CA2336900C - Filamentous porous films and methods for producing the same - Google Patents

Filamentous porous films and methods for producing the same Download PDF

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Publication number
CA2336900C
CA2336900C CA002336900A CA2336900A CA2336900C CA 2336900 C CA2336900 C CA 2336900C CA 002336900 A CA002336900 A CA 002336900A CA 2336900 A CA2336900 A CA 2336900A CA 2336900 C CA2336900 C CA 2336900C
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filamentous
filaments
porous film
film
thermoplastic polymer
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CA2336900A1 (en
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Richard L. Dunn
Deryl D. Swanbom
Michelle Botz
Kenneth C. Godowski
Scott Jeffers
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Tolmar Therapeutics Inc
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QLT USA Inc
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    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08JWORKING-UP; GENERAL PROCESSES OF COMPOUNDING; AFTER-TREATMENT NOT COVERED BY SUBCLASSES C08B, C08C, C08F, C08G or C08H
    • C08J5/00Manufacture of articles or shaped materials containing macromolecular substances
    • C08J5/18Manufacture of films or sheets

Abstract

The invention is directed to a filamentous porous film that can act as a support for cellular attachment, growth and organization. The film is formed from filaments which define a matrix structure with pores.

Description

Filamentous Porous Films and Methods for Producing the Same Background of the Invention Significant benefits can be derived from the ability to grow cells in vitro on biodegradable supports or scaffolds followed by transplantation to a human needing cells for tissue repair or replacement. Cells that could be grown for such tissue engineering include osteoblasts for new bone, chondrocytes for cartilage, fibroblasts for dermal tissue and retinal pigment epithelial cells (RPE) for the eye.

Some research regarding this aspect of tissue engineering has already been reported. For example, Mikos et al. have prepared poly(glycolic acid) bonded fiber structures for cell attachment and transplantation. J. of Biomedical Materials Research, Vol. 27, 183 - 189 (1993). Their preparations involved formation of a composite material between poly(glycolic acid) nonwoven fiber meshes and poly(L-lactic acid) (PLLA) followed by then:nal treatment and selective dissolution of the PLLA matrix. Others have investigated porous sheets of polymer for such cell growth. Although the growth of cells on such porous film has been demonstrated, there are difficulties with such an approach.

The task of tissue engineering is complicated by the need of most cells to have special surfaces for attachment, proliferation and cell interactions.
Additionally, some cells have distinctly different basal and apical characteristics and are polar in nature so that they function properly only when they are properly oriented.
There is a need, therefore, for a technique to develop and grow cells in vitro in a manner such that they will function properly when implanted. To this end, biodegradable polymers are needed to act as a scaffold or support for the development and growth of such cells. The scaffold should allow the growing cells to organize and develop special cellular function such as cell attachment, proliferation and maintenance of distinct basal and apical characteristics.
Summary of the Invention These needs are met by the present invention which provides a biodegradable scaffold for in vitro cell cultures, and a process for preparation of that scaffold. In particular, the biodegradable scaffold provides a suitable support for organization, proper attachment and growth of cells, especially those with special cellular functions.

In general, the invention is directed to the biodegradable scaffold which is composed of a filamentous porous thin film. The invention as well is directed to a process for preparing the filamentous porous film, and a method of using the filamentous porous film to provide a scaffold for cell growth and tissue engineering.
The filamentous, porous film can act as a support for cells to attach, grow and organize, including those with special functions and those requiring spatial orientation. The film has a matrix structure with two surfaces and is constructed primarily of filaments. The filaments define pores in the matrix structure.
The pores extend from one surface to the other surface without a substantial change in the cross sectional dimensions of the pores. The filaments are composed of a pharmaceutically acceptable, biodegradable, thermoplastic polymer that is substantially soluble in a pharmaceutically acceptable organic solvent and substantially insoluble in aqueous medium and body fluid.

The process of the invention is carried out by applying liquid filaments of a flowable thermoplastic polymer solution onto an aqueous medium in such a manner that a solid filamentous porous film forms. By controlling the viscosity of the polymer solution and applying the polymer solution by any technique that forms droplets or small multiple volumes of the solution, the elongated small multiple volumes of solution, i.e., liquid filaments, can be formed which will result in the formation of a solid filamentous, porous film rather than a smooth, nonporous sheet.

The method of using the filamentous, porous film according to the invention involves use of the film as a scaffold for cell growth in a cell culture method.
Brief Description of the Drawings Figures 1 through 9 depict scanning electron micrographs of films.
Figures 1 through 3, 8 and 9 illustrate films of the invention.
Figures 4 through 7 illustrate other kinds of films.

