WO2005058380A1 - Wound care products containing keratin - Google Patents

Wound care products containing keratin Download PDF

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Publication number
WO2005058380A1
WO2005058380A1 PCT/NZ2004/000323 NZ2004000323W WO2005058380A1 WO 2005058380 A1 WO2005058380 A1 WO 2005058380A1 NZ 2004000323 W NZ2004000323 W NZ 2004000323W WO 2005058380 A1 WO2005058380 A1 WO 2005058380A1
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Prior art keywords
protein
keratin
wound
protein fraction
treating
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PCT/NZ2004/000323
Other languages
French (fr)
Inventor
Robert James Kelly
Alisa Dawn Roddick-Lanzilotta
Mohammad Azam Ali
Original Assignee
Keratec Limited
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Publication date
Application filed by Keratec Limited filed Critical Keratec Limited
Priority to US10/583,445 priority Critical patent/US7732574B2/en
Priority to AU2004298392A priority patent/AU2004298392A1/en
Priority to EP04808918A priority patent/EP1694370B1/en
Priority to JP2006545264A priority patent/JP4662948B2/en
Priority to ES04808918T priority patent/ES2396972T3/en
Priority to EA200601191A priority patent/EA011388B1/en
Priority to DK04808918.9T priority patent/DK1694370T3/en
Publication of WO2005058380A1 publication Critical patent/WO2005058380A1/en

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    • 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
    • A61L15/22Bandages, dressings or absorbent pads for physiological fluids such as urine or blood, e.g. sanitary towels, tampons containing macromolecular materials
    • A61L15/32Proteins, polypeptides; Degradation products or derivatives thereof, e.g. albumin, collagen, fibrin, gelatin
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • A61K38/16Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • A61K38/17Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • A61K38/39Connective tissue peptides, e.g. collagen, elastin, laminin, fibronectin, vitronectin, cold insoluble globulin [CIG]
    • 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
    • A61L26/00Chemical aspects of, or use of materials for, wound dressings or bandages in liquid, gel or powder form
    • A61L26/0009Chemical aspects of, or use of materials for, wound dressings or bandages in liquid, gel or powder form containing macromolecular materials
    • A61L26/0028Polypeptides; Proteins; Degradation products thereof
    • A61L26/0047Specific proteins or polypeptides not covered by groups A61L26/0033 - A61L26/0042
    • 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
    • A61L26/00Chemical aspects of, or use of materials for, wound dressings or bandages in liquid, gel or powder form
    • A61L26/0061Use of materials characterised by their function or physical properties
    • A61L26/008Hydrogels or hydrocolloids
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P17/00Drugs for dermatological disorders
    • A61P17/02Drugs for dermatological disorders for treating wounds, ulcers, burns, scars, keloids, or the like

