~or IgM or IgG by a sandwich ELISA method. Flat-bottom polyvinyl chloride microtiter plates were incubated overnight at 4C with approximately 120 to 500 ~g of affinity-purified goat anti-human IgM or IgG in phosphate-buffered saline (PBS~. Th~ plates were washëd with PBS contai~ing-0.-05%
Twaen-20 (PT buffer) in order to remove unbound antibody. The culture supernatants were diluted either 1/10 or 1/100 in PBS containing 0.05% Tween-20 and 0.5%
bovine serum albumen (PTB buffer). To generate a standard cur~e, various concentrations (2 to 10 ng) of purified human IgG or IgM were added to the appropriate wells. After 2 hr at room temperature, the plates were washed with PT buf~er. One hundreds microliters of a 1~5,000 dilution of peroxidase-conjugated goat anti-human IgG or anti-human IgM were added to the wells. After a 1 hr incubation, the plates were washed with PT buffer, and 100 ~1 of freshly prepared substrate was added. The substrate consisted of ~BTS, 0.03~ (w/v), and 0.03% (v/v) hydrogen peroxide in 0.1 M
citrate buffer (pH 4.0). Color was allowed to develop for 30 min and the optical density was determined at 414 nm. The concentration of IgG or IgM was calculated from a standard curve run simultaneously with the assays.
Inhibition of IgG or IgM production ~y the B calls was calculated by comparing the CIF-~- or CIF-B-treated cultures to control cultures which were not treatQd with CIF. The following formula was used:
% inhibition ng/ml Ig (wi~h CIF) of antibody = 1 - - -- x 100 ng/ml Ig (wi~hout CIF) 6S~5 -31~
Results The results of the T cell proliferation assays are plotted in Figure 8. ~8 seen in this figure. both CIF-A and CIF-B were found to have comparable activities upon T lymphocyte proliferation. 3H-thymidine incorporation was inhibited by 78% to 80% by approximately 38 x 10 12 M CIF-~ or CIF-B. The half-maximal activity for CIF-A was less than 1 x 2 M. The half-maximal activity for ~IF-B was e5timated to be approximately 1.9 x 10 M. These results show clearly that both CIFs are potent inhibitors of human T lymphocy~e proliferation.
The results o~ the B cell activation assay are summarized in Table 2 below. The data presented represent the mean ~ SD for the three experiments.
o y ~ o o o o o o D ` , d' '~ ~ co N N O D ~ N
N i O N
C O ~ ~ I N O
~D ~O ~ ~ ~ '~ . I`
~ n N ~ ~ ~
s~
~ cl o o o o o o C I Y? O O N O O
N
N N ~
r ~ O O N O O
2 Q ~ N O O N O O
3 X ~ Nj Nl h ,~ o o o o o o X X X ~ ~4 ~C X . .
C ~ ~ ~
~ o c~ ,i ~ ,i ,i ,i ,1 ,1 ,~ ,1 ,~ ,~ , ,~ ,~ ~ ,~ ,.. , m ~ P~ m P~ ~ Ia + + + + + + ~
W ,~ ,~ ,~ ,1 ~ ,, . a) Ql ~ ~ ~ ~ a~
;54~
~ s shown in Table 2, CIF-A at 1.9 x 10 M
reduced ~he amount of IgM produced by 33% and IgG by 16%
when compared with ~he nontreated control culture.
There was complete inhibition of IgM production in cultures containing either 1.9 x 10 M or 1.~ x ~ concentrations of CIF-~. Similar concentrations of CIF-~ resulted in a 54~ to 56%
inhibition of IgG production.
CIF-B was found to be comparable to CIF A As seen in Table 2, cultures containing 1.9 x 10 M
concentrations o~ CIF-B contained no IgM and only 54% of the IgG when compared with the untreated control cultures. Cultures trsated with 1.5 x 10 M
concentrations of CIF-B contained no measurable IgM and very little (8g~ inhibition) or no IgG. These results show that both CIF-A and CIF-B are extremely potent inhibitors of antibody production by plasma cells.
These in vitro T cell proliferation and B cell activation experiments suggest that lymphocyte regulation may be one mechanism involved in the in vivo lymphohistiocytic anti-inflammatory activity of CIF
observed previously. The results of these tests confirm the work reported by Kehrl, J.H.. et al, Clinical Research (1985) 610~.