Detailed Description of the Invention The filamentous, porous, biodegradable film of the invention provides a scaffold which can act as a support for proper attachment, growth, and organization of cells including those with special functions and/or those requiring spatial orientation. The film is formed of filaments of a pharmaceutically acceptable biodegradable thermoplastic polymer. The filaments are arranged into a matrix, the interfilament spaces of which constitute pores. These pores are substantially uniformly distributed throughout the entire film including its upper and lower surfaces. The matrix arrangement of the filaments forming the film and the pores of the film are effective for allowing and promoting growth of cells, including those for which a special cellular function is preserved. The film of the invention provides a suitable biodegradable scaffold for cell implantation.

The process for forming the filamentous, porous film according to the invention enables the construction of filaments and their arrangement into the matrix constituting the film of the invention. The process involves applying liquid filaments of a flowable composition onto an aqueous medium to form the solid filaments. The density and arrangement of filaments provide the matrix structure of the film.

The flowable composition is a solution or dispersion of a pharmaceutically acceptable biodegradable thermoplastic polymer in a pharmaceutically acceptable organic solvent. The biodegradable thermoplastic polymer is substantially insoluble in an aqueous medium and body fluid. The organic solvent is slightly to completely soluble in aqueous medium.
The flowable composition is converted into liquid filaments by any process that is capable of converting the flowable composition into small multiple, separate volumes of solution or dispersion. These methods include, for example, spraying, misting, showering, drizzling, squirting, atomizing or aerosolizing. The preferred method of liquid filament formation is aerosolizing. The liquid filaments are applied onto the surface of an aqueous medium, preferably an aqueous medium having a high surface tension so that the liquid filaments rest upon its surface. The liquid filaments of flowable composition on the surface of the aqueous medium transform into solid filaments and the filaments are arranged to provide the matrix constituting the filamentous film.

While not intended as a limitation of the invention, it is believed that under ordinary circumstances, the contact of droplets of the flowable composition with an aqueous surface would form either a sheet or particles rather than filaments, However, by controlling the viscosity of the flowable composition, liquid filaments are formed and transform into solid filaments instead of a sheet or particles.
Although the actual mechanism of this surprising result is not fully understood, the multiple small volumes of flowable composition are formed into liquid filaments during the application process when the viscosity of the flowable composition is within a certain range. These liquid filaments impact the aqueous surface and coagulate to form the overlapping solid filaments of the porous film.
Definitions The term "biodegradable" means that the substance having this characteristic, such as the thermoplastic polymer, will degrade over time by the action of enzymes, by hydrolytic action and/or by other similar mechanisms and includes such characteristics as bioerodable and bioabsorbable.

The term "bioerodible," means that the substance having this characteristic, such as the matrix, will erode or degrade at its surfaces over time due, at least in part, to contact with substances found in the surrounding tissue fluids or cellular action.

The term "bioabsorbable," means that the substance having this characteristic, such as thermoplastic polymer matrix, will be broken down and absorbed within the living body, for example, by a cell or tissue.

The terms "biocompatible" and "pharmaceutically acceptable" mean that the 5 substance having these characteristics, such as the thermoplastic polymer, the solvent and the resulting filamentous porous film, will not cause substantial tissue irritation or necrosis at the implant site.

The term "flowable" means that the substance having this characteristic, such as the thermoplastic polymer solution, is manipulatable, may be transported through an orifice and is incapable of maintaining a definite shape. Flowable includes formulations with a low viscosity or water-like consistency to those with a high viscosity, such as a paste-like material. Advantageously, the flowability of the thermoplastic polymer formulation allows it to conform to irregularities, crevices, cracks, and/or holes on the aqueous medium.

"Special cellular function" means cell functions such as cell attachment, cell proliferation, and maintenance of cell differentiation.

The term "liquid filament" means a non-spherical, string-like or elongated volume of liquid material. The length may become much greater than the width when the viscosity of the flowable composition is sufficiently high or otherwise within a certain range.

"Applying liquid filaments" means using any method of producing liquid filaments such as spraying, misting, showering, drizzling, squirting, atomizing or aerosolizing.

Thermoplastic polymer Thermoplastic polymers useful in this invention include thermoplastic polymers that are biodegradable. The thermoplastic polymers are substantially insoluble in an aqueous or body fluid medium but are capable of substantially dissolving in a water-soluble carrier, or solvent, to form the flowable composition.

Upon contact between the flowable composition and an aqueous medium, the thermoplastic polymer component in the flowable composition will coagulate or precipitate to form a solid material, and the solvent component will dissipate into the aquoous medium. Flowable compositions with these characteristics have generally been described in US Patent No's_ 4,938,763; 5,077,049; 5,324,519; 5,632,727;
5,599,552; 5,702,716; 5,487,897; 5,660,849;5,278,201; 5,198220; 5,447,725 and 5,242,910.