Definitions

  • the invention relates to wound care products containing keratin.
  • Wounds and lesions can be caused by a variety of events, including surgery, traumatic injury, burns, abrasions and skin grafts. Healing of wounds may be difficult and may result in problems such as ulcers and septicemia. Of particular concern are clironic wounds, such as pressure sores and diabetic ulcers. The treatment of these conditions is of increasing importance as the population ages.
  • Wound dressing can be created using natural materials or through combination of synthetic materials and natural materials (JP# 47470/1988; Jen Ming Yang and Hao Tzu Lin, Properties of chitosan containing PP-g-AA-g-NIPAAm bigraft nonwoven fabric for wound dressing. Journal of Membrane Science, 243(1-2), 2004, p. 1-7).
  • the use of wound dressings is an extremely important part of wound management and vital to achieve successful healing outcomes [Gordon Freedman, Hyacinth Entero and Harold Brem, Practical treatment of pain in patients with chronic wounds: pathogenesis-guided management, The American Journal of Surgery, 188(1), 2004, p. 31-35].
  • An optimum wound dressing protects the injured tissue, maintains a moist environment, is water permeable, maintains microbial control, delivers healing agents to the wound site, is easy to apply, does not require frequent changes and is non-toxic and non-antigenic.
  • wound dressings materials are available commercially, including occlusive dressings, non-adherent dressings, absorbent dressings, and dressings in the form of sheets, foams, powders and gels.
  • occlusive dressings non-adherent dressings
  • absorbent dressings and dressings in the form of sheets, foams, powders and gels.
  • Attempts have been made to provide improved dressings, particularly for chronic wounds, that assist in the wound healing process by using biological materials such as cells and growth factors.
  • biologicals have proven very costly due to factors such as manufacturing processes and storage and stability issues, and in addition they have shown minimal clinical relevance in accelerating the chronic wound healing process.
  • wound management requires an understanding of the process of tissue repair and knowledge of the properties of the wound dressing materials. Only when these two factors are considered together can the process of dressing selection be undertaken in a rational and informed fashion.
  • Keratin proteins are present in a wide range of biological tissue, performing a structural role in skin, hair and other materials. Keratins extracted from hair have been shown to be a valuable component in wound dressings.
  • US 5932552 provides a biocompatible keratin material prepared by either reduction or oxidation for use as a component in wound care products. Those methods included in the art for the oxidation of keratins to create a polar group are harsh and degrading to the keratin, causing protein damage and loss of core physical characteristics arising from the protein amino acid composition and tertiary structure.
  • keratin fibres specifically the intermediate filament proteins and the matrix proteins present in wool and hair, play particular roles within the fibre which is reflected in their tertiary structure and amino acid composition
  • These same features can be capitalized upon to create materials with good physical properties and highly absorbing capacities when using purified forms of these proteins.
  • methods used for isolating keratins need to be mild, to prevent protein damage, create cystine modifications that are reversible, to allow for reconstitution of tough materials tlirough the creation of cystine bonds, and facilitate the isolation of specific keratin protein fractions from the keratin source.
  • the present invention provides new materials for use in wound care products that are prepared according to these principles.
  • the invention provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is intact.
  • the invention also provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is from the intermediate filament protein family.
  • the invention also provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is from the high sulphur protein family.
  • the invention also provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is s-sulfonated.
  • the protein fraction may be hydrolysed.
  • the protein is preferably s-sulfonated.
  • the protein may be from the high sulphur protein family.
  • the protein may be an intermediate filament protein.
  • the material is preferably a fibre, a film, a foam or a hydro gel.
  • the invention also provides a method a method for making a wound care product comprising a) preparing a 10% solution of a keratin protein; b) mixing the keratin protein and a water soluble polymer to form an intimate mixture; c) casting the aqueous mixture so produced; and d) freezing and thawing in sequence to produce a hydrogel.
  • the physico-mechanical properties of the biomaterials may be improved by introducing cross-linker agents to form disulfide bonds and thus remove sulfonate functionalities.
  • the cross-linking agent used as a reductant may be a thiol or thioglycollate salt.
  • the physico-mechanical properties may be wet and dry strength.
  • the thioglycollate salt may be ammonium thioglycollate solution.
  • the water soluble polymer may be polyvinyl alcohol, polyvinylpyrolidone, polyethylene glycol or the like.
  • the invention also provides a method of improving the wet strength properties of the wound care products produced by the method of the invention by incorporating a cross- liking agent into them.
  • the cross-linking agent is preferably an aldehyde.
  • the cross-linking agent may be selected form the group consisting of formaldehyde, glyoxal, glutaraldehyde and the like.
  • Figure 1 shows the response of wounds treated with keratin and other materials
  • Figure 2 shows sheep fibroblast proliferation on keratin materials
  • Figure 3 shows human fibroblast proliferation on keratin materials
  • Figure 4 shows the effect of Con(A) stimulation on T-cell growth in the presence of keratin matrices
  • Figure 5 shows the effect of Con(A) on stimulation of T-cell growth in the presence of keratin matrices after 72 hours.
  • the hard alpha keratin proteins such as those derived from human hair, wool, animal fibres, horns, hooves or other mammalian sources, can be classified into particular components according to their biochemical properties, specifically their molecular weight and amino acid composition.
  • Table 1 illustrates the amino acid composition dete ⁇ nined by conventional analytical methods of typical keratin protein fractions l ⁇ iown in the art and also the subject of tins invention. This involves acid hydrolysis of the analyte which converts all cystine and labile cystine derivatives to cysteine, typically recorded as half-cystine.
  • Table 1 amino acid composition of keratin fractions: S-sulfonated keratin intermediate filament protein (SIFP), S-sulfonated keratin high sulfur protein (SHSP). S-sulfonated keratin peptide (SPEP) as used in the invention Intermediate filament protein (IFP), high sulfur protein (HSP) and whole wool courtesy of Gillespie and Marshall, Variability in the proteins of wool and hair, Proc. Sixth Int. Wool Text. Res. Conf, Pretoria, 2, 67-77, 1980. All residues expressed as mol%. S-sulfocysteine, cystine and cysteine are measured as S-carboxymethyl cysteine following reduction and alkylation, and reported as cys.
  • SIFP S-sulfonated keratin intermediate filament protein
  • SHSP S-sulfonated keratin high sulfur protein
  • SPEP S-sulfonated keratin peptide
  • IFP Intermediate filament protein
  • Table 2 illustrates the molecular weight determined by conventional analytical methods of typical keratin protein fractions known in the art and also the subject of this invention.
  • Conventional analysis involves cleavage of cystine bonds within the keratin using reduction so that the protein mass is determined in its native, uncrosslinked state, most similar to the unkeratinsed state of the protein Mass is determined using polyacrylamide gel electrophoresis.
  • the peptide SPEP mass is determined using mass spectrometry. L sing these methods the keratin is made soluble without any hydrolysis of peptide bonds and an accurate measure of molecular weight is determined.
  • S-sulfonated keratin intermediate filament protein S-sulfonated keratin high sulfur protein (SHSP), S-sulfonated keratin peptide (SPEP) as used in the invention.
  • SIFP S-sulfonated keratin intermediate filament protein
  • SHSP S-sulfonated keratin high sulfur protein
  • SPEP S-sulfonated keratin peptide
  • the subject of the invention is materials containing intact S-sulfonated keratin protein fractions.
  • “Intact” refers to proteins that have not been significantly hydrolysed, with hydrolysis being defined as the cleavage of bonds through the addition of water. Gillespie (Biochemistry and physiology of the skin, vol 1, Ed. Goldsmith Oxford University Press, London, 1983, pp475-510) considers “intact” to refer to proteins in the keratinized polymeric state and further refers to polypeptide subunits which complex to form intact keratins in wool and hair.
  • “intact” refers to the polypeptide subunits described by Gillespie. These are equivalent to the keratin proteins in their native fo ⁇ n without the disulfide crosslinlcs formed tlirough the process of keratinisation.
  • Keratin protein fractions are distinct groups from within the keratin protein family, such as the intermediate filament proteins, the high sulfur proteins or the high glycine- tyrosine proteins well known in the art.
  • Intermediate filament proteins are described in detail by Orwin et al (Structure and Biochemistry of Mammalian Hard Keratin, Electron Microscopy Reviews, 4, 47,1991) and also referred to as low sulphur proteins by Gilliespie (Biochemistry and physiology of the skin, vol 1 , Ed. Goldsmith Oxford University Press, London, 1983, pp475-510).
  • Key characteristics of tins protein family are molecular weight in the range 40 - 60 kD and a cysteine content (measured as half cystine) of around 4%.
  • the high sulfur protein family are also well described by Orwin and Gillispie in the same publications. This protein family has a large degree of heterogeity but can be characterised as having a molecular weight in the range 10 - 30 kD and a cysteine content of greater than 10%. The subset of this family, the ultra high sulfur proteins can have a cysteine content of up to 34%.
  • the high glycine-tryosine protein family are also well described by Orwin and Gillespie in the same publications. Tins family is also referred to as the high tryrosine proteins and has characteristics of a molecular weight less than 10 kD, a tyrosine content typically greater than 10% and a glycine content typically greater than 20%.
  • keratin protein fraction is a purified form of keratin that contains predominantly, although not entirely, one distinct protein group as described above.
  • S-Sulfonated keratins have cysteine/cystine present predominantly in the form S-sulfocysteine, commonly known as the Bunte salt. This highly polar group imparts a degree of solubility to proteins.
  • S-sulfo group Whilst being stable in solution, the S-sulfo group is a labile cysteine derivative, highly reactive towards thiols, such as cysteine, and other reducing agents. Reaction with reducing agents leads to conversion of the S-sulfo cysteine group back to cysteine. S- sulfo cysteine is chemically different to cysteic acid, although both groups contain the
  • Cysteic acid is produced irreversibly by the oxidation of cysteine or cystine and once formed cannot form disulfide crosslinlcs back to cysteine.
  • S-sulfocysteine is reactive towards cysteine and readily forms disulfide crosslinlcs.
  • SIFP can be prepared by methods such as those described in WO03011894.
  • Purified wool keratin intermediate filament proteins are particularly well suited to reformation into matrices, due in part to their high molecular weight and their tertiary structure. Methods outlined in NZ/PCT/00169 make extensive use of these materials to form useful matrices. S-sulfo keratins can be prepared by a variety of methods, including those outlined in PCT NZ02/00125 (which is incorporated herein).