The T lymphocytes were isolated from the nonadherent cells by rosetting with 0.25% sheep red blood cells (E-ro~ettes) for 2 hr at 37C. ~he E-rosetted T
lymphocy~es were separated from the nonrosetted B
lymphocytes by centrifugation through Ficoll-Hypaque for 30 to 40 min at 500 x g. The pellet was >95% E-rosetted cells. The sheep red blood cells were lysed with 0.83%
ammonium chloride.
The nonrosetted B lymphocytes were collected from the ficoll-aqueQus interface.
~i5~
--2g--B. T Cell Mitoqen ~ssaY
T lymphocyte proliferation was evaluated using a mitogen microassay. The assay consisted of plating 0.2 x 10 T cells into s6-well microassay plates. The cells were cultured in RPMI 1~40 medium supplemented with L-glutamine, penicillinstreptomycin, and 10% FCS.
The cul~ures were mitogen stimulated with Concanavalin-A
~6.2 to 24 ~g/ml). CIF-~ or CIF-B was added to the microcultures between 0.01 to 40 ng/ml. The f~nal-culture volumes were adjusted to 250 ~1, and themixture was incubated for 5 days at 37C in a humidified incubator in a 5~ C0~ atmosphere. The cultures were pulsed with 1.0 ~Ci of 3H-thymidine (specific activity ~5 Ci/mmole) 18 hr prior to harvesting with an automated cell harvester. Inhibition of H-thymidîne incorporation by various concentrations of CIF-A or CIF-B was determined from triplicate cultures by the following formula:
mitogen treated with CIF (cpm) % inhibition = 1 - x 100 mitogen-treated control without CIF (cpm) C. B Cell ~ctivation AssaY
A lymphocyte culture was made by mixing 10 T
lymphocytes with 2.5 x 10 fresh autologous B
lymphocytes. The cells were cultured at 37C in 5 C2 in 1 ml RPMI 16~0 medium supplemented with L-glutamine, penicillin-streptomycin, and 10% FCS. The cultures were set up in 12 x 75 mm culture tubes.
Pokeweed mitogen was added to cultures at a 1/100 dilution.--To these cultures various concentrations (1.9 -12 -10 1 5 10-9 M) f either CIF-A or CIF-B were added to the cultures. The cells were cultured for 7 days.
At the end of the culture period, the cell-free culture supernatants were assayed ~or IgM or IgG by a sandwich ELISA method. Flat-bottom polyvinyl chloride microtiter plates were incubated overnight at 4C with approximately 120 to 500 ~g of affinity-purified goat anti-human IgM or IgG in phosphate-buffered saline (PBS~. Th~ plates were washëd with PBS contai~ing-0.-05%
Twaen-20 (PT buffer) in order to remove unbound antibody. The culture supernatants were diluted either 1/10 or 1/100 in PBS containing 0.05% Tween-20 and 0.5%
bovine serum albumen (PTB buffer). To generate a standard cur~e, various concentrations (2 to 10 ng) of purified human IgG or IgM were added to the appropriate wells. After 2 hr at room temperature, the plates were washed with PT buf~er. One hundreds microliters of a 1~5,000 dilution of peroxidase-conjugated goat anti-human IgG or anti-human IgM were added to the wells. After a 1 hr incubation, the plates were washed with PT buffer, and 100 ~1 of freshly prepared substrate was added. The substrate consisted of ~BTS, 0.03~ (w/v), and 0.03% (v/v) hydrogen peroxide in 0.1 M
citrate buffer (pH 4.0). Color was allowed to develop for 30 min and the optical density was determined at 414 nm. The concentration of IgG or IgM was calculated from a standard curve run simultaneously with the assays.
Inhibition of IgG or IgM production ~y the B calls was calculated by comparing the CIF-~- or CIF-B-treated cultures to control cultures which were not treatQd with CIF. The following formula was used:
% inhibition ng/ml Ig (wi~h CIF) of antibody = 1 - - -- x 100 ng/ml Ig (wi~hout CIF) 6S~5 -31~
Results The results of the T cell proliferation assays are plotted in Figure 8. ~8 seen in this figure. both CIF-A and CIF-B were found to have comparable activities upon T lymphocyte proliferation. 3H-thymidine incorporation was inhibited by 78% to 80% by approximately 38 x 10 12 M CIF-~ or CIF-B. The half-maximal activity for CIF-A was less than 1 x 2 M. The half-maximal activity for ~IF-B was e5timated to be approximately 1.9 x 10 M. These results show clearly that both CIFs are potent inhibitors of human T lymphocy~e proliferation.
