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US2598608A - Preparation of collagenous materials - Google Patents

Preparation of collagenous materials Download PDF

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US2598608A
US2598608A US676076A US67607646A US2598608A US 2598608 A US2598608 A US 2598608A US 676076 A US676076 A US 676076A US 67607646 A US67607646 A US 67607646A US 2598608 A US2598608 A US 2598608A
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collagen
gel
filaments
sol
fibrils
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US676076A
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Torsti P Salo
David F Waugh
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Research Corp
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    • DTEXTILES; PAPER
    • D01NATURAL OR MAN-MADE THREADS OR FIBRES; SPINNING
    • D01FCHEMICAL FEATURES IN THE MANUFACTURE OF ARTIFICIAL FILAMENTS, THREADS, FIBRES, BRISTLES OR RIBBONS; APPARATUS SPECIALLY ADAPTED FOR THE MANUFACTURE OF CARBON FILAMENTS
    • D01F4/00Monocomponent artificial filaments or the like of proteins; Manufacture thereof
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L15/00Chemical aspects of, or use of materials for, bandages, dressings or absorbent pads
    • A61L15/16Bandages, dressings or absorbent pads for physiological fluids such as urine or blood, e.g. sanitary towels, tampons
    • A61L15/40Bandages, dressings or absorbent pads for physiological fluids such as urine or blood, e.g. sanitary towels, tampons containing ingredients of undetermined constitution or reaction products thereof, e.g. plant or animal extracts
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L17/00Materials for surgical sutures or for ligaturing blood vessels ; Materials for prostheses or catheters
    • A61L17/06At least partially resorbable materials
    • A61L17/08At least partially resorbable materials of animal origin, e.g. catgut, collagen
    • CCHEMISTRY; METALLURGY
    • C08ORGANIC MACROMOLECULAR COMPOUNDS; THEIR PREPARATION OR CHEMICAL WORKING-UP; COMPOSITIONS BASED THEREON
    • C08LCOMPOSITIONS OF MACROMOLECULAR COMPOUNDS
    • C08L89/00Compositions of proteins; Compositions of derivatives thereof
    • C08L89/04Products derived from waste materials, e.g. horn, hoof or hair
    • C08L89/06Products derived from waste materials, e.g. horn, hoof or hair derived from leather or skin, e.g. gelatin
    • DTEXTILES; PAPER
    • D01NATURAL OR MAN-MADE THREADS OR FIBRES; SPINNING
    • D01DMECHANICAL METHODS OR APPARATUS IN THE MANUFACTURE OF ARTIFICIAL FILAMENTS, THREADS, FIBRES, BRISTLES OR RIBBONS
    • D01D5/00Formation of filaments, threads, or the like
    • D01D5/06Wet spinning methods
    • DTEXTILES; PAPER
    • D01NATURAL OR MAN-MADE THREADS OR FIBRES; SPINNING
    • D01DMECHANICAL METHODS OR APPARATUS IN THE MANUFACTURE OF ARTIFICIAL FILAMENTS, THREADS, FIBRES, BRISTLES OR RIBBONS
    • D01D5/00Formation of filaments, threads, or the like
    • D01D5/18Formation of filaments, threads, or the like by means of rotating spinnerets
    • YGENERAL 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
    • Y10TECHNICAL SUBJECTS COVERED BY FORMER USPC
    • Y10STECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y10S128/00Surgery
    • Y10S128/08Collagen

Definitions

  • the present invention relates to collagenous articles 'andtheir. preparation, with particular emphasis on the preparation of articles of substantially purecollagen for. surgical uses and the p r o wo nds
  • the ote'in collagen is found in animal tendons, shin, and in the supporting and integrating fibrous material oi all tissues. It is distinctive, as coxnpared with other. proteins, in its slight tendency to excit foreign body reaction when carried from one. animal to the tiss'uesof another.
  • collagenous tissues may be shredded to produce fibers or strands that are thereafter woven or spun in the manner of textile fibers.
  • collagenous tissues when subjected to suitabl treatment hereinafter described in detail, may be formed into filaments, sheets, and tubes of substantially pure collagen In another type 2 exhibiting high and uniform strength and possessing high qiiityfsun' products are ideally suited for surgical uses.
  • Th present 'process is characterized by the preparation'of acollagen' gel, 'in' which the collagen is present inhighly fiurified, homogeneous cond tion anti innit, "for or fibrils rather than in the molecular sense;
  • the gelf'i's .thusin the nature of highly solvated collagen fibrils rather than one in which the'orig'inaliibrous structure has been aumatised b ri d or by hydrolysis.
  • long filaments and st'rands may beff orm'ed by appropriate techniques to be'dscribed, which involve dehydration oithe gel'to leave the substantially ur c lle e?
  • Another object Qf the invent on s. to Prov d n p o ed pro ess fo the. produc ion o artificial s u o substant a l pure colla en, wherein the sutures are formed of a plurality. of fine collagen filaments to provide a strong and flexible suture of predetermined uniform properties.
  • nequiliefi as has already been pointed out, that partioula'r care be ken t e mina e? on a a materials which, if allowed to remain, would deleteriously affect thev chemical and physical characteristics of th c la e u arti les n q r df em the It is likewise important to attain a high degree o hem ne t wi h R5 to th oll e itself in th el; i the iormeti n of filem n i high I nd uni o m stren th s to be successive u While the gel m k n process.
  • Figs. 3 and 4 are detail views of the extrusion nozzle unit for multi-filament spinning.