  • Porous sponge matrices are of particular use in a wound environment as they can play an important role in absorbing wound exudates and maintaining a healthy environment for healing a wound. In addition they can act as media for the delivery of other healing agents, such as growth factors, antibacterial agents or cultured cells, that stimulate the healing process. These features are enhanced through using S-sulfonated keratin protein fractions to construct the matrices.
  • S-sulfonated keratin protein fractions to construct the matrices.
  • the highly polar nature of the S-sulfo group makes matrices derived from this material highly absorbing.
  • S-sulfonated keratins are biocompatible and do not invoke an adverse response in vitro.
  • Films are an important component in dressings for the treatment of wounds, providing a barrier to protect the wound and maintaining an appropriate environment to encourage healing.
  • S-sulfonated keratins films are biocompatible and do not invoice an adverse response in vitro. As such, they are useful components in a wound dressing.
  • Fibres reconstituted from S-sulfonated keratin intermediate filament proteins can be used as a component for wound dressings. Fibres are particularly versatile as they can be formed into woven or non-woven constructs and fibre design can be used as well control of the chemistry of the material to effect the interaction of the dressing with the wound. Much work has been undertaken into the use of regenerated fibres in wound care, in particular alginate fibres. Reconstituted keratin fibres derived from S- sulfonated intermediate filament proteins are a new material for use in similar applications.
  • Hydrogels are frequently used in wound dressings and play an in important role in controlling the wound environment and provide a suitable medium for the delivery of actives to stimulate or assist healing.
  • S-sulfonated keratins in particular S-sulfonated intact keratin intermediate filament protein, is an excellent substrate for the formation of hydrogels as a result of the high degree of order and intermolecular interaction achievable as a result of the intact nature of the proteins.
  • Keratin materials derived from the SIFP and SHSP protein fractions contain differing amounts of the highly polar S-sulfo group, and consequently differ in their physicochemical characteristics, in particular their ability to absorb moisture Wound dressings derived from a combination of these absorb moisture to a greater or lesser extent, and so can be controlled in the degree to which they will absorb wound exudates.
  • S-sulfonated keratin proteins prepared as spray or freeze dried powders are highly absorbing materials that are a valuable component in wound dressings, in particular for use in the hydrogel type dressing in which alginates or collagen derivatives are the materials used frequently in currently available products.
  • Combination of the SIFP and SHSP proteins leads to a degree of control over the absorbing capacity of the powder and the nature of the gel formed on absorbance, due to the variation in the amount of S- sulfo groups present within each protein fraction.
  • S-sulfonated keratin protein fractions in particular the keratin intermediate filament protein fraction, can be readily formed into a variety of matrices and the physical properties of these matrices are such that they can provide a useful physical role in a wound environment.
  • the materials can be chemically treated following reformation into films, fibres or sponges, to remove the S-sulfonate functionality and generate disulfide crosslinks within the material, similar to those present in the native keratin. Methods for this treatment are described in
  • the keratin matrices When treated in this way, the keratin matrices are less absorbing and retain their structure in a wound environment. They are well suited to the delivery of bioactives to the wound site, such as antibacterial agents, growth factors, antibiotic treatments, cultured cells or other drugs.
  • bioactives such as antibacterial agents, growth factors, antibiotic treatments, cultured cells or other drugs.
  • the physical and mechanical properties of the wound dressing or healing membranes can be readily improved through a variety of methods.
  • a method for the improvement of the physical and mechanical strength of keratin hydrogel biomaterials is to increase the hydrogen bonding network between the keratin protein chains or the keratin protein and other polymers, such as polyvinyl alcohol and polyvinyl pyrolidone. This can be achieved by using a freezing-thawing process during the constructing hydrogel sheets. This is confirmed by an increase in the insolubility of hydrogels formed using this process.
  • Production of a chemically cross-linked hydrogel biomaterial is another embodiment in the invention. Improving physical properties such as insolubility and strength in swollen states can be achieved by using chemical cross-linkers such as glutaraldehyde, that allow the formation of chemical cross-links between keratin protein chains.
  • chemical cross-linkers such as glutaraldehyde
  • the physical properties of the keratin based membranes and hydrogels can be increased by standard protein cross-linking methods including using, typical chemical cross-linkers such as, glutaraldehyde, formaldehyde, carbodiimides, e.g., l-efhyl-3- (dimethyaminopropyl)carbodiimide, 2,5-hexanedione, diimidates, e.g., dimethylsuberimidate, or bisacrylamides, e.g., N,N'-methylenebisacrylamide.
  • typical chemical cross-linkers such as, glutaraldehyde, formaldehyde, carbodiimides, e.g., l-efhyl-3- (dimethyaminopropyl)carbodiimide, 2,5-hexanedione, diimidates, e.g., dimethylsuberimidate, or bisacrylamides, e.g., N,
  • the films with the disulfide chemical configuration support sheep fibroblast growth most satisfactorily (material D).
  • a second sodium S-sulfonate salt configuration demonstrated by film material C supports cell growth to a lesser degree and tends to swell in culture. Cells on these films showed typical multi- or bipolar elongated fibroblastic morphology with good spread.
  • Fibroblast growth porous sponge material B (disulfide configuration) matched that of some of the better films. During the assay, cells were witnessed to attach to the upper surface of the sponge. By light microscopy, the morphological appearance of these cells was deemed similar on all substrates compared to the no-matrix control. Cells were observed by microscopy to infiltrate the sponge material.
  • Figure 3 is a graph showing the effect of different keratin matrices on human dermal fibroblast cell proliferation relative to cell media alone (control)
  • Figure 4 demonstrates the effect of ConA stimulation on T cells grown in the presence/absence of keratin matrices over a 10-day period. Tritiated thymidine counts were converted to cell numbers per well (against a series of standards) for each of the treatment groups.
  • Figure 5 shows the effect of ConA stimulation on T-lymphocytes cells grown in the presence of a variety of matrices at 72h. Total counts reflect the level of thymidine uptake and incorporation into DNA, which is then used as a measure of proliferation (see in the previous gi'aph). A 72h culture is regarded as the best measure of time for comparison between treatments as the cells are well within exponential phase growth.
  • Unprimed T cells were shown to proliferate at the same degree in the presence or absence of the matrices. This showed the biomaterials were not non-immunogenic but instead inert. No single matrix tested stimulated the normal immune response to any degree greater than the control (no matrix well series).
  • the tested matrices do not interfere with the body's cell-mediated immune response and are biocompatible with a sheep T lymphocyte cell line. In vivo testing
  • the effect of keratin matrices in a wound environment was determined using an animal model.
  • a randomised trial was conducted applying 4 samples to groups of rats with excision wounds. There were 6 male rats per group. Two wounds (8 mm diameter) were established on the back of each rat along the mid-line. One wound served as the control with the veliicle or saline was applied and the test material was applied to the other wound. The rate of healing was monitored by regular photographs. The wounds were photographed every second day and the area of the healing wounds were quantified. The percentage (%) change for each wound was determined at each time point and relative rate of healing of the experimental to the control wound determined for each rat. The mean difference at each time was then calculated and is detailed in table 4.
  • KP-U Keratin membrane wound dressing
  • KP-T Keratin membrane wound dressing
  • HG-GL Keratin hydrogel
  • HG-O Keratin hydrogel
  • HG-C commercially available hydrogel wound dressing product.
  • Results based on wound healing rate can be summarized as follows: i) the HG-GL wound dressing material significantly hastened the healing, with the most marked difference occurring in the early stages of healing, ii) the KP-T wound dressing material showed some improvement in healng rate, especially over the first 3 to 5 days.
  • KP-U Keratin membrane wound dressing (example 1)
  • KP-T Keratin membrane wound dressing (example 3)
  • HG-GL Keratin hydrogel (example 4)
  • HG- O Keratin hydrogel (example 2)
  • HG-C commercially available hydrogel wound dressing product.
  • S-sulfonated keratin intemiediate filament protein (SIFP) solution was prepared using of S-sulfonated keratin intermediate filament protein powder dissolved in distilled water with gradual addition of 1M NaOH over 2 hours under mechanical stirring. The pH was maintained in the range 8.0-9.5, and finally adjusted to 8.5.
  • the keratin protein solution was centrifuged at 27000 g for 10 mins in order to remove any air bubbles and undissolved material.
  • the resulting keratin protein solution was cast into a pettri dish and the solvents evaporated under ambient conditions to leave a keratin membrane.
  • the solvent can also include some percentage of organic based aqueous miscible solvent, such as an alcohol.
  • Example 2 PRODUCTION OF A KERATIN HYDROGEL FOR USE IN WOUND CARE PRODUCTS
  • SIFP S-sulfonated keratin intermediate filament protein
  • PVA polyvinyl alcohol
  • PVP polyvinyl pyrrolidone
  • the combined solution was then cast, and hardened through a freezing- thawing cycle to produce a keratin based hydrogel. This involved freezing the material at -80°C for 1 hr and thawing at 23 °C for 1 hour. Tins freeze-thaw cycle was repeated up to 7 times to obtain a hydrogel. The resulting hydrogel was washed with distilled water multiple times to remove any unreacted keratin and polymers.
  • membranes were treated with reductants to induce chemical cross-linlcing.
  • Immersion of the membranes in a solution of 0.25M ammonium thioglycollate adjusted to pH 7.0 for 60 minutes was used to remove the sulfonate group from the S-sulfonated keratin protein (SIFP), and allow the formation of disulfide bonds (-S-S-).
  • SIFP S-sulfonated keratin protein
  • -S-S- disulfide bonds
  • SIFP 0.25M ammonium thioglycollate solution
  • S-sulfonated keratin intermediate filament protein (SIFP) solution was prepared as describe in Example 1.
  • NH4TG 0.25M ammonium thioglycollate solution
  • the blended solution was then cast, and hardened through a freezing- thawing cycle to produce a disulfide cross-linked keratin hydrogel. This involved freezing the material at -80°C for 1 hour and thawing at 23 °C for 1 horn-. Tins freeze- thaw cycle was repeated up to 7 times to obtain a chemical cross-linked hydrogel.
  • Example 7 PRODUCTION OF AN UNCROSSLINKED KERATIN HYDROGEL FOR USE IN A WOUND CARE PRODUCT A 10%) S-sulfonated keratin intermediate filament protein (SIFP) solution was prepared as describe in Example 1. The solution was cast, and hardened through a freezing- thawing cycle to produce a keratin based hydrogel. This involved freezing the material at -80°C for 1 hour and thawing at 23 °C for 1 hour. This freeze-thaw cycle was repeated up to 7 times to obtain a keratin protein hydrogel.
  • SIFP S-sulfonated keratin intermediate filament protein
  • the invention will be useful in a wide range of wound care products. Such products will assist in the healing and rate of healing of wounds by providing a biochemical environment around the wound site that induces healing.