Thermoplastic polymers that are suitable for use in the therrnoplastic polymer solution generally include any having the foregoing charactenstics.
Suitable therrnoplastic polymers include those with repeating functional group units in the polymer backbone, including but not limited to such functional group units as ester (including those formed from hydroxycarboxylic acids and those forrned from polycarboxylic acids and polyols), amide (including those formed from aminocarboxylic acids and those formed from polycarboxylic acids and polyamines), urethane, carbonate, anhydride, esteraxnide, dioxanone, acetal, ketal, and phosphazene. Structural classes of such polymers are disclosed in US
Patent No's 4,938,763; 5,077,049; 5,324,519; 5,632,727; 5,599,552; 5,702,716;
5,487,897;
5,660,849;5,278,201; 5,198220; 5,447,725 and 5,242,910.

Preferred thermoplastic polymers have repeating ester units within their backbones. Especially preferred thermoplastic polymers are those formed from such monorneric units as lactide, glycolide, caprolactone, hydroxbutyrate, C2 to C6 diol ester with a dicarboxylate selected from oxalate, malonate or succinate, and any combination thereof as a copolymer or terpolymer with random, ordered or block distribution of the various rnonomeric units_ The Brookfield relative viscosity measurement of the flowable composition indicates the concentration of thermoplastic polymer, the interaction between the thennoplastic polymer and solvent and the molocular weight of the thermoplastic polymer itself. The relative viscosity of the flowable composition determines how readily or how slowly it will flow. The relative viscosity also determines whether the flowable composition will form spherical droplets which coalesce into particles or sheets, or elongated droplets (liquid filaments) which coalesce irrto solid filaments. In general, the Brookl'ield relative viscosity of the flowable composition will range from about 1,000 to about 90,000 centipoise (cps) and preferably from 1,000 to about 10,000 cps in order to form the filarnentous film of the invention.
Organic Solvent Suitable organic solvents for use in the flowable composition are those which are pharmaceutically acceptable and will at least partially dissolve the thermoplastic polymer. According to the invention, the solvent has a solubility in aqueous medium, ranging from moderately soluble to completely miscible and is capable of diffusing into an aqueous medium such as water, hydrogel, agar and the like.
Classes of pharmaceutically acceptable organic solvents suitable for the present invention include aliphatic and alicyclic alcohols and polyols, aliphatic, alicyclic and aromatic esters, aliphatic and alicyclic lactams, aliphatic and alicyclic lactones, aliphatic and alicyclic amides, aliphatic and alicyclic carbonates, aliphatic and alicyclic acids, aliphabc and alicyclic ethers, aliphatic and alicyclic sulfoxides and sulfones, heterocyclic compounds, and aliphatic and alicyclic ketones_ Examples of such organic solvents include those disclosed in US Patent No's_ 4,938,763; 5,077,049; 5,324,519; 5,632,727; 5,599,552; 5,702,716; 5,487,897;
5,660,849;5,278,201; 5,198220; 5,447,725 and 5,242,910.

Specific examples include N-methyl-2-pyrtolidone (NMP), 2-pyrrolidone, propyleme carbonate, ethylene carbonate, dimethyl carbonate, acetic acid, lactic acid, heptanoic acid, 2-etboxyethyl acetate, ethyl acetate, methyl acetate, ethyl lactate, ethyl butyrate, diethyl malonate, diethyl glutonate, tributyl citrate, diethyl succinate, tri6utyrin, isopropyl myristate, dimethyl adipate, dmiethyl succinate, dimethyl oxalate, dimethyl citrate, triethyl citrate, acetyl tributyl citrate, glyceryl triacetate, acetone, methyl ethyl ketone, 2-Ethoxyethanol, ethylene glycol dimethyl ether, glycofurol, glycerol fozmal, 1,3 butyleueglycol, isopropylidene glycol (2,2-dimethyl-1,3-dioxolone4-methanol; Solketal, dimethylforniarnide, dimethylacetam.ide; dimethyisulfoxide (DMSO), dimethylsulfone, tetrahydrofinan, M-caprolactone, butyrolactone, caprolactam, such as N,lv-dimethyl-:n-toluamide, and 1-dodecylazacycloheptan-2-one and any mixture of two or rnore of the organic solvents.
The choice of solvent will also depend upon its rate of evaporation and the rate at which it promotes coagulation of thermoplastic polymer from the flowable composition. The rate of evaporation will affect the polymer concentration in the liquid filaments and will change the physical form of coagulation if the polymer concentration changes dramatically. Generally, the organic solvent is chosen so that minimal evaporation occurs during the liquid filament formation and transition to solid filaments. The rate of promotion of coagulation will depend upon the solubility of the organic solvent in water. The highly soluble solvents promote a rapid rate of coagulation while the slightly soluble solvents promote a slow rate of coagulation. Generally, the rate of coagulation will be moderate so that filament formation can occur.