  • beef tendon As a starting material for the source of collagen, beef tendon has been found particularly suitable, the tendons from freshly killed steers being preferred. The tendons are stripped of their sheaths and trimmed free of fat and other extraneous tissues. The cleaned tendon will be found to have a shank portion of soft tendon, and branching portions of hard tendon. While both portions contain collagen, the soft portions are somewhat more amenable to the processing treatment hereinafter described. The hard portion may be retained temporarily toserve as a handle in the preliminary operations, or it may be subjected to separate treatment in suitable swelling reagents. Following a thorough soaking and washing of the tendons to remove soluble impurities such as blood, they are frozen to permit slicing, only the soft parts being sliced and retained.
  • distilled water preferably in distilled water, are caused to swell v by the action of acid to obtan a jelly-like mass.
  • Acetic acid has been found satisfactory, using about 20 volumes of 2.5 to 5% acid. This generally will reduce the tendon slices to the desired swollen state in a three-hour period, although an appreciably longer period may be used.
  • the mass of swollen tendon is then blended with distilled water to form adilute sol, using roughly eight volumes of water to one volume of the swollen tendon.
  • the dispersion should be so carried out as to .provide a longitudinal shearing action which separates theswollen tendon units into uniform solvated fibers. Extreme shearing action should be carefuly avoided, however, as should heat, since the collagen is heat sensitive.
  • the blending may be effected in conventional blending equipment, such as a Waring blendor, or the requisite dispersion may be provided by extruding the tendon mass through a perforated plate and the water added thereafter. In either event, it is desirable to screen or filter the dilute sol to remove any large unblended tendon pieces. Filtration through a twenty mesh stainless steel screen is suitable for this purpose.
  • the dilute sol which passes through the screen stillcontains unswollen particles, including noncollagenous substances such as mucoprotein, which if permitted to remain in the gel would. seriously interfere with the success of subsequent processing. Particularly in the case of formation of filaments by extrusion, these unswollen particles or non-homogeneities in the gel, even if small enough to pass freely through the extrusion nozzles, result in discontinuities cute the ultimate strength of the fiber.
  • the dilute sol may be passed through a centrifuge, the most efficient method being to employ the socalled super-centrifuge.
  • the particles may be removed by passing the sol through suitable filters. Whatever the actual manner of removal, the formation of a dilute sol appears to be a prerequisite to successful removal of the unswollen matter.
  • the blending and centrifugation steps cause a large amount of air to be trapped in the sol. This must be removed to prevent floating of precipitated collagen during subsequent steps. Removal'of air is readily effected by subjecting the sol to evacuation, or by allowing the sol to stand for sufiicient time.
  • the deaerated sol at this stage will contain approximately 0.1% collagen. Since this is too dilute to permit spinning into filaments, the sol must be concentrated to a gel. This is effectively carried out by precipitating the collagen, which step likewise permits additional purification to be accomplished.
  • the precipitation is effected by adding normal ammonium hydroxide to the sol until a pH of substantially 7.0 is reached. Not only does a pH of 7.0 provide a high collagen concentration, but it results in neutralization of all the free acid and alkali of the dilute sol. In adding the base to the sol, it is preferable to add roughly three-fourths of the required amount of hydroxide rapidly while slowly stirring the sol. The remaining ammonium hydroxide is then added slowly, but with rapid stirring, until the desired pH value is reached.
  • the precipitated collagen is now thoroughly washed in distilled water to remove all traces of salts, the collagen being fluffed up in the liquid to permit free diffusion. Several changes of liquid may be necessary before the wash water shows a negligible amount of electrolyte.
  • the thoroughly washed precipitate is converted to a gel by the addition of an organic acid, such as malonic acid.
  • an organic acid such as malonic acid.
  • the final gel should contain approximately 1.8% collagen and 0.6% acid by weight.
  • the gel is smoothed or homogenized by conventional techniques and apparatus to give a uniform and homogeneous gel of collagen fibrils.
  • the smoothing should be so carried out as to produce a uniform dispersion of the collagen fibrils without appreciably affecting the fibrillar units themselves.
  • the gel is ready for extrusion to form filaments, or for formation into other types of product.
  • the gel if stored in sterile containers kept at a temperature of the order of 4 C., will remain usable for two to three weeks following its preparation, but it is preferable to use the gel as soon as possible after it has been made.
  • an extrusion technique is preferably employed. If high strength and, in the case of fibers for surgical uses, resistance to enzymatic digestion are to be attained, it is necessary to insure proper orientation and longitudinal alignment of the individual fibrils. These fibrils, submicroscopic in size, are in various states of coiling and tan gling in the gel, and, as heretofore indicated, account for between 1.5 and 2.0% of the weight of the gel.
  • Such a gel is relatively stringy-and cohesive, but only slightly elastic.
  • the gel column When discharged froma suitable nozzle that is directed generally in. a downward direction, the gel column will remain coherent for: a free drop of the order of forty centimeters.
  • the weight of the lower portions of the column gives rise to tension in the region adjacent the jet, and this tension causes the gel column to contract or neck down.
  • anappreciable increase in elasticity may be observed, indicative of a progressive. orientation of the fibrils from their initial random and tangledarrangement into. a more or" less orderly longitudinal alignment.
  • nozzle or jet through which the gel is extruded, a relatively long tube or capillary.
  • a tube ten to twenty cm. in length is appropriate.
  • the jet diameter, or tube bore is preferably within the range of 0.6 mm. 1
  • the gel carefully prepared according to the previously described technique to minimize local diiierences in the gel characteristics, is supplied by a metering pump 8 to downwardly directed nozzle 0.
  • the nozzle has a length many times its internal diameter, and is some distance above the surface of a tank I2 to bring about stretching of the discharged gel by the action of gravity. Heights greater than about twenty cm., and up to thirty to forty cm. will generally be found to provide adequate stretch, and can satisfactorily be employed with a properly prepared gel.