Abstract

The invention relates to a wound care product that provides a biochemical environment around a wound to promote wound healing. The wound care product includes a keratin protein fraction material in which the protein fraction is intact, is from the intermediate filament protein family or the high sulphur protein family and in which the protein fraction is s-sulfonated. The invention also describes a method of making a wound care product.

Description

WOUND CARE PRODUCTS CONTAINING KERATIN
Field The invention relates to wound care products containing keratin.
Background of the invention
Wounds and lesions can be caused by a variety of events, including surgery, traumatic injury, burns, abrasions and skin grafts. Healing of wounds may be difficult and may result in problems such as ulcers and septicemia. Of particular concern are clironic wounds, such as pressure sores and diabetic ulcers. The treatment of these conditions is of increasing importance as the population ages. The conventional cascade of biochemical processes which occurs in wound healing, involving hemostasis and inflammation, granulation tissue formation and reepithelization and remodeling, is disrupted in the case of clironic wounds due in part to the prolonged inflammatory response which occurs, and the release of destructive enzymes by inflammatory cells.
It has been recognized for some time that maintaining a moist environment can improve the rate of wound healing. Many products have been developed which provide this environment in order to increase the rate of repair of clironic wounds. The materials used in these dressings are biocompatible to some extent, and include polylactic acid, chitin, alginate derivatives and collagen. The response of these materials to wound exudates, and the biochemical environment that these materials provide are fundamental to their performance in the wound.
Commercially available dressings include various synthetic materials such as silicone compounds, nylon fabrics, or petrolatum gauzes and the like [A. J. Platt, A. Phipps and K. Judkins, A comparative study of silicone net dressing and paraffin gauze dressing in skin-grafted sites, Burns, 22(7), 1996, p. 543-545; Claudia Valenta and Barbara G. Auner, The use of polymers for dermal and transdemial delivery, European Journal of Pharmaceutics and Biopharmaceutics, 58(2), 2004, p. 279-289]. Whilst these conventional wound dressing materials are inexpensive and easily available, they generally have poor affinity with the wounded area, insufficient vapour permeability are ultimately unsatisfactory with regards to long term healing of clironic wounds [Marcel F. Jonkman, Izaak Molenaar, Paul Nieuwenhuis, Peter Bruin and Albert .1. Pennings, New method to assess the water vapour permeance of wound coverings, Biomaterials, 9(3), 1988, p. 263-267], High-performance wound dressing materials are often derived from natural materials having properties similar to those of the patients' skin.
Wound dressing can be created using natural materials or through combination of synthetic materials and natural materials (JP# 47470/1988; Jen Ming Yang and Hao Tzu Lin, Properties of chitosan containing PP-g-AA-g-NIPAAm bigraft nonwoven fabric for wound dressing. Journal of Membrane Science, 243(1-2), 2004, p. 1-7). The use of wound dressings is an extremely important part of wound management and vital to achieve successful healing outcomes [Gordon Freedman, Hyacinth Entero and Harold Brem, Practical treatment of pain in patients with chronic wounds: pathogenesis-guided management, The American Journal of Surgery, 188(1), 2004, p. 31-35]. An optimum wound dressing protects the injured tissue, maintains a moist environment, is water permeable, maintains microbial control, delivers healing agents to the wound site, is easy to apply, does not require frequent changes and is non-toxic and non-antigenic.
Currently several forms of wound dressings materials are available commercially, including occlusive dressings, non-adherent dressings, absorbent dressings, and dressings in the form of sheets, foams, powders and gels. Attempts have been made to provide improved dressings, particularly for chronic wounds, that assist in the wound healing process by using biological materials such as cells and growth factors. To date, these biologicals have proven very costly due to factors such as manufacturing processes and storage and stability issues, and in addition they have shown minimal clinical relevance in accelerating the chronic wound healing process. Above all effective, wound management requires an understanding of the process of tissue repair and knowledge of the properties of the wound dressing materials. Only when these two factors are considered together can the process of dressing selection be undertaken in a rational and informed fashion.
Keratin proteins are present in a wide range of biological tissue, performing a structural role in skin, hair and other materials. Keratins extracted from hair have been shown to be a valuable component in wound dressings. US 5932552 provides a biocompatible keratin material prepared by either reduction or oxidation for use as a component in wound care products. Those methods included in the art for the oxidation of keratins to create a polar group are harsh and degrading to the keratin, causing protein damage and loss of core physical characteristics arising from the protein amino acid composition and tertiary structure. In addition the oxidation processes used in the preparation of these materials are irreversible and the cysteic acid groups formed cannot be reconverted to cystine to perfoπn a useful structural function Those methods included in the art for reduction to create soluble proteins are conducted under harsh alkaline conditions that also cause damage to the protein and loss of the core physical characteristics of the keratin proteins.
The core components of keratin fibres, specifically the intermediate filament proteins and the matrix proteins present in wool and hair, play particular roles within the fibre which is reflected in their tertiary structure and amino acid composition These same features can be capitalized upon to create materials with good physical properties and highly absorbing capacities when using purified forms of these proteins. In order to do this, methods used for isolating keratins need to be mild, to prevent protein damage, create cystine modifications that are reversible, to allow for reconstitution of tough materials tlirough the creation of cystine bonds, and facilitate the isolation of specific keratin protein fractions from the keratin source. The present invention provides new materials for use in wound care products that are prepared according to these principles.
Object of the Invention It is an object of the invention to provide a wound care product which uses a keratin protein fraction. It is a further object of the invention to provide a keratin protein fraction that is intact and S-sulfonated for use in wound care, or to at least provide the public with a useful choice.
Summary of the Invention
The invention provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is intact. The invention also provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is from the intermediate filament protein family.
The invention also provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is from the high sulphur protein family. The invention also provides a material for treating a wound comprising a keratin protein fraction in which the protein fraction is s-sulfonated.
The protein fraction may be hydrolysed.
The protein is preferably s-sulfonated.
The protein may be from the high sulphur protein family. The protein may be an intermediate filament protein.
The material is preferably a fibre, a film, a foam or a hydro gel.
The invention also provides a method a method for making a wound care product comprising a) preparing a 10% solution of a keratin protein; b) mixing the keratin protein and a water soluble polymer to form an intimate mixture; c) casting the aqueous mixture so produced; and d) freezing and thawing in sequence to produce a hydrogel.
The physico-mechanical properties of the biomaterials may be improved by introducing cross-linker agents to form disulfide bonds and thus remove sulfonate functionalities.
The cross-linking agent used as a reductant may be a thiol or thioglycollate salt.
The physico-mechanical properties may be wet and dry strength.
The thioglycollate salt may be ammonium thioglycollate solution.
The water soluble polymer may be polyvinyl alcohol, polyvinylpyrolidone, polyethylene glycol or the like.
The invention also provides a method of improving the wet strength properties of the wound care products produced by the method of the invention by incorporating a cross- liking agent into them.
The cross-linking agent is preferably an aldehyde. The cross-linking agent may be selected form the group consisting of formaldehyde, glyoxal, glutaraldehyde and the like. Brief Description of the Drawings
The invention will now be described, by way of example only, with reference to the following specific embodiments:
Figure 1 shows the response of wounds treated with keratin and other materials Figure 2 shows sheep fibroblast proliferation on keratin materials; Figure 3 shows human fibroblast proliferation on keratin materials; Figure 4 shows the effect of Con(A) stimulation on T-cell growth in the presence of keratin matrices; and
Figure 5: shows the effect of Con(A) on stimulation of T-cell growth in the presence of keratin matrices after 72 hours.
Detailed Description of the Invention
The hard alpha keratin proteins such as those derived from human hair, wool, animal fibres, horns, hooves or other mammalian sources, can be classified into particular components according to their biochemical properties, specifically their molecular weight and amino acid composition. Table 1 illustrates the amino acid composition deteπnined by conventional analytical methods of typical keratin protein fractions lαiown in the art and also the subject of tins invention. This involves acid hydrolysis of the analyte which converts all cystine and labile cystine derivatives to cysteine, typically recorded as half-cystine.
Figure imgf000006_0001
Figure imgf000007_0001
Table 1: amino acid composition of keratin fractions: S-sulfonated keratin intermediate filament protein (SIFP), S-sulfonated keratin high sulfur protein (SHSP). S-sulfonated keratin peptide (SPEP) as used in the invention Intermediate filament protein (IFP), high sulfur protein (HSP) and whole wool courtesy of Gillespie and Marshall, Variability in the proteins of wool and hair, Proc. Sixth Int. Wool Text. Res. Conf, Pretoria, 2, 67-77, 1980. All residues expressed as mol%. S-sulfocysteine, cystine and cysteine are measured as S-carboxymethyl cysteine following reduction and alkylation, and reported as cys.
Table 2 illustrates the molecular weight determined by conventional analytical methods of typical keratin protein fractions known in the art and also the subject of this invention. Conventional analysis involves cleavage of cystine bonds within the keratin using reduction so that the protein mass is determined in its native, uncrosslinked state, most similar to the unkeratinsed state of the protein Mass is determined using polyacrylamide gel electrophoresis. In the case of the peptide SPEP mass is determined using mass spectrometry. L sing these methods the keratin is made soluble without any hydrolysis of peptide bonds and an accurate measure of molecular weight is determined.
Figure imgf000007_0002
Table 2: Molecular weight of keratin fractions: S-sulfonated keratin intermediate filament protein (SIFP), S-sulfonated keratin high sulfur protein (SHSP), S-sulfonated keratin peptide (SPEP) as used in the invention. Intermediate filament protein (IFP) and high sulfur protein (HSP) courtesy of Gillespie and Marshall, Variability in the proteins of wool and hair, Proc. Sixth Int. Wool Text. Res. Conf, Pretoria, 2, 67-77, 1980.
Both amino acid composition and molecular weight varies, to a small extent, across keratin types, between species and also within breeds of one species, for example between wools from different breeds of sheep. The figures given in Tables 1 and 2 are indicative for the keratin source stated. However, individual types of keratin proteins, or keratin protein fractions, have distinctive characteristics, particularly molecular weight and amino acid content.