The concentration of thermoplastic polymer in the flowable composition also affects the ability to form filaments. Generally, this concentration may range from about 0.01 gram of thermoplastic polymer per ml of solvent to an about saturated concentration, preferably from about 0.1 gram per ml to an about 2.0 gram per ml., more preferably from about 0.1 gram per ml to an about 0.7 gram per ml.
Formation of Filamentous Porous Film In general, the filamentous porous film of the invention is formed by contacting the flowable composition with an aqueous medium. The flowable composition can be applied to the aqueous medium by any technique that converts the flowable composition into liquid filaments. For example, the flowable composition can be applied by spraying, misting, showering, drizzling, squirting, atomizing or aerosolizing. Aerosolization is a preferred method of administration because it minimizes the amount of flowable composition applied to the aqueous medium while maximizing uniformity and pore size. Typically, the flowable composition is placed in the reservoir of an atomizer or spray gun and aerosolized by inert gas pressure. The aerosol flow is directed toward the aqueous medium which it contacts and forms liquid filaments on the surface of the aqueous medium. The aqueous medium preferably has a high surface tension, high density and/or high viscosity so that the liquid filaments of flowable composition do not sink into the medium but rest upon its surface. Upon application of the liquid filaments to the aqueous medium, the liquid filaments convert into solid filaments as the thermoplastic polymer coagulates to a solid. The result is that the coagulating polymer adopts a filament form as a solid. The filamentous porous film generally has a thickness of about 10 m to about 100 m, more preferably from about 20 m to about 50 m.

Structure of the Filamentous Porous Film The matrix structure of the filamentous porous film defines pores which are a minimum of about 1 m in size. The pores also range in size from about 1 m to about 30 m, preferably from 5 to 10 m. The filaments diameters are about 0.01-4 m, preferably 0.1 to 2 m and lengths of about 1 to 240 m, preferably 1 to m. The pores are large enough to permit cells to attach and grow within the pores and the filamentous character of the film permits the nutrient medium to diffuse to and bathe all surfaces of the cell rather than only a portion such as the basal or apical portion.

The matrix structure of the film of the invention has two surfaces with the pores extending substantially uniformly throughout the matrix structure and from one surface to the other. Thus, the pores of the matrix structure communicate through the surfaces. Generally the filamentous porous film will have a porosity in the range of about 20% to about 90% throughout the entire matrix structure, preferably about 60% to 90%.

Use of the Filamentous Porous Film The filamentous porous film can be used as a scaffold to allow cell growth and tissue engineering such as cell attachment, cell proliferation and maintenance of differentiated cellular function. For example the filamentous, porous film may be used as a scaffold for culturing oriented cells such as RPE cells or osteoblast cells.
The filamentous, porous film used as such a scaffold has filament dimensions of 0.1 - 2 microns in diameter and 1 to 100 microns in length and the film has a porosity of 60 to 80 % with pore sizes of 5 to 10 microns.

In use, the film is combined with a nutrient medium such as Dulbecco's minimum essential medium and the specialized cells transferred from living tissue to 5 the film. Incubating the cell culture will allow the cells to attach, grow and multiply into the pores of interfilament spaces of the entire film. This construct of the filamentous porous film and specialized cells can be used for cellular transplant into patients. The construct will facilitate correct implantation and possibly correct orientation of the specialized cells. As degradation of the thermoplastic polymer 10 proceeds, regenerated specialized cells with a proper function, and possibly a correct orientation will be established such that cellular interactions dependent upon the cellular functions and possibly the orientation will be re-established.

The invention has been described with reference to various specific and preferred embodiments and techniques. However, it should be understood that many variations and modifications may be made while remaining within the spirit and scope of the invention.

Examples Example 1 Formation of Flowable Thermoplastic polymer Solution A thermoplastic copolymer poly(DL-lactide-co-glycolide) (PLG) with 50 mol % of the polymer being glycolide was dissolved in N-methyl-2-pyrrolidone (NMP). The copolymer, with an intrinsic viscosity (IV) of 1.03 dl/g, can be purchased from Birmingham Polymers, Inc. (BPI). The copolymer solution, prepared by placing 20 g of the copolymer and 80 g of NMP in a glass jar, was initially mixed with a spatula or wooden stick. The nitrogen-purged jar was kept at room temperature for one hour and then placed in a room temperature shaker.
The contents were shaken until all the polymer was in solution (generally 24 to 48 hours).

Examples 2-12:

Additional copolymers of PLG, poly(DL-lactide-co-glycolide) with acid end groups (PLG-H) and poly(DL-lactide-caprolactone) (PLC) were dissolved in NMP
using the same procedure described in example 1. The copolymer manufacturers were either Birmingham Polymers, Inc. (BPI) or Boehinger Ingelheim (BI). The compositions, intrinsic viscosities, manufacturers and solution concentrations are summarized in Table 1.