  • the tank into which the gel is discharged from the jet contains a liquid for dehydrating the gel.
  • Acetone has been found preferable for this purpose. It has been established that during the initial. stages of dehydration the fiber becomes weaker than the original gel column, before it increases in strength. Accordingly, the loop of fiber in the first bath is so adjusted that the weak spot occurs near the bottom of the loop.
  • Additional stretch is provided in a second dehydrating bath IS.
  • the pulley I8 is arranged to provide a predetermined stretch between it and pulley I4. In general a stretch of not over 15% is sufiicient in this region.
  • the fiber is returned to the bath for still further dehydration, and then taken up on a winding reel 20. A constant tension is maintained by means of the weight 22.
  • the fiber as it comes from the acetone is, in
  • a multi-filament extrusion process may be employed. out this method, a rotating nozzle head having a plurality-oi nozzlesis arranged to discharge multiple gel streams into the coagulating bath. By reason of the nozzle rotation, the individual filaments a'retwisted into a strand, and in the event a filamentbreaks, the loose end is automatically picked'sup.
  • the gel is supplied by pump 31!) to. the rotating nozzle assembly 32 shown in detail" in Fig. 3..
  • the multiple gel filaments are discharged: into a. bath to of flowing acetone to impart. stretch for purposes of fibril orientation andzto cause morerapidinitial dehydration.
  • the acetone is caused toflow continuously from one end, of the bath to, the other by means of a circulating pump, 35.
  • Further dehydration and stretching is carried out in thesecond bath 38, aftenwhich the strand is wound at it under the tensioniafforded by weight t2. Washing and drying maybe carried out inthe same fashion as for the mono-filament.
  • the nozzle assembly for multiple filament extrusion comprises a head d8rotatably mounted in a support 50.
  • a plurality of nozzles 52 are arranged parallel to the axis of rotation of the head and opening into the chamber 54 within the head. These. nozzles are preferably similar to those employed for single filament extrusion, having a bore of 0.6 mm. to 1.5 mm. and a length of 10 cm. to 20 cm.
  • The, gel is supplied, through an axial tube5'6 to the chamber 54, a rotatable seal being provided, by a suitable stuffing box.
  • the head is rotated during extrusion by means of a worm gear 62, that is driven by worm 64 from a suitable driving motor.
  • the extrusion rate and the speed. of' rotation are coordinated to provide the desired twist in the finished collagen strand.
  • chrome tanning techniques analogous to those employed in the treatment of leather are effective in minimizing absorption of water and in increasing resistance to In carrying enzyme digestion.
  • Chrome alum solutions containing sodium adipate or sodium adipate and sodium lactate may be used to advantage, employing a considerable excess of chrome liquor in the tannage.
  • the fibers produced in accordance with the invention exhibit substantial tensile strength.
  • a dry strength of more than 40 kilograms per square millimeter of fiber cross section may readily be attained, and wet strengths of the order of 30 kilograms per square millimeter.
  • these fibers when implanted as sutures exhibit substantial resistance to enzymatic digestion, so that over 50% of the initial Wet strength may be realized at the end of a seven day period in tissue.
  • Such strengths compare favorably with catgut sutures, but they are materially greater than are afforded by processes wherein the collagen is converted to gelatine rather than retained as fibrillar units.
  • the collagen gel may be formed into sheets, tubes, and other shapes by appropriate dehydrating techniques.
  • the steps which comprise blending the swollen mass with a Water to form a dilute sol containing less than approximately 0.5% collagen by weight, centrifuging the dilute sol to remove unswollen particles therefrom, and precipitating the collagen from the sol, prior to conversion of the collagen to a gel for spinning.
  • steps which comprise blending the mass with water to form a dilute s01 containing approximately 0.1 collagen by weight, treating the dilute sol by centrifuging to remove unswollen hard particles therefrom, and precipitat- .ing the collagen from the treated sol, prior to conversion of the collagen to a gel for spinning.

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Description

May 27, 1952 T. P. SALO ETAL 2,598,608
PREPARATION OF COLLAGENOUS MATERIALS Filed June 11, 1946 INVENTORS Torsf/ I? 50/0 y David F Waugh Patented May 27; 1952 PREPARATION OF COLL G Us MATERIALS Torstiv P. Salo, Cambridge, and DavidF. Waugh,
Belmont, 'Massg assignors, by mesne assignments'f'to Research Corporation, New York, NJYL, a corporation of New York Appiication June 11, 1946, Serial No. 6 76,Q7
4 Claims. (Cl. 260-417) The present invention relates to collagenous articles 'andtheir. preparation, with particular emphasis on the preparation of articles of substantially purecollagen for. surgical uses and the p r o wo nds The ote'in collagen is found in animal tendons, shin, and in the supporting and integrating fibrous material oi all tissues. It is distinctive, as coxnpared with other. proteins, in its slight tendency to excit foreign body reaction when carried from one. animal to the tiss'uesof another. Fur thermore, it is relatively slo'wto yield to proteolytie enzymes, such as are found in the tissues and in he d e e rac The puss litythat collagen mi ht be separated from ninfal tissues and then reconstituted to form articles such'as sheets or filaments of collagen has been of considerable interest for some time. A number of attempts have heretofore been made to devise techniques to accomplish this, but i l 1 333 uccess has been reported. In general, these attempts hav been directed along markedly different lines. According to one prior teclmique,'the collagenous tissues are subjected to treatment which hydrolyzes th collagen to gelatine, so that the collagen is present in a molecular sense only. The gelatine is then sub- ,iectedprocessing to yield filaments or the like. The products, however, are usually found to be seriously lacking in strength. of approach, collagenous tissues may be shredded to produce fibers or strands that are thereafter woven or spun in the manner of textile fibers. This method obviously does not permit the prouoti n 01 rtic s of co la en l n Not onl do hese p ior techn ues i o ode he re u si e stren h and un fo m i of product, but they laol; the essential purity for imp an ation in h man ss sl m e s as elastin (protein of elastic tissues), the muco proteins or muoins associated with collagen, and the blood constituents which contaminate any extirpated tissue, must be effectively removed if the final collagen product is not to cause undue tissue reacti'onl Furthermore, any non-homogeneity, Whether due to collagenoi s or to nonoollagenous substances, if not removed in the coursof the process, causes discontinuitiesin the'final collagen structure. Such discontinuities seriously impair the strength of the finished articles, particularly those of afilamentary origin such as suturesf We have found that collagenous tissues, when subjected to suitabl treatment hereinafter described in detail, may be formed into filaments, sheets, and tubes of substantially pure collagen In another type 2 exhibiting high and uniform strength and possessing high qiiityfsun' products are ideally suited for surgical uses.