The subject of the invention is materials containing intact S-sulfonated keratin protein fractions. "Intact" refers to proteins that have not been significantly hydrolysed, with hydrolysis being defined as the cleavage of bonds through the addition of water. Gillespie (Biochemistry and physiology of the skin, vol 1, Ed. Goldsmith Oxford University Press, London, 1983, pp475-510) considers "intact" to refer to proteins in the keratinized polymeric state and further refers to polypeptide subunits which complex to form intact keratins in wool and hair. For the purpose of this invention "intact" refers to the polypeptide subunits described by Gillespie. These are equivalent to the keratin proteins in their native foπn without the disulfide crosslinlcs formed tlirough the process of keratinisation.
Keratin protein fractions are distinct groups from within the keratin protein family, such as the intermediate filament proteins, the high sulfur proteins or the high glycine- tyrosine proteins well known in the art. Intermediate filament proteins are described in detail by Orwin et al (Structure and Biochemistry of Mammalian Hard Keratin, Electron Microscopy Reviews, 4, 47,1991) and also referred to as low sulphur proteins by Gilliespie (Biochemistry and physiology of the skin, vol 1 , Ed. Goldsmith Oxford University Press, London, 1983, pp475-510). Key characteristics of tins protein family are molecular weight in the range 40 - 60 kD and a cysteine content (measured as half cystine) of around 4%. The high sulfur protein family are also well described by Orwin and Gillispie in the same publications. This protein family has a large degree of heterogeity but can be characterised as having a molecular weight in the range 10 - 30 kD and a cysteine content of greater than 10%. The subset of this family, the ultra high sulfur proteins can have a cysteine content of up to 34%. The high glycine-tryosine protein family are also well described by Orwin and Gillespie in the same publications. Tins family is also referred to as the high tryrosine proteins and has characteristics of a molecular weight less than 10 kD, a tyrosine content typically greater than 10% and a glycine content typically greater than 20%.
For the purpose of this invention a "keratin protein fraction" is a purified form of keratin that contains predominantly, although not entirely, one distinct protein group as described above. In the context of this invention S-Sulfonated keratins have cysteine/cystine present predominantly in the form S-sulfocysteine, commonly known as the Bunte salt. This highly polar group imparts a degree of solubility to proteins.
Whilst being stable in solution, the S-sulfo group is a labile cysteine derivative, highly reactive towards thiols, such as cysteine, and other reducing agents. Reaction with reducing agents leads to conversion of the S-sulfo cysteine group back to cysteine. S- sulfo cysteine is chemically different to cysteic acid, although both groups contain the
S03 " group. Cysteic acid is produced irreversibly by the oxidation of cysteine or cystine and once formed cannot form disulfide crosslinlcs back to cysteine. S-sulfocysteine is reactive towards cysteine and readily forms disulfide crosslinlcs.
SIFP can be prepared by methods such as those described in WO03011894.
The aspect and other details of the invention will now be more particularly described.
Highly S-sulfonated keratins have been shown to be able to be formed into a variety of matrices including porous sponges, films and fibres using methods such as those outlined inNZ/PCT/00169 (which is incorporated herein).
Purified wool keratin intermediate filament proteins are particularly well suited to reformation into matrices, due in part to their high molecular weight and their tertiary structure. Methods outlined in NZ/PCT/00169 make extensive use of these materials to form useful matrices. S-sulfo keratins can be prepared by a variety of methods, including those outlined in PCT NZ02/00125 (which is incorporated herein).
Porous sponge matrices are of particular use in a wound environment as they can play an important role in absorbing wound exudates and maintaining a healthy environment for healing a wound. In addition they can act as media for the delivery of other healing agents, such as growth factors, antibacterial agents or cultured cells, that stimulate the healing process. These features are enhanced through using S-sulfonated keratin protein fractions to construct the matrices. The highly polar nature of the S-sulfo group makes matrices derived from this material highly absorbing. In addition, S-sulfonated keratins are biocompatible and do not invoke an adverse response in vitro.
Films are an important component in dressings for the treatment of wounds, providing a barrier to protect the wound and maintaining an appropriate environment to encourage healing. S-sulfonated keratins films are biocompatible and do not invoice an adverse response in vitro. As such, they are useful components in a wound dressing.
Fibres reconstituted from S-sulfonated keratin intermediate filament proteins can be used as a component for wound dressings. Fibres are particularly versatile as they can be formed into woven or non-woven constructs and fibre design can be used as well control of the chemistry of the material to effect the interaction of the dressing with the wound. Much work has been undertaken into the use of regenerated fibres in wound care, in particular alginate fibres. Reconstituted keratin fibres derived from S- sulfonated intermediate filament proteins are a new material for use in similar applications.
Hydrogels are frequently used in wound dressings and play an in important role in controlling the wound environment and provide a suitable medium for the delivery of actives to stimulate or assist healing. S-sulfonated keratins, in particular S-sulfonated intact keratin intermediate filament protein, is an excellent substrate for the formation of hydrogels as a result of the high degree of order and intermolecular interaction achievable as a result of the intact nature of the proteins.
Keratin materials derived from the SIFP and SHSP protein fractions contain differing amounts of the highly polar S-sulfo group, and consequently differ in their physicochemical characteristics, in particular their ability to absorb moisture Wound dressings derived from a combination of these absorb moisture to a greater or lesser extent, and so can be controlled in the degree to which they will absorb wound exudates.
S-sulfonated keratin proteins prepared as spray or freeze dried powders are highly absorbing materials that are a valuable component in wound dressings, in particular for use in the hydrogel type dressing in which alginates or collagen derivatives are the materials used frequently in currently available products. Combination of the SIFP and SHSP proteins leads to a degree of control over the absorbing capacity of the powder and the nature of the gel formed on absorbance, due to the variation in the amount of S- sulfo groups present within each protein fraction.
Due to the intact nature of the proteins, and the water solubility of the material arising from the presence of the polar S-sulfonate group, S-sulfonated keratin protein fractions, in particular the keratin intermediate filament protein fraction, can be readily formed into a variety of matrices and the physical properties of these matrices are such that they can provide a useful physical role in a wound environment. Furthermore, the materials can be chemically treated following reformation into films, fibres or sponges, to remove the S-sulfonate functionality and generate disulfide crosslinks within the material, similar to those present in the native keratin. Methods for this treatment are described in
NZ/PCT/00169. When treated in this way, the keratin matrices are less absorbing and retain their structure in a wound environment. They are well suited to the delivery of bioactives to the wound site, such as antibacterial agents, growth factors, antibiotic treatments, cultured cells or other drugs. The physical and mechanical properties of the wound dressing or healing membranes can be readily improved through a variety of methods. One method involves treatment with a reducing reagent such as ammonium thioglycolate solution at pH = 7.0 for 1 hour in order to remove the sulfonate functionality from S-sulfonate keratin and introduce cystine disulfides as crosslinlcs. This causes significant improvement in the mechanical properties particularly wet strength of the membranes materials. Chemical conversion is confirmed using Fourier-Transform Infra-Red (FT-IR) spectroscopic studies as the S- sulfonated group gives rise to a strong and sharp absorbance at 1022 cm"1 which is observed to disappear on exposure of the S-sulfonated to the reagents described.
A method for the improvement of the physical and mechanical strength of keratin hydrogel biomaterials is to increase the hydrogen bonding network between the keratin protein chains or the keratin protein and other polymers, such as polyvinyl alcohol and polyvinyl pyrolidone. This can be achieved by using a freezing-thawing process during the constructing hydrogel sheets. This is confirmed by an increase in the insolubility of hydrogels formed using this process.
Production of a chemically cross-linked hydrogel biomaterial is another embodiment in the invention. Improving physical properties such as insolubility and strength in swollen states can be achieved by using chemical cross-linkers such as glutaraldehyde, that allow the formation of chemical cross-links between keratin protein chains.
Further, the physical properties of the keratin based membranes and hydrogels can be increased by standard protein cross-linking methods including using, typical chemical cross-linkers such as, glutaraldehyde, formaldehyde, carbodiimides, e.g., l-efhyl-3- (dimethyaminopropyl)carbodiimide, 2,5-hexanedione, diimidates, e.g., dimethylsuberimidate, or bisacrylamides, e.g., N,N'-methylenebisacrylamide.
In vitro testing The biological response for the materials described above has been determined in vitro through growth of cells relevant in wound healing, and immunogenic response, specifically fibroblasts and lymphocytes.
Figure imgf000013_0001
Table 3: Keratin materials tested in vitro.
Sheep Fibroblasts:
Figure 2 is a graph showing the effect of different keratin matrices on ovine deπnal fibroblast cell proliferation relative to cell media alone (control). Parallel samples of n = 3 were used for each time point.
The proliferation kinetics of ovine fibroblasts on most of the keratin matrices is similar Wells are initially seeded with -10,000 cells (0 hours). During the first 24h post- seeding, the culture experiences a lag time as evidenced by the decline in cell numbers. This phenomenon has been recognised in all assays perforaied and the drop is observed in control wells in addition to those containing the test materials. Additional shorter time-course experimentation has shown that this lag time lasts for less than 12h (data not shown) and that the exponential phase of growth begins at this point Population doublings occur approximately every 24h-48h with subconfluency (approximately 80%> confluencv) marking the end of logaritlimic growth. This corresponds to the end of the experimental time course (5 days or 120h). Extended time-course experiments have indicated a plateau in cell growth shortly after this with full confluence of the culture. Contact inhibition and depletion of nutrients play a key role in limiting the growth rate at this point and the monolayer culture exhibits signs of cell death (i.e. loss of membrane integrity, reduction in cell numbers, vacuolisation of individual cells).
Such kinetics are exhibited by sheep fibroblasts on most of the biopolymer substrates, particularly the films and sponge samples. With respect to the individual matrix types, the following observations were made:
Films. The films with the disulfide chemical configuration support sheep fibroblast growth most satisfactorily (material D). A second sodium S-sulfonate salt configuration demonstrated by film material C supports cell growth to a lesser degree and tends to swell in culture. Cells on these films showed typical multi- or bipolar elongated fibroblastic morphology with good spread.
Sponge. Fibroblast growth porous sponge material B (disulfide configuration) matched that of some of the better films. During the assay, cells were witnessed to attach to the upper surface of the sponge. By light microscopy, the morphological appearance of these cells was deemed similar on all substrates compared to the no-matrix control. Cells were observed by microscopy to infiltrate the sponge material.