Table 1: Summary of Flowable Compositions (Examples I - 12) Exa[nple Copolymer Copolymer Intrinsic Manufacturer wt %
Ratio Viscosity 1 PLG 50/50 1.03 dL/g BPI 20 2 PLG 50/50 0.7 dL/g BPI 20 3 PLG 50/50 0.26 dL/g BPI 20 4 PLG 75/25 1.08 dL/g BPI 20 5 PLG 75/25 0.72 dL/g BPI 20 6 PLG 75/25 0.31 dL/g BPI 20 7 PLC 75/25 0.74 dL/g BPI 20 8 PLG 65/35 1.02 dL/g BPI 20 9 PLG 65/35 0.65 dL/g BPI 20 PLG 65/35 0.36 dL/g BPI 20 11 PLG-H 50/50 0.4 dL/g BI 30 12 PLG-H 50/50 0.4 dL/g BI 20 10 Example 13:

A film was prepared from the flowable composition in Example 1. The aerosol applicator (Air Brush, Badger Model 150) was connected to the propellant source (nitrogen gas) and cleaned for approximately 15 to 30 seconds by spraying acetone through the unit. Following complete removal of any acetone residue, a 1 cc vial containing the polymer formulation was attached to the applicator. The aerosol unit was activated over a sterile purified agar plate. The unit was held approximately 3 to 6 inches from the plate to avoid blowing the film from the agar plate and moved in a circular motion to ensure even coverage.

The aerosol unit was deactivated after 15 seconds. The activation time, which determines the film thickness, is based on the appearance of the film.
That is, the surface will appear matted or flat when the thickness is about 50 m but glossy when the thickness is greater than approximately 70 m.

The agar plate was filled with approximately 25 ml of sterile water with a pipette to float the film above the agar surface and then rotated to allow water to flow underneath the film. To remove the film from the agar plate, a piece of Teflon was placed underneath the film with the assistance of sterile forceps. The Teflon piece and the film were transferred to a petri dish. Approximately 25 ml of sterile water was added to the petri dish allowing the removal of the Teflon piece.
After 15 minutes, the rinse water was removed and the film was washed with an additiona125 ml of sterile water. A Teflon piece was placed underneath the film for removal from the petri dish. The film was dried overnight on the Teflon piece in a laminar flow hood.

The film was cut into smaller pieces (approximately 10 X 10 mm) and placed into a ATRISORB case housing and placed into a nitrogen purged pouch. The film pieces were sterilized using gamma irradiation at 14 kGy +/- 10%. This corresponds to a 10-6 sterility assurance level (SAL) with a bioburden level of approximately 1 CFU per film.

The film thickness, measured with digital calipers, varied from 35 to 60 m (43 m average) before irradiation and from 25 to 50 m (35 m average) after irradiation. The overall handling characteristics of the film was very good.
Example 13 - 24:

Additional films were prepared from flowable compositions prepared in examples 2 - 12 using the procedure described for example 13. Table 2 contains a summary of the film characteristics.

Table 2: Summary of Film Characteristics Exam le Flowable Volume Spray Thickness Thickness Overall Handling Com~osition used, Time, re- after Characteristics EI sec irradiation, Irradiation, Wai Am~
13 Ex. 1 50 15 43 35 very good 14 Ex.2 100 10-15 37 33 good; cracking Ex. 3 75 5-10 10 not measured not good ; very flaky 16 Ex. 4 25 15-20 28 34 good / fair; sticky 17 Ex. 5 25 not 35 53 fair; some stickiness timed 18 Ex. 6 50 not 31 35 not good; cracking timed 19 Ex. 7 50 not not measured not measured not good; sticky timed Ex. 8 25 not 28 19 fair; very thin and timed sticky 21 Ex. 9 50 not 45 28 not good; very brittle timed 22 Ex. 10 100 not 25 not measured not good; stuck to timed plate and fell apart 23 Ex. 11 25 not 29 not measured good; some timed stickiness 24 Ex. 12 50 not 31 25 fair; brittle timed 'Average Examples 25 - 46:

Flowable compositions of PLG, (PLG-H) and poly(DL-lactide) (PLA) were 10 prepared as described in example 1. The polymer compositions, inherent viscosities, manufacturers and solution concentrations are summarized in Table 3.