Th present 'process is characterized by the preparation'of acollagen' gel, 'in' which the collagen is present inhighly fiurified, homogeneous cond tion anti innit, "for or fibrils rather than in the molecular sense; The gelf'i's .thusin the nature of highly solvated collagen fibrils rather than one in which the'orig'inaliibrous structure has been aumatised b ri d or by hydrolysis. 'From thisgel of solvated fibrils, long filaments and st'rands may beff orm'ed by appropriate techniques to be'dscribed, which involve dehydration oithe gel'to leave the substantially ur c lle e? u tu e It is one'of thefseireral objects of the invention to provide a process for the" production ofa col lagen gel having such properties that collagenous min hi h an usiio'rm rt t m be ade her ir m- Mor spec f cally i s a obj t produte a el fr m w ch c lla en mom n s m e tr e that are well adapted for surgical sutures, bein i -t et ut n uni sarm tvl t s rte th and non-antigenicity,
Another object Qf the invent on s. to Prov d n p o ed pro ess fo the. produc ion o artificial s u o substant a l pure colla en, wherein the sutures are formed of a plurality. of fine collagen filaments to provide a strong and flexible suture of predetermined uniform properties.
e pr dutt n 9 99 g! nequiliefi: as has already been pointed out, that partioula'r care be ken t e mina e? on a a materials which, if allowed to remain, would deleteriously affect thev chemical and physical characteristics of th c la e u arti les n q r df em the It is likewise important to attain a high degree o hem ne t wi h R5 to th oll e itself in th el; i the iormeti n of filem n i high I nd uni o m stren th s to be succes u While the gel m k n process. o be desc i ed pllows. in its b oade aspec s. t s n -u s an p in i l i is. dist n uishe i on; ri P cesse in its inclusion of steps which are important to the produ tion o Wha ma be term for Wa of a be er e s on. a hom ene u elht f ee el o h hly pur fied colla en. w rein the ol a e is n a fib l ar and o a. mo e ar 2 persion.
nthe ccompan ng draw gs, Fi l ustrates the mannerof orminss n le l a en fi er ments irogn thepreper si ge Fi ;2 illus rates the manner of forming a multi-fllament strand, and Figs. 3 and 4 are detail views of the extrusion nozzle unit for multi-filament spinning.
In th gel making process to be described, certain of the steps are concerned with purification of the collagen, while other steps involve the provision of a homogeneous fibrillar dispersion without excessive disintegration of th individual fibrils. It will be understood that the invention is not to be rigidly limited to the identical steps set forth, as equivalent procedures may be substituted.
As a starting material for the source of collagen, beef tendon has been found particularly suitable, the tendons from freshly killed steers being preferred. The tendons are stripped of their sheaths and trimmed free of fat and other extraneous tissues. The cleaned tendon will be found to have a shank portion of soft tendon, and branching portions of hard tendon. While both portions contain collagen, the soft portions are somewhat more amenable to the processing treatment hereinafter described. The hard portion may be retained temporarily toserve as a handle in the preliminary operations, or it may be subjected to separate treatment in suitable swelling reagents. Following a thorough soaking and washing of the tendons to remove soluble impurities such as blood, they are frozen to permit slicing, only the soft parts being sliced and retained. It has been found that slicing to a thickness of the order of 1 mm. is of aid in securing a uniform gel. It is likewise considered advantageous to allow no drying of the tendon material at any stage prior to the final dehydration in the formation of the finished product.
The tendon slices, after soaking and washing,
preferably in distilled water, are caused to swell v by the action of acid to obtan a jelly-like mass. Acetic acid has been found satisfactory, using about 20 volumes of 2.5 to 5% acid. This generally will reduce the tendon slices to the desired swollen state in a three-hour period, although an appreciably longer period may be used.
To permit the effective removal of unswollen particles by a subsequent operation, the mass of swollen tendon is then blended with distilled water to form adilute sol, using roughly eight volumes of water to one volume of the swollen tendon. The dispersion should be so carried out as to .provide a longitudinal shearing action which separates theswollen tendon units into uniform solvated fibers. Extreme shearing action should be carefuly avoided, however, as should heat, since the collagen is heat sensitive. The blending may be effected in conventional blending equipment, such as a Waring blendor, or the requisite dispersion may be provided by extruding the tendon mass through a perforated plate and the water added thereafter. In either event, it is desirable to screen or filter the dilute sol to remove any large unblended tendon pieces. Filtration through a twenty mesh stainless steel screen is suitable for this purpose. I
The dilute sol which passes through the screen stillcontains unswollen particles, including noncollagenous substances such as mucoprotein, which if permitted to remain in the gel would. seriously interfere with the success of subsequent processing. Particularly in the case of formation of filaments by extrusion, these unswollen particles or non-homogeneities in the gel, even if small enough to pass freely through the extrusion nozzles, result in discontinuities duce the ultimate strength of the fiber.