Powder. A keratin powder dilution series was established and the result presented in the graph as material E. This result represents the observed growth curve for the concentration 2mgml"1. Higher concentration solutions than this resulted in the same curve, lower demonstrated a slightly higher cell proliferation rate than the control. Extract tests suggest the keratin powder itself may be, at sufficient concentration, mitogenic for sheep fibroblasts.
Human Fibroblasts:
Figure 3 is a graph showing the effect of different keratin matrices on human dermal fibroblast cell proliferation relative to cell media alone (control)
Human fibroblastic data for the corresponding keratin substrates more or less mirrored that observed with the sheep cell line. Again a typical growth curve was established over the 120h period, however 100% confluence was reached in the control wells by the end of this time. At 120h, cultures grown in the presence of the majority of test materials ranged from 83-89% confluence. Sheep Lymphocytes
Figure 4 demonstrates the effect of ConA stimulation on T cells grown in the presence/absence of keratin matrices over a 10-day period. Tritiated thymidine counts were converted to cell numbers per well (against a series of standards) for each of the treatment groups.
Resulting analysis suggests:
1. There is a marked difference in cell numbers over the 240h experiment between ConA stimulated and non-activated sheep T lymphocyte cells. Control (grown in the absence of keratin biopolymers) cell numbers show a 6-fold difference between unstimulated and stimulated cells at 240h. Cells grown in the absence of conA reached concentrations of 50000 cells/well at Day 10, whilst control cells with ConA supplementation exceeded 300000 cells/well at the same point. Such high concentrations were obtainable as the cells were maintained in suspension culture therefore reduced nutrient supply and not surface area requirement was the limiting factor.
2. There was little difference in cell proliferation rates between sample (matrix presence) and control (matrix absence) wells. This effect was noted for both stimulated cells and unstimulated cells. In other words: (a) Unstimulated cells grown in the presence of matrices proliferated at the same degree as those grown purely on tissue culture reference wells. This indicates that although the keratin biomaterials are not non- immunogenic, they look to be antigenically inert If they were non- immunogenic, one would expect no proliferation of lymphocytes exposed to the biomaterial. If indeed it is inert, cell proliferation rates would mimic those of the control as appears the case.
(b) Stimulated cells grown in the presence of the matrices proliferated at a similar rate or slightly higher than the control wells (which contained no keratin matrix). This suggests the activated T-cells are not being inhibited in any way by the matrix itself or any degradative by-products it may produce over this short time-course. Failure to inhibit active T- cells by the tested biomaterials demonstrates the product does not interfere with the normal cell-mediated immune response.
Figure 5 shows the effect of ConA stimulation on T-lymphocytes cells grown in the presence of a variety of matrices at 72h. Total counts reflect the level of thymidine uptake and incorporation into DNA, which is then used as a measure of proliferation (see in the previous gi'aph). A 72h culture is regarded as the best measure of time for comparison between treatments as the cells are well within exponential phase growth.
The results are presented as a vertical bar graph with stimulated and non-stimulated treatments beside each other. Error bars represent means ± SD for n = 3. The unstimulated well counts (unlabelled) show very little variation with small error scores Total counts for stimulated cells are slightly more variable although student T test analyses indicate only the material C is significantly different (p = 0.075) from the control.
Unprimed T cells were shown to proliferate at the same degree in the presence or absence of the matrices. This showed the biomaterials were not non-immunogenic but instead inert. No single matrix tested stimulated the normal immune response to any degree greater than the control (no matrix well series).
Activated T cells maintained in culture with keratin matrices proliferated normally at a similar or greater than rate compared to those of the control (no matrix present). This demonstrates the biomaterials are biocompatible with stimulated T cells, mitogenic to a degree and most certainly do not interfere with the normal immune response. There was no inhibition of activated T cells by any matrix or its byproducts.
In summary, the tested matrices do not interfere with the body's cell-mediated immune response and are biocompatible with a sheep T lymphocyte cell line. In vivo testing
The effect of keratin matrices in a wound environment was determined using an animal model.
A randomised trial was conducted applying 4 samples to groups of rats with excision wounds. There were 6 male rats per group. Two wounds (8 mm diameter) were established on the back of each rat along the mid-line. One wound served as the control with the veliicle or saline was applied and the test material was applied to the other wound. The rate of healing was monitored by regular photographs. The wounds were photographed every second day and the area of the healing wounds were quantified. The percentage (%) change for each wound was determined at each time point and relative rate of healing of the experimental to the control wound determined for each rat. The mean difference at each time was then calculated and is detailed in table 4.
The dressings studied were: KP-U: Keratin membrane wound dressing (example 1), KP-T: Keratin membrane wound dressing (example 3), HG-GL: Keratin hydrogel (example 4), HG-O: Keratin hydrogel (example 2), HG-C commercially available hydrogel wound dressing product.
Twenty-four rats were used in the trial and trial studies were carried up to healing endpoint.
Results based on wound healing rate can be summarized as follows: i) the HG-GL wound dressing material significantly hastened the healing, with the most marked difference occurring in the early stages of healing, ii) the KP-T wound dressing material showed some improvement in healng rate, especially over the first 3 to 5 days.
Days after wounc Wound area, % of original administration KP-U KP-T HG-O HG-GL HG-C Blank 1 100 100 100 100 100 100 3 102 90 97 77 97 93 5 94 90 81 70 90 84 9 64 69 - - - - 11 39 35 24 40 36 13 28 24 23 13 25 23 15 15 11 19 9 13 18 17 18 11 14 5 6 12 19 5 3 8 2 6
Table 4: Area occupied by wound site following administration of various wound dressings. KP-U: Keratin membrane wound dressing (example 1), KP-T: Keratin membrane wound dressing (example 3), HG-GL: Keratin hydrogel (example 4), HG- O: Keratin hydrogel (example 2), HG-C commercially available hydrogel wound dressing product.
Examples
The methods for the preparation of various forms of keratin are now described by way of example.
Example 1: PRODUCTION OF KERATIN MEMBRANES FOR USE IN A WOUND CARE PRODUCT
A 10%) S-sulfonated keratin intemiediate filament protein (SIFP) solution was prepared using of S-sulfonated keratin intermediate filament protein powder dissolved in distilled water with gradual addition of 1M NaOH over 2 hours under mechanical stirring. The pH was maintained in the range 8.0-9.5, and finally adjusted to 8.5. The keratin protein solution was centrifuged at 27000 g for 10 mins in order to remove any air bubbles and undissolved material. The resulting keratin protein solution was cast into a pettri dish and the solvents evaporated under ambient conditions to leave a keratin membrane. The solvent can also include some percentage of organic based aqueous miscible solvent, such as an alcohol. Example 2: PRODUCTION OF A KERATIN HYDROGEL FOR USE IN WOUND CARE PRODUCTS
A 10% S-sulfonated keratin intermediate filament protein (SIFP) solution was prepared as describe in Example 1. The solution was then intimately mixed with water soluble polymers such as, polyvinyl alcohol (PVA) comprising 20% solid content and polyvinyl pyrrolidone (PVP) comprising 10% solid content to a achieve a optimum rheology and optimal composition i.e., SIFP: PVA: PVP = 100: 60: 40 (w/w, %) for creating hydrogel. The combined solution was then cast, and hardened through a freezing- thawing cycle to produce a keratin based hydrogel. This involved freezing the material at -80°C for 1 hr and thawing at 23 °C for 1 hour. Tins freeze-thaw cycle was repeated up to 7 times to obtain a hydrogel. The resulting hydrogel was washed with distilled water multiple times to remove any unreacted keratin and polymers.
Example 3: PRODUCTION OF CROSS-LINKED KERATIN MEMBRANES FOR USE IN A WOUND CARE PRODUCT
In order to improve the physical strength and also mechanical properties of materials produced as described in Example 1 membranes were treated with reductants to induce chemical cross-linlcing. Immersion of the membranes in a solution of 0.25M ammonium thioglycollate adjusted to pH 7.0 for 60 minutes was used to remove the sulfonate group from the S-sulfonated keratin protein (SIFP), and allow the formation of disulfide bonds (-S-S-). The resulting membranes were washed multiple times with distilled water to remove any residual reagents.
Example 4: PRODUCTION OF CHEMICAL CROSS-LINKED KERATIN HYDROGEL FOR USE IN A WOUND CARE PRODUCT
Following preparation of the keratin, PVA, PVP solution as described in example 2, 0.05% to 0.1%o of glutaraldehyde cross-linlcing agent was added into the blended solution. The combined solution was then cast, and hardened tlirough a freezing- thawing cycle to produce a keratin based hydrogel. This involved freezing the material at -80°C for 1 hr and thawing at 23 °C for 1 hour. This freeze-thaw cycle was repeated up to 7 times to obtain a hydrogel. The resulting hydrogel was washed with distilled water multiple times to remove any unreacted keratin and polymers, as well residues of unreacted glutaraldehyde. Physical observation showed significant improvement oftheir dimension stability or strength. These characteristics are also confirmed by the hydrogels insolubility behaviour in aqueous solvent, after having been made as an intimate blending keratin protein and polymers from an aqueous solvent (i.e., water).
Example 5: PRODUCTION OF DISULFIDE CROSS-LINKED KERATIN MEMBRANE FOR USE IN A WOUND CARE PRODUCT
A 10%o S-sulfonated keratin intermediate filament protein (SIFP) solution was prepared as describe in Example 1. The solution was then intimately mixed with 1% of 0.25M ammonium thioglycollate solution (NFLTG), where compositions are as: SIFP: NH4TG = 99 : 1 (w/w, %>). The blended solution was then cast into a petri dish and the solvents evaporated under ambient conditions to create a disulfide cross-linked keratin membrane. The resulting membrane was washed with distilled water multiple times to remove any residual NH TG.
Example 6: PRODUCTION OF DISULFIDE CROSS-LINKED KERATIN HYDROGEL FOR USE IN A WOUND CARE PRODUCT
A 10%) S-sulfonated keratin intermediate filament protein (SIFP) solution was prepared as describe in Example 1. The solution was then intimately mixed with 1%> of 0.25M ammonium thioglycollate solution (NH4TG), where compositions were: SIFP: NFLTG = 99 : 1 (w/w, %>). The blended solution was then cast, and hardened through a freezing- thawing cycle to produce a disulfide cross-linked keratin hydrogel. This involved freezing the material at -80°C for 1 hour and thawing at 23 °C for 1 horn-. Tins freeze- thaw cycle was repeated up to 7 times to obtain a chemical cross-linked hydrogel.
Example 7: PRODUCTION OF AN UNCROSSLINKED KERATIN HYDROGEL FOR USE IN A WOUND CARE PRODUCT A 10%) S-sulfonated keratin intermediate filament protein (SIFP) solution was prepared as describe in Example 1. The solution was cast, and hardened through a freezing- thawing cycle to produce a keratin based hydrogel. This involved freezing the material at -80°C for 1 hour and thawing at 23 °C for 1 hour. This freeze-thaw cycle was repeated up to 7 times to obtain a keratin protein hydrogel.
Industrial Applicability
The invention will be useful in a wide range of wound care products. Such products will assist in the healing and rate of healing of wounds by providing a biochemical environment around the wound site that induces healing.