Table 3: Summary of Flowable Compositions (Examples 25 -46) Example Polymer Copolymer Intrinsic Manufacturer wt %
Ratio Viscosity 25 PLG 50/50 1.03 dL/g BPI 10 26 PLG 50/50 1.03 dL/g BPI 20 27 PLG 50/50 1.03 dL/g BPI 30 28 PLG 50/50 0.26 dL/g BPI 10 29 PLG 50/50 0.26 dL/g BPI 20 30 PLG 50/50 0.26 dL/g BPI 30 31 PLG 75/25 0.31 dL/g BPI 10 32 PLG 75/25 0.31 dL/g BPI 20 33 PLG 75/25 0.31 dL/g BPI 30 34 PLG 75/25 1.08 dL/g BPI 10 35 PLG 75/25 1.08 dL/g BPI 20 36 PLG 75/25 1.08 dL/g BPI 30 37 PLGH 50/50 0.48 dL/g BI 10 38 PLGH 50/50 0.48 dL/g BI 20 39 PLGH 50/50 0.48 dL/g BI 30 40 PLGH 50/50 0.48 dL/g BI 40 41 PLA - 0.33 dL/g BPI 10 42 PLA - 0.33 dL/g BPI 20 43 PLA - 0.33 dL/g BPI 30 44 PLA - 0.83 dL/g BPI 10 45 PLA - 0.83 dL/g BPI 20 46 PLA - 0.83 dL/g BPI 30 Examples 47- 68:

Films were prepared from the flowable compositions prepared in examples 25 - 46. The aerosol applicator (Air Brush, Badger Model 150) was connected to the propellant source (nitrogen gas) and cleaned for approximately 15 to 30 seconds by spraying acetone through the unit. Following complete removal of any acetone residue, a 3 cc vial containing the polymer formulation was attached to the applicator. The aerosol unit was activated over a sterile purified agar plate.
The unit was held approximately 3 to 6 inches from the plate to avoid blowing the film from the agar plate and a circular motion was used to ensure an even coverage.

The agar plate was filled with approximately 25 ml of sterile water with a pipette to float the fihn above the agar surface and then rotated to allow water to 5 flow underneath the film. To remove the film from the agar plate, a piece of Teflon was placed underneath the film with the assistance of sterile forceps. The Teflon piece and the film were transferred to a petri dish. Approximately 25 ml of sterile water was added to the petri dish allowing the removal of the Teflon piece.
After 15 minutes, the rinse water was removed and the film was washed with an additiona125 10 ml of sterile water. A Teflon piece was placed underneath the film for removal from the petri dish. The film was dried overnight on the Teflon piece in a laminar flow hood.

Pieces of the film were placed in vials, frozen at -86 C for approximately one hour, and lyophilized overnight to completely dry the films. The thickness was 15 measure using digital calipers. The film was then mounted and coated with gold for viewing by scanning electron microscopy (SEM). The structure of the film was characterized and reported in Table 4.

The Brookfield relative viscosity was measured for each flowable composition.

Table 4: Characterization of Films (Examples 47 - 68) Example Flowable Thickness, Brookfield Structure Characteristics Composition Bm Relative Viscosity, cps 47 Ex. 25 90 112 plate like material with foam like porous structure 48 Ex. 26 150 1,176 filament structure with bead like masses 49 Ex. 27 310 72,160 broad filaments that melt together 50 Ex. 28 310 24 solid surface; no filaments 51 Ex. 29 170 40 plate like material with foam like porous structure 52 Ex. 30 190 88 plate like material with foam like porous structure Exam le Flowable Thickness, Brookfield Structure Characteristics Composition Bm Relative Viscosity, cps 53 Ex. 31 not 16 solid smooth surface; see measured Figure 7 (2020X) 54 Ex. 32 130 64 plate like structures 55 Ex. 33 150 248 plate like structures with early stages of filament formation;
see Figure 6 (2020X) 56 Ex. 34 230 360 plates with some underlying filaments 57 Ex. 35 210 8,526 filament structure; starting to merge together; see Figure 8 (2020X) 58 Ex. 36 430 86,880 thick network with smaller rough and rigid filaments; tree like 59 Ex. 37 200 24 foam like structure with plate formation 60 Ex. 38 140 280 flat surface with sporadic pores; beginnings of filament formation 61 Ex. 39 1709 2696 filaments with round sphere like masses 62 Ex. 40 70 19,840 thick broad filaments laying over one another; see Figure 9 (2020X) 63 Ex. 41 130 16 very small spheres in a porous structure; foam core 64 Ex. 42 110 48 flat plate formation 65 Ex. 43 200 192 flat plates melting into a solid structure 66 Ex. 44 80 80 large pores; foam structure with plate like structure 67 Ex. 45 70 1,304 filaments laying on top of each other; melting and branching characteristics 68 Ex. 46 50 15,110 thick broad filaments with some melting together Examples 69 - 77:

Films from examples 13 -23 were evaluated for in vitro growth of human osteoblast cells. Osteoblasts were allowed to grow for three weeks in cell growth medium RPMI 1640 with 10% fetal calf serum and 2 mM glutamine. The film clinical handling characteristics as well as osteoblast attachment and growth were evaluated. The results are summarized in Table 5.