To remove these unswollen particles, the dilute sol may be passed through a centrifuge, the most efficient method being to employ the socalled super-centrifuge. Alternatively, the particles may be removed by passing the sol through suitable filters. Whatever the actual manner of removal, the formation of a dilute sol appears to be a prerequisite to successful removal of the unswollen matter.
The blending and centrifugation steps cause a large amount of air to be trapped in the sol. This must be removed to prevent floating of precipitated collagen during subsequent steps. Removal'of air is readily effected by subjecting the sol to evacuation, or by allowing the sol to stand for sufiicient time.
The deaerated sol at this stage will contain approximately 0.1% collagen. Since this is too dilute to permit spinning into filaments, the sol must be concentrated to a gel. This is effectively carried out by precipitating the collagen, which step likewise permits additional purification to be accomplished. The precipitation is effected by adding normal ammonium hydroxide to the sol until a pH of substantially 7.0 is reached. Not only does a pH of 7.0 provide a high collagen concentration, but it results in neutralization of all the free acid and alkali of the dilute sol. In adding the base to the sol, it is preferable to add roughly three-fourths of the required amount of hydroxide rapidly while slowly stirring the sol. The remaining ammonium hydroxide is then added slowly, but with rapid stirring, until the desired pH value is reached.
The precipitated collagen is now thoroughly washed in distilled water to remove all traces of salts, the collagen being fluffed up in the liquid to permit free diffusion. Several changes of liquid may be necessary before the wash water shows a negligible amount of electrolyte.
The thoroughly washed precipitate is converted to a gel by the addition of an organic acid, such as malonic acid. For satisfactory spinning properties, the final gel should contain approximately 1.8% collagen and 0.6% acid by weight. After stirring until all unswollen or ropy strands have disappeared, the gel is smoothed or homogenized by conventional techniques and apparatus to give a uniform and homogeneous gel of collagen fibrils. The smoothing should be so carried out as to produce a uniform dispersion of the collagen fibrils without appreciably affecting the fibrillar units themselves. Following deaeration, the gel is ready for extrusion to form filaments, or for formation into other types of product. The gel, if stored in sterile containers kept at a temperature of the order of 4 C., will remain usable for two to three weeks following its preparation, but it is preferable to use the gel as soon as possible after it has been made.
To form collagen fibers from the gel, an extrusion technique is preferably employed. If high strength and, in the case of fibers for surgical uses, resistance to enzymatic digestion are to be attained, it is necessary to insure proper orientation and longitudinal alignment of the individual fibrils. These fibrils, submicroscopic in size, are in various states of coiling and tan gling in the gel, and, as heretofore indicated, account for between 1.5 and 2.0% of the weight of the gel.
5. Such a gel is relatively stringy-and cohesive, but only slightly elastic. When discharged froma suitable nozzle that is directed generally in. a downward direction, the gel column will remain coherent for: a free drop of the order of forty centimeters. The weight of the lower portions of the column gives rise to tension in the region adjacent the jet, and this tension causes the gel column to contract or neck down. Along with the necking down, anappreciable increase in elasticity may be observed, indicative of a progressive. orientation of the fibrils from their initial random and tangledarrangement into. a more or" less orderly longitudinal alignment.
The importance of securing and maintaining the maximum degree of longitudinal orientationof the fibrils'in the extruded filament is dueto the belief that the ultimate strength of the finished fiber is not so much a function of the ten sile strength of the individual fibrils as it is dependent on the lateral bonds between fibrils. On this theory, breaking under tension occurs because of disruption ofthese lateral bonds, with subsequent slippage of the fibrils past one another. Tangles of fibrils, and fibrils at an angle to the longitudinal axis of the main fiber thus reduce the number, of lateral bonds available to carry a load in tension.
To aid in attaining the desired orientation of fibrils, it is advantageous to employ as the nozzle or jet, through which the gel is extruded, a relatively long tube or capillary. By way of example, a tube ten to twenty cm. in length is appropriate. In general, the jet diameter, or tube bore, is preferably within the range of 0.6 mm. 1
to 1.5 mm.
In carrying out the extrusion of the gel into filaments and fibers, it is desirable to provide for careful control of the elongation at the various stages of the process. A procedure appropriate to the extrusion of single filaments is illustrated in Fig. 1 of thedrawings.
The gel, carefully prepared according to the previously described technique to minimize local diiierences in the gel characteristics, is supplied by a metering pump 8 to downwardly directed nozzle 0. The nozzle has a length many times its internal diameter, and is some distance above the surface of a tank I2 to bring about stretching of the discharged gel by the action of gravity. Heights greater than about twenty cm., and up to thirty to forty cm. will generally be found to provide adequate stretch, and can satisfactorily be employed with a properly prepared gel.
The tank into which the gel is discharged from the jet contains a liquid for dehydrating the gel. Acetone has been found preferable for this purpose. It has been established that during the initial. stages of dehydration the fiber becomes weaker than the original gel column, before it increases in strength. Accordingly, the loop of fiber in the first bath is so adjusted that the weak spot occurs near the bottom of the loop.
By the time the fiber reaches pulley M, the fiber has gained considerable strength.