Claims

CLAIMS:
1. A material for treating a wound comprising a keratin protein fraction in which the protein fraction is intact.
2. A material for treating a wound comprising a keratin protein fraction in which the protein fraction is from the intermediate filament protein family.
3. A material for treating a wound comprising a keratin protein fraction in which the protein fraction is from the high sulphur protein family.
4. A material for treating a wound comprising a keratin protein fraction in which the protein fraction is s-sulfonated.
5. A material for treating a wound comprising a keratin protein fraction according to any one of claims 2-4 in which the protein fraction is hydrolysed.
6. A material for treating a wound according to any one of claims 1, 2, 3 or 5 in which the protein is s-sulfonated.
7. A material for treating a wound according to any one of claims 1, 4 or 5 in which the protein is from the high sulphur protein family.
8. A material for treating a wound according to any one of claims 1 or 4-5 in which the protein is an intemiediate filament protein.
9. A material according to any preceding claim wherein the material is selected from the group consisting of: a fibre, a film, a foam, and a hydrogel.
10. A method for making a wound care product comprising (a) preparing a 10% solution of a keratin protein; (b) mixing the keratin protein and a water soluble polymer to form an intimate mixture; (c) casting the aqueous mixture so produced; and (d) freezing and thawing in sequence to produce a hydrogel.
11. A method according to claim 10 in which the physico-mechanical properties of the biomaterials are improved by introducing cross-linker agents to form disulfide bonds and thus remove sulfonate functionalities.
12. A method according to claim 11 in wliich the cross-linlcing agent used as a reductant is a thiol or thioglycollate salt.
13. The method according to claim 11 or claim 12 in which the physico-mechanical properties are wet and dry strength.
14. A method according to claim 12 in which the thioglycollate salt is ammonium thioglycollate solution.
15. The method according to any one of claims 10-14 wherein the keratin protein is s- sulfonated.
16. The method according to any one of claims 10-15 wherein the keratin protein is a protein fraction.
17. A method according to claim 16 in which the protein fraction is intact.
18. The method according to claim 16 or 17 wherein the keratin protein is from the intermediate filament protein family.
19. A method according to any one of claims 10-18 wherein the water soluble polymer is selected from the group consisting of polyvinyl alcohol, polyvinylpyrolidone, polyethylene glycol and the like.
20. A method of improving the wet strength properties of the wound care products produced by the method of any one of claims 10-19 by incorporating a cross- linlcing agent into them.
21. A method according to claim 20 in which the cross-linlcing agent is an aldehyde.
22. A method according to claim 21 in which the cross-linlcing agent is selected from the group consisting of formaldehyde, glyoxal, glutaraldehyde and the like.
PCT/NZ2004/000323 2003-12-19 2004-12-16 Wound care products containing keratin WO2005058380A1 (en)

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Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2008040357A1 (en) * 2006-10-02 2008-04-10 Coloplast A/S Cross-linking of foams of s-sulfonated keratin
EP2099437A2 (en) * 2006-12-11 2009-09-16 Keratec Limited Porous keratin construct and method of making the same
US9045600B2 (en) 2009-05-13 2015-06-02 Keraplast Technologies, Ltd. Biopolymer materials

Families Citing this family (20)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2005028560A1 (en) * 2003-09-19 2005-03-31 Keratec Limited Composite materials containing keratin
US8030615B2 (en) * 2008-06-20 2011-10-04 Bowling Green State University Method and apparatus for detecting organic materials and objects from multispectral reflected light
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US9023399B2 (en) 2012-11-16 2015-05-05 NU Technology, LLC Water-soluble anti-inflammatory cream with natural ingredients base
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JP2017516869A (en) * 2014-06-04 2017-06-22 ジム バイオサイエンシズ,インコーポレイテッド Compositions and methods for improving skin quality
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US10723774B2 (en) * 2016-11-17 2020-07-28 University Of South Carolina Keratin-based hydrogels
CN109881279B (en) * 2018-03-26 2021-08-03 新乡化纤股份有限公司 Ion liquid method for regenerating animal keratin fiber and preparation method thereof
CN111202868B (en) * 2020-01-17 2022-01-28 重庆大学 Composition for preparing keratin gel dressing, preparation method and application thereof
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CN113209361B (en) * 2021-04-01 2022-05-31 南京医科大学 Biological material composite hydrogel wound dressing and preparation method thereof

Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPS6347470B2 (en) 1984-04-16 1988-09-22 Terumo Corp
US5932552A (en) 1997-11-26 1999-08-03 Keraplast Technologies Ltd. Keratin-based hydrogel for biomedical applications and method of production
WO2003011894A1 (en) 2001-07-17 2003-02-13 Keratec Limited The production of soluble keratin derivatives
WO2003103737A1 (en) * 2002-06-10 2003-12-18 Wool Research Organisaton Of New Zealand (Inc) Orthopaedic materials derived from keratin
AU2002330798B2 (en) * 2001-08-31 2007-06-21 Keratec Limited The production of biopolymer film, fibre, foam and adhesive materials from soluble S-sulfonated keratin derivatives