Table 5: Osteoblast Cell Growth on Films:
Film Handling (Examples 69 - 77) Example Film Sticking Sticking Curlin Curlin Before After Before After Hydration Hydration Hydration Hydration 69 Ex. 13 slight moderate slight slight 70 Ex. 14 moderate moderate none moderate 71 Ex. 16 moderate moderate slight moderate 72 Ex. 17 none none moderate severe 73 Ex. 18 moderate moderate none -74 Ex. 20 slight none moderate severe 75 Ex. 21 moderate severe slight slight 76 Ex.22 slight moderate slight slight 77 Ex.23 slight severe moderate moderate Table 6: Osteoblast Cell Growth on Films:
Growth Results (Examples 69 - 77) Example Film Overall Cell Nodule Cells Good Cell Overall Cell Growth on Present Inside Growth Evaluation Growth Both Sides Film Around of Film Film 69 Ex. 13 10+ yes yes yes yes very good 70 Ex. 14 7-8+ yes yes yes yes good / fair 71 Ex. 16 5+ ND no ND yes good 72 Ex. 17 3+ ND no ND no fair 73 Ex. 18 5+ ND no ND no fair / poor 74 Ex.20 3+ ND no ND no fair 75 Ex. 21 6+ yes no yes yes fair 76 Ex. 22 5+ ND no ND yes fair 77 Ex. 23 9-10+ yes yes yes yes very good Examples 78-86:

Films from examples 13 -23 were evaluated for in vitro growth of Human Fetal Retinal Pigment Epithelial Spheroids (HFRPE). Sheets of HFRPE cells were isolated and loosely attached to the films in the presence of Dulbecco's minimum essential medium. Within 48 to 72 hours, the cells attached themselves firmly to the polymer films. The HFRPE cells proliferated and covered each piece of film tested.
The cells did not dedifferentiate, an important indication that the films provide a suitable attachment structure. They possessed a cuboidal morphology with numerous apical microvilli. The HFRPE cells produced extracellular matrix (collagen type IV) at their basal side, filling the pores of the film. All the isolated cells were pigmented and expressed cytokeratine. In vivo, the transplanted films degraded within 2-3 weeks without any signs of inflammation in rabbit eyes.

Table 7: HFRPE Cell Growth on Films Film Handling (Examples 78 - 86) Examp Film Sticking Sticking Curling Curling le Before After Before After Hydration Hydration Hydration Hydration 78 Ex. 13 slight slight none slight 79 Ex. 14 very slight very slight none none 80 Ex. 16 slight very slight very slight very slight 81 Ex. 17 slight very slight none slight 82 Ex. 18 none very slight none none 83 Ex. 20 very slight none none none 84 Ex. 21 none none none slight 85 Ex. 22 slight very slight none very slight 86 Ex. 23 very slight very slight very slight very slight Table 8: HFRPE Cell Growth on Films Growth Results (Examples 79 - 86) Example Film Cell Cell Overall Adhesion Proliferation Evaluation on Plate 78 Ex. 13 yes yes very best 79 Ex. 14 could not could not brittle manipulate manipulate 80 Ex. 16 could not could not brittle manipulate manipulate 81 Ex. 17 yes yes not given 82 Ex. 18 could not could not brittle manipulate manipulate 83 Ex. 20 yes yes not given 84 Ex. 21 yes yes not given 85 Ex. 22 yes yes not given 86 Ex. 23 yes no not given Example 87: SEM Photos Films prepared as examples 13, 15, 18 and 23 were place in vials, frozen at -86 C for approximately one hour, and lyophilized overnight to completely dry the films. The thickness was measured using digital calipers. The films were then mounted and coated with gold for viewing by scanning electron microscopy (SEM).
The structure of each film was characterized.

The film from example 13 can be seen in Figure 1(2020X) and Figure 2(cross-section, 2100X). The film is composed of many filaments of varying widths that weave together to form a mesh-like matrix. The film from example 23 can be seen in Figure 3(2020X). Again, the example 23 film is composed of filaments forming a mesh-like matrix. Example 23 appears to have larger filaments than example 13. Both films have void spaces between the filaments larger than 10 m, an optimal size for cells to attach and proliferate.

The film from example 15 can be seen in Figure 4(1010X). This film was too brittle for cell growth experiment and appears porous on one side but non-porous on the opposite side. The film from example 18 can be seen in Figure 5 (2020X).
This film had a predominately smooth, plate-like surface and some very small pores.

5 Neither example 15 nor 18 had pores that extending from one side of the polymer to the other side. Likewise, neither film was filamentous.