The results o~ the B cell activation assay are summarized in Table 2 below. The data presented represent the mean ~ SD for the three experiments.
o y ~ o o o o o o D ` , d' '~ ~ co N N O D ~ N
N i O N
C O ~ ~ I N O
~D ~O ~ ~ ~ '~ . I`
~ n N ~ ~ ~
s~
~ cl o o o o o o C I Y? O O N O O
N
N N ~
r ~ O O N O O
2 Q ~ N O O N O O
3 X ~ Nj Nl h ,~ o o o o o o X X X ~ ~4 ~C X . .
C ~ ~ ~
~ o c~ ,i ~ ,i ,i ,i ,1 ,1 ,~ ,1 ,~ ,~ , ,~ ,~ ~ ,~ ,.. , m ~ P~ m P~ ~ Ia + + + + + + ~
W ,~ ,~ ,~ ,1 ~ ,, . a) Ql ~ ~ ~ ~ a~
;54~
~ s shown in Table 2, CIF-A at 1.9 x 10 M
reduced ~he amount of IgM produced by 33% and IgG by 16%
when compared with ~he nontreated control culture.
There was complete inhibition of IgM production in cultures containing either 1.9 x 10 M or 1.~ x ~ concentrations of CIF-~. Similar concentrations of CIF-~ resulted in a 54~ to 56%
inhibition of IgG production.
CIF-B was found to be comparable to CIF A As seen in Table 2, cultures containing 1.9 x 10 M
concentrations o~ CIF-B contained no IgM and only 54% of the IgG when compared with the untreated control cultures. Cultures trsated with 1.5 x 10 M
concentrations of CIF-B contained no measurable IgM and very little (8g~ inhibition) or no IgG. These results show that both CIF-A and CIF-B are extremely potent inhibitors of antibody production by plasma cells.
These in vitro T cell proliferation and B cell activation experiments suggest that lymphocyte regulation may be one mechanism involved in the in vivo lymphohistiocytic anti-inflammatory activity of CIF
observed previously. The results of these tests confirm the work reported by Kehrl, J.H.. et al, Clinical Research (1985) 610~.
6. In ~ivo Tests Usin~ CIF in Rodent ~rthritis Model Experimental collagen-induced arthritis (ECI~) can be induced in rats by intradermal injection of native type II collagen (bovine or rat) emulsified in incomplete Freund's adjuvant. The inbred Lewi6 rat strain, LEW ~RTl ), has been ~hown to develop pe~ipheral polyar~hriti~ within 14 to 30 days following immunization. Joint and ear cartilage develop a diffuse mononuclear cell infiltrate. Sensitized rats respond to -3~-in~radermal skin test challenge and develop circulating antibodies to native type II collagen.
Twelve LEW rats (12-15 weeks old) are divided into three groups o~ four animals each. Groups I and II
are sensitized to type II bovine collagen by intradermal injection of bovine type II in comple~e Freund's adjuvant at 2.5 ml/kg weight. Group III serve6 as a nonsensiti~ed control.
Ankle measurements and subjective gra~ing (0 to ~4) of arthritis based on the degree of inflammation and swelling of digits, feet and ankles are made prior to sensitization and regularly throughout the test. Ra~s in Group I exhibiting a significant inflammatory response are treated by injection of CIF (500 ng in 0.05 ml sterile PBS) directly into the joint on days 1, 3, 5, and 7 following the observed response. Rats of Grou~ II
showing such a response are treated similarly by injection of PBS without CIF.
Sera are collected from the rats pre-treatment and post-trea~ment and assayed for antibodies to type II
collagen using an ELIS~. The rats are given an intradermal skin test challenge at 3 days prior to sacrifice using 50 ~g of type II collagen in the abdomen. Erythema and induration are measured at 24, 4R, and 7~ hr post challenge. ~t 72 hr the challenge site is biopsied and examined histologically.