Family Cites Families (64)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US2591945A (en) * 1948-11-12 1952-04-08 Botany Mills Inc Process for the recovery of protein from wool and other keratinous materials
US3567363A (en) * 1965-09-20 1971-03-02 Gillette Co Modification of keratin to the s-sulfo form
NO125657B (en) 1965-09-20 1972-10-16 Gillette Co
US3644084A (en) * 1968-11-25 1972-02-22 Gillette Co Treatment of keratin fibers
US3619116A (en) * 1969-04-02 1971-11-09 Thomas Burnley & Sons Ltd Method for scouring wool
US3883647A (en) * 1972-12-06 1975-05-13 Ives Lab Tablet formulation
JPS537760A (en) * 1976-07-12 1978-01-24 Agency Of Ind Science & Technol Modified keratin membrane
US4172073A (en) * 1976-11-09 1979-10-23 Chemetron Corporation Method for the preparation of water-soluble keratinaceous protein using saturated steam and water
JPS53119900A (en) 1977-03-23 1978-10-19 Agency Of Ind Science & Technol Preparation of aqueous solution of high viscosity and high molecular weight keratin
JPS609531B2 (en) 1978-04-17 1985-03-11 積水化学工業株式会社 Method for manufacturing porous membrane material
JPS57144213A (en) * 1981-03-03 1982-09-06 Kao Corp Hair treatment
FR2521571B1 (en) * 1982-02-17 1986-07-18 Oreal KERATINIC POLYMER WITH S-SULFOCYSTEIN RESIDUES, PREPARATION METHOD THEREOF AND TREATMENT COMPOSITION THEREOF
US4407793A (en) * 1982-05-26 1983-10-04 Akimova Alla Y Composition for temporary substitution of bone tissue defects
JP2723203B2 (en) * 1984-01-06 1998-03-09 ザ リージェンツ オブ ザ ユニバーシティ オブ カリフォルニア Cytokeratin tumor markers and assays for their detection
US4904602A (en) * 1985-11-27 1990-02-27 Repligen Corporation Thioredoxin shufflease and use thereof
JPH0737480B2 (en) 1987-06-01 1995-04-26 花王株式会社 Method for producing water-soluble keratin
US5154916A (en) * 1988-04-07 1992-10-13 L'oreal Eyelash make-up composition based on wax and keratin hydrolysate
US4973475A (en) * 1988-10-07 1990-11-27 Revlon, Inc. Hair treatment and conditioning agents
US4969880A (en) * 1989-04-03 1990-11-13 Zamierowski David S Wound dressing and treatment method
JP2777196B2 (en) 1989-06-06 1998-07-16 株式会社成和化成 Method for producing keratin hydrolyzate
JP2907938B2 (en) 1990-04-13 1999-06-21 株式会社成和化成 Cosmetic base
US5292362A (en) 1990-07-27 1994-03-08 The Trustees Of Columbia University In The City Of New York Tissue bonding and sealing composition and method of using the same
GB9119984D0 (en) * 1991-09-19 1991-11-06 Scholl Plc A hydrogel and process for the manufacture thereof
JPH05222100A (en) 1992-02-14 1993-08-31 San Orient Kagaku Kk Production of reduced-type keratin peptide
FR2687577B1 (en) 1992-02-26 1995-06-30 Icp Sa BIOMATERIAL FOR THE PRODUCTION OF PRODUCTS APPLICABLE IN HUMAN MEDICINE PARTICULARLY IN ORTHOPEDICS AND ITS MANUFACTURING METHOD.
JPH05320358A (en) 1992-05-22 1993-12-03 Ajinomoto Takara Corp:Kk Keratin protein article molded by high-pressure molding
JP3283302B2 (en) 1992-09-22 2002-05-20 株式会社成和化成 Method for producing reduced keratin
US5358935A (en) * 1992-11-19 1994-10-25 Robert Allen Smith Nonantigenic keratinous protein material
JP2527120B2 (en) 1992-12-24 1996-08-21 共栄社化学株式会社 Method for producing hard keratin substance powder
JPH06220713A (en) 1993-01-28 1994-08-09 Toray Ind Inc Production of polyvinyl alcoholic fiber
CN1105029A (en) * 1993-05-24 1995-07-12 花王株式会社 Process for producing solubilized protein
US5316942A (en) * 1993-06-16 1994-05-31 Battelle Memorial Institute Process for the production of low-cost soluble high-molecular weight collagen
US5602094A (en) * 1994-03-29 1997-02-11 Goddard; David Treatment of tumors
FR2725130B1 (en) 1994-09-29 1996-10-31 Oreal COSMETIC COMPOSITIONS CONTAINING A CERAMID-LIKE COMPOUND AND A FATTY CHAIN PEPTIDE, AND USES THEREOF
GB9721585D0 (en) 1997-10-10 1997-12-10 Geistlich Soehne Ag Chemical product
US6013250A (en) 1995-06-28 2000-01-11 L'oreal S. A. Composition for treating hair against chemical and photo damage
FR2740036B1 (en) * 1995-10-20 1997-11-28 Oreal NOVEL OXIDIZING COMPOSITION AND NEW PROCESS FOR PERMANENT DEFORMATION OR HAIR DECOLORATION
EP1704878B1 (en) * 1995-12-18 2013-04-10 AngioDevice International GmbH Crosslinked polymer compositions and methods for their use
US5866165A (en) * 1997-01-15 1999-02-02 Orquest, Inc. Collagen-polysaccharide matrix for bone and cartilage repair
US6348201B2 (en) * 1997-05-30 2002-02-19 Kibun Food Chemifa Co., Ltd. External composition for skin comprising sphingoglycolipid
FR2769499B1 (en) 1997-10-10 2000-01-14 Oreal PROCESS OF PERMANENT DEFORMATION OF KERATINIC MATERIAL WITHOUT INTERMEDIATE RINSING
US6110487A (en) * 1997-11-26 2000-08-29 Keraplast Technologies Ltd. Method of making porous keratin scaffolds and products of same
JP3360810B2 (en) * 1998-04-14 2003-01-07 ペンタックス株式会社 Method for producing bone replacement material
US6572845B2 (en) 1998-10-16 2003-06-03 Burt D. Ensley Recombinant hair treatment compositions
AU2414300A (en) 1999-01-15 2000-08-01 Brigham Young University Attachment of acid moiety-containing biomolecules to activated polymeric surfaces
US6696073B2 (en) * 1999-02-23 2004-02-24 Osteotech, Inc. Shaped load-bearing osteoimplant and methods of making same
WO2000054821A1 (en) * 1999-03-16 2000-09-21 Regeneration Technologies, Inc. Molded implants for orthopedic applications
EP1179066A2 (en) 1999-05-19 2002-02-13 Incyte Genomics, Inc. Extracellular signaling molecules
US6762158B2 (en) * 1999-07-01 2004-07-13 Johnson & Johnson Consumer Companies, Inc. Personal care compositions comprising liquid ester mixtures
ES2157807B1 (en) 1999-07-09 2002-03-16 Consejo Superior Investigacion COMPOSITIONS AND EXTRACT USE OF WOOL INTERNAL LIPIDS IN THE PREPARATION OF PRODUCTS FOR THE TREATMENT AND CARE OF THE SKIN.
US6544548B1 (en) * 1999-09-13 2003-04-08 Keraplast Technologies, Ltd. Keratin-based powders and hydrogel for pharmaceutical applications
US6783546B2 (en) * 1999-09-13 2004-08-31 Keraplast Technologies, Ltd. Implantable prosthetic or tissue expanding device
US6270793B1 (en) * 1999-09-13 2001-08-07 Keraplast Technologies, Ltd. Absorbent keratin wound dressing
US20020004068A1 (en) * 2000-01-28 2002-01-10 Isotta Di Drusco Composition
DE10036749A1 (en) 2000-07-28 2002-02-07 Schwarzkopf Gmbh Hans Permanent wave method
US20020183858A1 (en) * 2001-06-05 2002-12-05 Contiliano Joseph H. Attachment of absorbable tissue scaffolds to scaffold fixation devices
EP1406951A1 (en) * 2001-07-13 2004-04-14 Stichting Nederlands Instituut voor Zuivelonderzoek Keratin-based products and methods for their production
CN1158416C (en) 2001-08-30 2004-07-21 陈福库 Composite kerating fiber and its production process
CN1425813A (en) 2001-12-12 2003-06-25 中国科学院化学研究所 Synthetic fibre containing animal protein and its preparing method
KR100440239B1 (en) * 2002-01-09 2004-07-15 한국원자력연구소 Method for the preparation of hydrogels for wound dressings
US6846940B2 (en) * 2002-01-22 2005-01-25 L'oreal Ceramides, compositions thereof and methods of use thereof
AU2003221870B2 (en) * 2002-04-10 2009-06-04 Keraplast Technologies, Ltd. Heterogeneous protein networks crosslinked with silicone-containing links, and methods for producing them
NZ563477A (en) * 2002-11-28 2010-02-26 Keratec Ltd Personal care formulations containing keratin
US7671012B2 (en) * 2004-02-10 2010-03-02 Biosurface Engineering Technologies, Inc. Formulations and methods for delivery of growth factor analogs

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPS6347470B2 (en) 1984-04-16 1988-09-22 Terumo Corp
US5932552A (en) 1997-11-26 1999-08-03 Keraplast Technologies Ltd. Keratin-based hydrogel for biomedical applications and method of production
WO2003011894A1 (en) 2001-07-17 2003-02-13 Keratec Limited The production of soluble keratin derivatives
AU2002330798B2 (en) * 2001-08-31 2007-06-21 Keratec Limited The production of biopolymer film, fibre, foam and adhesive materials from soluble S-sulfonated keratin derivatives
WO2003103737A1 (en) * 2002-06-10 2003-12-18 Wool Research Organisaton Of New Zealand (Inc) Orthopaedic materials derived from keratin

Non-Patent Citations (10)

* Cited by examiner, † Cited by third party
Title
A.J. PLATT, A. PHIPPS, K. JUDKINS: "A comparative study of silicone net dressing and paraffin gauze dressing in skin-grafted sites", BURNS, vol. 22, no. 7, 1996, pages 543 - 545
CLAUDIA VALENTA, BARBARA G. AUNER: "The use of polymers for dermal and transdermal delivery", EUROPEAN JOURNAL OF PHARMACEUTICS AND BIOPHARMACEUTICS, vol. 58, no. 2, 2004, pages 279 - 289, XP004526312, DOI: doi:10.1016/j.ejpb.2004.02.017
GILLESPIE, MARSHALL: "Variability in the proteins of wool and hair", PROC. SIXTH INT. WOOL TEXT. RES. CONF, PRETORIA, vol. 2, 1980, pages 67 - 77, XP008099318
GILLESPIE, MARSHALL: "Variability in the proteins of wool and hair", PROC. SIXTH INT. WOOL TEXT. RES. CONJ., PRETORIA, vol. 2, 1980, pages 67 - 77, XP008099318
GILLESPIE: "Biochemistry and physiology of the skin", vol. 1, 1983, OXFORD UNIVERSITY PRESS, pages: 475 - 510
GILLIESPIE: "Biochemistry and physiology of the skin", vol. 1, 1983, OXFORD UNIVERSITY PRESS, pages: 475 - 510
GORDON FREEDMAN, HYACINTH ENTERO, HAROLD BREM: "Practical treatment of pain in patients with chronic wounds: pathogenesis-guided management", THE AMERICAN JOURNAL OF SURGERY, vol. 188, no. 1, 2004, pages 31 - 35
JEN MING YANG, HAO TZU LIN: "Properties of chitosan containing PP-g-AA-g-NIPAAm bigraft nonwoven fabric for wound dressing", JOURNAL OF MEMBRANE SCIENCE, vol. 243, no. 1-2, 2004, pages 1 - 7, XP004572516, DOI: doi:10.1016/j.memsci.2004.03.019
MARCEL F. JONKMAN, IZAAK MOLENAAR, PAUL NIEUWENHUIS, PETER BRUIN, ALBERT J. PENNINGS: "New method to assess the water vapour penneanee of wound coverings", BIOMATERIALS, vol. 9, no. 3, 1988, pages 263 - 267
ORWIN ET AL., STRUCTURE AND BIOCHEMISTRY OF MAMMALIAN HARD KERATIN, ELECTRON MICROSCOPY REVIEWS, vol. 4, 1991, pages 47

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2008040357A1 (en) * 2006-10-02 2008-04-10 Coloplast A/S Cross-linking of foams of s-sulfonated keratin
EP2099437A2 (en) * 2006-12-11 2009-09-16 Keratec Limited Porous keratin construct and method of making the same
EP2099437A4 (en) * 2006-12-11 2013-06-19 Keratec Ltd Porous keratin construct and method of making the same
US9045600B2 (en) 2009-05-13 2015-06-02 Keraplast Technologies, Ltd. Biopolymer materials

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US20080038327A1 (en) 2008-02-14
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