Additional stretch is provided in a second dehydrating bath IS. The pulley I8 is arranged to provide a predetermined stretch between it and pulley I4. In general a stretch of not over 15% is sufiicient in this region. The fiber is returned to the bath for still further dehydration, and then taken up on a winding reel 20. A constant tension is maintained by means of the weight 22.
The fiber as it comes from the acetone is, in
6, effect, a loosenetwork of collagenfibrils containing' some residual acid. Not only is it necessary'to'remove the acid, but alsothe fibrils must be furtheroriented and bonded tov one another. Washing is preferably carried out bypassing the fiber into-distilled water, orinto a. solution containing a dilute bufier at pH 9.1. A tension of 1.2 to 1.5 g. tension is advisable, and the subsequent drying should also'be carried out with tension maintained.
To provide collagen strands of greater effective cross section than can conveniently be extruded from a single nozzle, a multi-filament extrusion process may be employed. out this method, a rotating nozzle head having a plurality-oi nozzlesis arranged to discharge multiple gel streams into the coagulating bath. By reason of the nozzle rotation, the individual filaments a'retwisted into a strand, and in the event a filamentbreaks, the loose end is automatically picked'sup.
In carrying out the mult-i-filament spinning according to Fig. 2, the gel is supplied by pump 31!) to. the rotating nozzle assembly 32 shown in detail" in Fig. 3.. The multiple gel filaments are discharged: into a. bath to of flowing acetone to impart. stretch for purposes of fibril orientation andzto cause morerapidinitial dehydration. The acetone is caused toflow continuously from one end, of the bath to, the other by means of a circulating pump, 35. Further dehydration and stretching is carried out in thesecond bath 38, aftenwhich the strand is wound at it under the tensioniafforded by weight t2. Washing and drying maybe carried out inthe same fashion as for the mono-filament.
The nozzle assembly for multiple filament extrusion comprises a head d8rotatably mounted in a support 50. A plurality of nozzles 52 are arranged parallel to the axis of rotation of the head and opening into the chamber 54 within the head. These. nozzles are preferably similar to those employed for single filament extrusion, having a bore of 0.6 mm. to 1.5 mm. and a length of 10 cm. to 20 cm. The, gel, is supplied, through an axial tube5'6 to the chamber 54, a rotatable seal being provided, by a suitable stuffing box. The head is rotated during extrusion by means of a worm gear 62, that is driven by worm 64 from a suitable driving motor. The extrusion rate and the speed. of' rotation are coordinated to provide the desired twist in the finished collagen strand.
It, is likewise possible to provide collagen strands which are made up of mono-filaments or small multi-filaments, braided together to form a strand of the desired effective cross-section. Such a strand offers great flexibility and is particularly effective for surgical uses, since the flexibility aids in tying small but secure knots.
The pure collagen strands and fibers formed according to the techniques hereinbefore described, when immersed in water or implanted in tissue, swell substantially. Along with the swelling, there is a considerable loss in strength. In the case of fibers implanted in tissue, absorption occurs relatively rapidly.
To minimize swelling and to increase the Wet strength of the collagen strands, it is desirable to subject the strands to appropriate tanning treatment. Such treatment likewise increases the re sistance to enzymatic digestion.
It has been found that chrome tanning techniques analogous to those employed in the treatment of leather are effective in minimizing absorption of water and in increasing resistance to In carrying enzyme digestion. Chrome alum solutions containing sodium adipate or sodium adipate and sodium lactate may be used to advantage, employing a considerable excess of chrome liquor in the tannage.
Following the tanning, a heat sterilization procedure is necessary where the collagen strands are to have surgical uses, as in sutures or the like. Heating at approximately 130 for three to six hours may be considered typical.
The fibers produced in accordance with the invention exhibit substantial tensile strength. By way of illustration, a dry strength of more than 40 kilograms per square millimeter of fiber cross section may readily be attained, and wet strengths of the order of 30 kilograms per square millimeter. Furthermore, these fibers when implanted as sutures exhibit substantial resistance to enzymatic digestion, so that over 50% of the initial Wet strength may be realized at the end of a seven day period in tissue. Not only do such strengths compare favorably with catgut sutures, but they are materially greater than are afforded by processes wherein the collagen is converted to gelatine rather than retained as fibrillar units.
In addition to formation into fibers and strands, it will be understood that the collagen gel may be formed into sheets, tubes, and other shapes by appropriate dehydrating techniques.
We have described as our invention a procedure for the preparation of highly purified and homogeneous collagen gels, and the formation of articles, particularly fibers and strands, that are well adapted for surgical uses. In the case of fibers and strands for sutures, a technique has been evolved that permits the production, in continuous lengths measured in thousands of feet, of strong, uniform, and extremely pure collagen filaments, both single and multiple, that are well qualified to replace the usual catgut.
We claim:
1. In the process of converting a swollen mass of tendon pieces to a gel of solvated fibrils of substantially pure collagen from which filaments may be spun, the steps which comprise blending the swollen mass with a water to form a dilute sol and centrifuging the ,dilute sol prior to conversion to a gel for spinning.
2. In the process of converting a swollen mass of tendon pieces to a gel of solvated fibrils of substantially pure collagen from which filaments may be spun, the steps which comprise blending the swollen mass with a water to form a dilute 8. sol, centrifuging the dilute sol to remove unswollen particles therefrom, precipitating the collagen and washing the precipitate, prior to conversion of the collagen to a gel for spinning.
3. In the process of converting a swollen mass of tendon pieces to a gel of solvated fibrils of substantially pure collagen from which filaments may be spun, the steps which comprise blending the swollen mass with a Water to form a dilute sol containing less than approximately 0.5% collagen by weight, centrifuging the dilute sol to remove unswollen particles therefrom, and precipitating the collagen from the sol, prior to conversion of the collagen to a gel for spinning.