Rats are sacrificed 5 to 7 days after the final injection, exsanguinated, and their paws fixed in 10%
neutral formalin for histologic examination.
The results of these tests show that treatment with CIF reduces inflammation significantly compared to the nontreated con~rol group. The CIF-treated groups exhibit a reduced res~onse to a skin test challenge of type II collagen when compared with the nontreated ~Z~i5~4S
control group. Further, the treated group has significantly reduced antibody titers to ~ype II
collagen. These results sugge6t that administration of CIF into tha affected joints not only controls the inflammation locally, but acts as a systemic immuno-6upprassi~e agent for the treatment of arthritis.
Twelve LEW rats (12-15 weeks old) are divided into three groups o~ four animals each. Groups I and II
are sensitized to type II bovine collagen by intradermal injection of bovine type II in comple~e Freund's adjuvant at 2.5 ml/kg weight. Group III serve6 as a nonsensiti~ed control.
Ankle measurements and subjective gra~ing (0 to ~4) of arthritis based on the degree of inflammation and swelling of digits, feet and ankles are made prior to sensitization and regularly throughout the test. Ra~s in Group I exhibiting a significant inflammatory response are treated by injection of CIF (500 ng in 0.05 ml sterile PBS) directly into the joint on days 1, 3, 5, and 7 following the observed response. Rats of Grou~ II
showing such a response are treated similarly by injection of PBS without CIF.
Sera are collected from the rats pre-treatment and post-trea~ment and assayed for antibodies to type II
collagen using an ELIS~. The rats are given an intradermal skin test challenge at 3 days prior to sacrifice using 50 ~g of type II collagen in the abdomen. Erythema and induration are measured at 24, 4R, and 7~ hr post challenge. ~t 72 hr the challenge site is biopsied and examined histologically.
Rats are sacrificed 5 to 7 days after the final injection, exsanguinated, and their paws fixed in 10%
neutral formalin for histologic examination.
The results of these tests show that treatment with CIF reduces inflammation significantly compared to the nontreated con~rol group. The CIF-treated groups exhibit a reduced res~onse to a skin test challenge of type II collagen when compared with the nontreated ~Z~i5~4S
control group. Further, the treated group has significantly reduced antibody titers to ~ype II
collagen. These results sugge6t that administration of CIF into tha affected joints not only controls the inflammation locally, but acts as a systemic immuno-6upprassi~e agent for the treatment of arthritis.
Claims (9)
1. A composition for use in treating inflammation, which composition comprises a cartilage-inducing factor.
2. A composition for use in treating a dysfunction or malfunction of hematopoiesis or lymphopoiesis, which composition comprises a cartilage-inducing factor.
3. The composition of claims 1 or 2, wherein the cartilage-inducing factor is a homodimer whose chains each have:
(a) the following partial N-terminal amino acid sequence: Ala-Leu-Asp-Thr-Asn-Tyr-Cys-Phe-Ser-Ser-Thr-Glu-Lys-Asn-Cys-Cys-Val-Arg-Gln-Leu-Tyr-Ile-Asp-Phe-Arg-Lys-Asp-Leu-Gly-Trp-; or (b) the following partial N-terminal amino acid sequence: Ala-Leu-Asp-Ala-Ala-Tyr-Cys-Phe-Arg-Asn-Val-Glu-Asp-Asn-Cys-Cys-Leu-Arg-Pro-Leu-Tyr-Ile-Asp-Phe-Lys-Arg-Asp-Leu-Gly-Trp.
(a) the following partial N-terminal amino acid sequence: Ala-Leu-Asp-Thr-Asn-Tyr-Cys-Phe-Ser-Ser-Thr-Glu-Lys-Asn-Cys-Cys-Val-Arg-Gln-Leu-Tyr-Ile-Asp-Phe-Arg-Lys-Asp-Leu-Gly-Trp-; or (b) the following partial N-terminal amino acid sequence: Ala-Leu-Asp-Ala-Ala-Tyr-Cys-Phe-Arg-Asn-Val-Glu-Asp-Asn-Cys-Cys-Leu-Arg-Pro-Leu-Tyr-Ile-Asp-Phe-Lys-Arg-Asp-Leu-Gly-Trp.
4. The composition of claims 1 or 2, wherein the cartilage-inducing factor is a homodimer whose chains each have the amino acid sequence shown in Figure 1.