Claims (23)

What is claimed is:
1. A process for preparing a filamentous porous film, comprising:
applying liquid filaments of a flowable composition onto an aqueous medium to form a matrix structure of filaments, wherein the flowable composition comprises a pharmaceutically acceptable, biodegradable thermoplastic polymer that is substantially insoluble in an aqueous or body fluid medium, dissolved or dispersed in a pharmaceutically acceptable organic solvent that is moderately soluble to completely miscible in the aqueous or body fluid medium.
2. A process of claim 1, wherein the concentration of thermoplastic polymer is about 10 to 50 wt. % in the organic solvent.
3. The process of claim 1, wherein the thermoplastic polymer is bioerodible.
4. A process of claim 1, wherein the thermoplastic polymer contains repeating functional group units in its polymer backbone, which are selected from hydroxycarboxylic acid ester, polycarboxylic acid and polyol ester, aminocarboxylic acid amide, polycarboxylic acid and polyamine amide, urethane, carbonate, anhydride, esteramide, dioxanone, acetal, ketal, phosphazene and any combination thereof.
5. A process of claim 4, wherein the thermoplastic polymer is formed from at least one monomeric unit selected from the group consisting of lactide, glycolide, caprolactone, hydroxbutyrate, and C2 to C6 diol ester with a dicarboxylate selected from oxylate, malonate and succinate, and any combination thereof as a copolymer or terpolymer with random, ordered or block distribution of the various monomeric units.
6. A process of claim 5, wherein the thermoplastic polymer is poly(DL-lactide-co-glycolide).
7. A process of claim 1, wherein the organic solvent is selected from the group consisting of aliphatic and alicyclic alcohols and polyols, aliphatic, alicyclic and aromatic esters, aliphatic and alicyclic lactams, aliphatic and alicyclic lactones, aliphatic and alicyclic amides, aliphatic and alicyclic carbonates, aliphatic and alicyclic acids, aliphatic and alicyclic ethers, aliphatic and alicyclic sulfoxides and sulfones, heterocyclic compounds, and aliphatic and alicyclic ketones.
8. A process of claim 7, wherein the organic solvent is N-methyl-2-pyrrolidone.
9. A process of claim 1, wherein the flowable composition has a viscosity which effectively allows for formation of liquid filaments.
10. A process of claim 9, wherein the flowable composition has a Brookfield relative viscosity of about 1,000 to 90,000 centipoise.
11. The process of claim 1, wherein the step of applying the liquid filaments of flowable composition comprises spraying, misting, showering, drizzling, squirting, atomizing or aerosolizing the flowable composition.
12. The process of claim 11, wherein the step of applying the liquid filaments of flowable composition comprises aerosolizing the flowable composition.
13. The process of claim 1, wherein the aqueous medium is a hydrogel.
14. The process of claim 13, wherein the hydrogel is agar.
15. A filamentous, porous film, comprising: a matrix structure of filaments, interfilament spaces and two surfaces; wherein the interfilament spaces define pores extending from one surface to the other, the pores have cross sectional dimensions which do not substantially change from one surface to the other, and the filaments comprise a pharmaceutically acceptable biodegradable thermoplastic polymer that is substantially insoluble in aqueous fluid or body fluid.
16. The filamentous porous film of claim 15, wherein the thermoplastic polymer contains repeating functional group units in its polymer backbone, which are selected from hydroxycarboxylic acid ester, polycarboxylic acid and polyol ester, aminocarboxylic acid amide, polycarboxylic acid and polyamine amide, urethane, carbonate, anhydride, esteramide, dioxanone, acetal, ketal, phosphazene and any combination thereof.
17. The filamentous porous film of claim 16, wherein the thermoplastic polymer is formed from at least one monomeric unit selected from the group consisting of lactide, glycolide, caprolactone, hydroxbutyrate , C2 to C6 diol ester with a dicarboxylate selected from oxalate, malonate and succinate, and any combination thereof as a copolymer or terpolymer with random, ordered or block distribution of the various monomeric units.
18. A filamentous porous film of claim 17, wherein the thermoplastic polymer is poly(DL-lactide-co-glycolide).
19. A filamentous, porous film of claim 15, wherein the filaments have diameters of about 0.01 to about 4 µm.
20. A filamentous, porous film of claim 15, wherein the filaments have lengths of about 1 to about 240 µm.
21. A filamentous, porous film of claim 15, wherein the filamentous porous film has a thickness of about 10 to about 100 µm.
22. A filamentous, porous film of claim 21, wherein the filamentous porous film has a thickness of about 20 to about 50 µm .
23. A filamentous porous film of claim 15, wherein the pores have a cross-sectional dimension of about 5 to about 30 µm.
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