4. In the process of converting a swollen mass of tendon pieces to a gel of solvated fibrils of substantially pure collagen from which filaments may be spun, the steps which comprise blending the mass with water to form a dilute s01 containing approximately 0.1 collagen by weight, treating the dilute sol by centrifuging to remove unswollen hard particles therefrom, and precipitat- .ing the collagen from the treated sol, prior to conversion of the collagen to a gel for spinning.
TORSTI P. SALO. DAVID F. WAUGH.
REFERENCES CITED The following references are of record in the file of this patent:
UNITED STATES PATENTS Number Name Date 1,712,077 Hrubesky May 7, 1929 1,999,641 Sharp Apr. 30, 1935 2,039,262 Schulte Apr. 28, 1936 2,046,670 Beattey July 7, 1936 2,056,595 Becker Oct. 6, 1936 2,058,835 Schulte Oct. 27, 1936 2,114,220 Freudenberg et a1. Apr. 12, 1938 2,167,251 Rogers July 25, 1939 2,267,488 Becker Dec. 23, 1941 2,337,775 Schultz Dec. 28, 1943 2,461,602 Hollihan Feb. 15, 1949 FOREIGN PATENTS Number Country Date 422,990 Great Britain Jan. 23, 1935 464,406 Great Britain Apr. 15, 1937 471,954 Great Britain Sept. 14, 1937 OTHER REFERENCES Ser. No. 313,138, Freudenberg (A. P. C.), published April 27, 1943.

Claims (1)

1. IN THE PROCESS OF CONVERTING A SWOLLEN MASS OF TENDON PIECES TO A GEL OF SOLVATED FIBRILS OF SUBSTANTIALLY PURE COLLAGEN FROM WHICH FILAMENTS MAY BE SPUN, THE STEP WHICH FILAMENTS ING THE SWOLLEN MASS WITH A WATER TO FORM A DILUTE SOL AND CENTRIFUGING THE DILUTE SOL PRIOR TO CONVERSION TO A GEL FOR SPINING.
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Cited By (20)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2740774A (en) * 1953-01-16 1956-04-03 Armour & Co Extraction of animal glue in presence of insoluble basic substance
US2992213A (en) * 1957-11-08 1961-07-11 Eastman Kodak Co Acid cooked pigskin gelatins for photographic subbing
US3014024A (en) * 1958-03-19 1961-12-19 Johnson & Johnson Collagen film
US3034852A (en) * 1960-01-26 1962-05-15 Japan Leather Mfg Co Ltd Solubilization of insoluble collagen fibers and reconstitution thereof
US3114591A (en) * 1961-04-12 1963-12-17 Ethicon Inc Process for the manufacture of suture material from animal tendons
US3114372A (en) * 1961-04-12 1963-12-17 Ethicon Inc Collagenous article and the manufacture thereof
DE1193197B (en) * 1961-03-07 1965-05-20 Ethicon Inc Multi-hole spinning nozzle for spinning collagen fiber dispersions
US3376869A (en) * 1964-02-21 1968-04-09 Ethicon Inc Surgical collagen film formed from random lengths of collagen tapes or strands
DE1298280B (en) * 1960-05-12 1969-06-26 Leeuwen Henri Bernard Van Process for the production of molded articles, in particular sausage casings, from collagen-containing material
DE2064604A1 (en) * 1970-12-30 1972-07-06 Chemisches Laboratorium Dr. Kurt Richter Gmbh, 1000 Berlin Skin care products
US4307055A (en) * 1978-12-06 1981-12-22 Fuji Photo Film Co., Ltd. Apparatus and process for noodling gelatin dispersion
US4544516A (en) * 1982-07-28 1985-10-01 Battelle Development Corporation Collagen orientation
US5106949A (en) * 1989-09-15 1992-04-21 Organogenesis, Inc. Collagen compositions and methods for preparation thereof
US5256418A (en) * 1990-04-06 1993-10-26 Organogenesis, Inc. Collagen constructs
WO1996014453A1 (en) * 1994-11-02 1996-05-17 E.R. Squibb & Sons Inc. Alginate ropes, method of preparation and use
US6361551B1 (en) 1998-12-11 2002-03-26 C. R. Bard, Inc. Collagen hemostatic fibers
US6454787B1 (en) 1998-12-11 2002-09-24 C. R. Bard, Inc. Collagen hemostatic foam
US20030183978A1 (en) * 2001-03-14 2003-10-02 Tetsuo Asakura Method of producing fiber and film of silk and silk-like material
US20130040885A1 (en) * 2009-08-28 2013-02-14 Tissue Science Laboratories Plc Collagen pad
US20150359929A1 (en) * 2013-02-04 2015-12-17 Northeastern University Mechanochemical Collagen Assembly

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US1712077A (en) * 1928-03-14 1929-05-07 Clarence E Hrubesky Water-resistant animal glue
GB422990A (en) * 1933-02-11 1935-01-23 Koninklijke Pharma Fab Nv A process and apparatus for the manufacture of threads, strings, bands, films and the like from elasin- and collagen-containing materials
US1999641A (en) * 1932-07-30 1935-04-30 Davis & Sharp Strand for suture and other purposes and method of making the same
US2046670A (en) * 1933-06-28 1936-07-07 Beattey Earle J Richard Making of rayon
US2056595A (en) * 1932-12-19 1936-10-06 Firm Naturin Gmbh Method for working up fibrous material from hides
GB464406A (en) * 1934-10-15 1937-04-15 Freudenberg Carl Gmbh A process for working up untanned animal hyde material
GB471954A (en) * 1935-10-30 1937-09-14 Freudenberg Carl Gmbh Improvements in or relating to flexible tubes