5. The composition of claims 1 or 2, wherein the cartilage-inducing factor is substantially free of activating agent or co-factor.
6. The composition of claim 1, wherein the cartilage-inducing factor is applied systemically.
7. The composition of claim 1, wherein the cartilage-inducing factor is applied locally.
8. The composition of claim 7, wherein the cartilage-inducing factor is applied as an implant in combination with a pharmaceutically acceptable carrier.
9. The composition of claim 8, wherein the carrier is a collagenous carrier.
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US76333785A | 1985-08-06 | 1985-08-06 | |
| US763,337 | 1985-08-06 | ||
| US836,672 | 1986-03-06 | ||
| US06/836,672 US4806523A (en) | 1985-08-06 | 1986-03-06 | Method of treating inflammation |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1265445A true CA1265445A (en) | 1990-02-06 |
Family
ID=27117266
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA000514887A Expired - Lifetime CA1265445A (en) | 1985-08-06 | 1986-07-29 | Composition for use in treating inflammation |
Country Status (7)
| Country | Link |
|---|---|
| US (2) | US4806523A (en) |
| EP (2) | EP0451439B1 (en) |
| JP (1) | JPH0798754B2 (en) |
| AT (2) | ATE135231T1 (en) |
| AU (1) | AU591513B2 (en) |
| CA (1) | CA1265445A (en) |
| DE (2) | DE3650499T2 (en) |
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|---|---|---|---|---|
| US7763257B2 (en) | 2004-12-09 | 2010-07-27 | Christina Juneau | Compositions comprising transforming growth factor (TGF)-β1 and TGF-β2 in admixture of proteins obtained from dairy products |
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| US3400199A (en) * | 1965-02-26 | 1968-09-03 | Leslie L. Balassa | Wound-healing cartilage powder |
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-
1986
- 1986-03-06 US US06/836,672 patent/US4806523A/en not_active Expired - Lifetime
- 1986-07-29 CA CA000514887A patent/CA1265445A/en not_active Expired - Lifetime
- 1986-08-04 DE DE3650499T patent/DE3650499T2/en not_active Expired - Fee Related
- 1986-08-04 DE DE8686306000T patent/DE3687099T2/en not_active Expired - Fee Related
- 1986-08-04 EP EP91100255A patent/EP0451439B1/en not_active Expired - Lifetime
- 1986-08-04 AT AT91100255T patent/ATE135231T1/en not_active IP Right Cessation
- 1986-08-04 EP EP86306000A patent/EP0213776B1/en not_active Expired - Lifetime
- 1986-08-04 AT AT86306000T patent/ATE82133T1/en not_active IP Right Cessation
- 1986-08-05 AU AU60875/86A patent/AU591513B2/en not_active Ceased
-
1988
- 1988-08-09 US US07/230,330 patent/US5008240A/en not_active Expired - Lifetime
-
1993
- 1993-12-28 JP JP5337499A patent/JPH0798754B2/en not_active Expired - Lifetime
Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US7763257B2 (en) | 2004-12-09 | 2010-07-27 | Christina Juneau | Compositions comprising transforming growth factor (TGF)-β1 and TGF-β2 in admixture of proteins obtained from dairy products |
Also Published As
| Publication number | Publication date |
|---|---|
| EP0213776A2 (en) | 1987-03-11 |
| ATE135231T1 (en) | 1996-03-15 |
| ATE82133T1 (en) | 1992-11-15 |
| JPH06228005A (en) | 1994-08-16 |
| DE3687099T2 (en) | 1993-03-18 |
| DE3687099D1 (en) | 1992-12-17 |
| EP0213776A3 (en) | 1989-05-03 |
| EP0451439A1 (en) | 1991-10-16 |
| US4806523A (en) | 1989-02-21 |
| DE3650499T2 (en) | 1996-07-25 |
| DE3650499D1 (en) | 1996-04-18 |
| AU591513B2 (en) | 1989-12-07 |
| EP0451439B1 (en) | 1996-03-13 |
| AU6087586A (en) | 1987-02-12 |
| US5008240A (en) | 1991-04-16 |
| JPH0798754B2 (en) | 1995-10-25 |
| EP0213776B1 (en) | 1992-11-11 |
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Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| MKLA | Lapsed |