US2114220A (en) * 1932-11-28 1938-04-12 Freudenberg Hans Manufacture of artificial sausage skins or casings
US2167251A (en) * 1938-08-20 1939-07-25 Davis & Geck Inc Surgical tape of submucosa tissue
US2267488A (en) * 1936-11-21 1941-12-23 Becker & Co Naturinwerk Method and apparatus for producing sausage skins
US2337775A (en) * 1941-04-25 1943-12-28 Armour & Co Manufacture of sausage casings and the like
US2461602A (en) * 1946-01-17 1949-02-15 American Viscose Corp Method of manufacturing synthetic sutures and the like

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Publication number Priority date Publication date Assignee Title
US1712077A (en) * 1928-03-14 1929-05-07 Clarence E Hrubesky Water-resistant animal glue
US1999641A (en) * 1932-07-30 1935-04-30 Davis & Sharp Strand for suture and other purposes and method of making the same
US2114220A (en) * 1932-11-28 1938-04-12 Freudenberg Hans Manufacture of artificial sausage skins or casings
US2056595A (en) * 1932-12-19 1936-10-06 Firm Naturin Gmbh Method for working up fibrous material from hides
US2039262A (en) * 1933-02-11 1936-04-28 Koninklijke Pharma Fab Nv Process for the manufacture of threads, strings, bands, films, and the like
US2058835A (en) * 1933-02-11 1936-10-27 Koninklijke Pharma Fab Nv Process for the manufacture of threads, strings, bands, films, and the like
GB422990A (en) * 1933-02-11 1935-01-23 Koninklijke Pharma Fab Nv A process and apparatus for the manufacture of threads, strings, bands, films and the like from elasin- and collagen-containing materials
US2046670A (en) * 1933-06-28 1936-07-07 Beattey Earle J Richard Making of rayon
GB464406A (en) * 1934-10-15 1937-04-15 Freudenberg Carl Gmbh A process for working up untanned animal hyde material
GB471954A (en) * 1935-10-30 1937-09-14 Freudenberg Carl Gmbh Improvements in or relating to flexible tubes
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US2167251A (en) * 1938-08-20 1939-07-25 Davis & Geck Inc Surgical tape of submucosa tissue
US2337775A (en) * 1941-04-25 1943-12-28 Armour & Co Manufacture of sausage casings and the like
US2461602A (en) * 1946-01-17 1949-02-15 American Viscose Corp Method of manufacturing synthetic sutures and the like

Cited By (22)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2740774A (en) * 1953-01-16 1956-04-03 Armour & Co Extraction of animal glue in presence of insoluble basic substance
US2992213A (en) * 1957-11-08 1961-07-11 Eastman Kodak Co Acid cooked pigskin gelatins for photographic subbing
US3014024A (en) * 1958-03-19 1961-12-19 Johnson & Johnson Collagen film
US3034852A (en) * 1960-01-26 1962-05-15 Japan Leather Mfg Co Ltd Solubilization of insoluble collagen fibers and reconstitution thereof
DE1298280B (en) * 1960-05-12 1969-06-26 Leeuwen Henri Bernard Van Process for the production of molded articles, in particular sausage casings, from collagen-containing material
DE1193197B (en) * 1961-03-07 1965-05-20 Ethicon Inc Multi-hole spinning nozzle for spinning collagen fiber dispersions
US3114591A (en) * 1961-04-12 1963-12-17 Ethicon Inc Process for the manufacture of suture material from animal tendons
US3114372A (en) * 1961-04-12 1963-12-17 Ethicon Inc Collagenous article and the manufacture thereof
US3376869A (en) * 1964-02-21 1968-04-09 Ethicon Inc Surgical collagen film formed from random lengths of collagen tapes or strands
DE2064604A1 (en) * 1970-12-30 1972-07-06 Chemisches Laboratorium Dr. Kurt Richter Gmbh, 1000 Berlin Skin care products
US4307055A (en) * 1978-12-06 1981-12-22 Fuji Photo Film Co., Ltd. Apparatus and process for noodling gelatin dispersion
US4544516A (en) * 1982-07-28 1985-10-01 Battelle Development Corporation Collagen orientation
US5106949A (en) * 1989-09-15 1992-04-21 Organogenesis, Inc. Collagen compositions and methods for preparation thereof
US5256418A (en) * 1990-04-06 1993-10-26 Organogenesis, Inc. Collagen constructs
WO1996014453A1 (en) * 1994-11-02 1996-05-17 E.R. Squibb & Sons Inc. Alginate ropes, method of preparation and use
US6361551B1 (en) 1998-12-11 2002-03-26 C. R. Bard, Inc. Collagen hemostatic fibers
US6454787B1 (en) 1998-12-11 2002-09-24 C. R. Bard, Inc. Collagen hemostatic foam
US20030183978A1 (en) * 2001-03-14 2003-10-02 Tetsuo Asakura Method of producing fiber and film of silk and silk-like material
US20130040885A1 (en) * 2009-08-28 2013-02-14 Tissue Science Laboratories Plc Collagen pad
US20150359929A1 (en) * 2013-02-04 2015-12-17 Northeastern University Mechanochemical Collagen Assembly
US10213523B2 (en) * 2013-02-04 2019-02-26 Northeastern University Mechanochemical collagen assembly
US10888637B2 (en) 2013-02-04 2021-01-12 Northeastern University Mechanochemical collagen assembly

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