WO2009104005A1 - Chronic wound treatment - Google Patents

Chronic wound treatment Download PDF

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Publication number
WO2009104005A1
WO2009104005A1 PCT/GB2009/000504 GB2009000504W WO2009104005A1 WO 2009104005 A1 WO2009104005 A1 WO 2009104005A1 GB 2009000504 W GB2009000504 W GB 2009000504W WO 2009104005 A1 WO2009104005 A1 WO 2009104005A1
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WIPO (PCT)
Prior art keywords
polyphosphate
inhibition
sodium
pepsin
use according
Prior art date
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PCT/GB2009/000504
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English (en)
French (fr)
Inventor
Johnathan Craig Richardson
Peter William Dettmar
Rebecca Louise Allen
Cathal Padraig Coyle
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Technostics Ltd
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Technostics Ltd
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Priority claimed from GB0803284A external-priority patent/GB0803284D0/en
Priority claimed from GB0803283A external-priority patent/GB0803283D0/en
Application filed by Technostics Ltd filed Critical Technostics Ltd
Priority to US12/918,826 priority Critical patent/US20110117208A1/en
Priority to EP09712875A priority patent/EP2254585A1/en
Priority to JP2010547251A priority patent/JP2011512394A/ja
Publication of WO2009104005A1 publication Critical patent/WO2009104005A1/en
Anticipated expiration legal-status Critical
Ceased legal-status Critical Current

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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K33/00Medicinal preparations containing inorganic active ingredients
    • A61K33/42Phosphorus; Compounds thereof
    • 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
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P41/00Drugs used in surgical methods, e.g. surgery adjuvants for preventing adhesion or for vitreum substitution
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P43/00Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00

Definitions

  • the present invention is concerned with chronic wound healing and, in that connection, includes the use of certain compounds, as well as methods of treatment and pharmaceutical compositions.
  • Wound healing is a complex physiological process; however, it normally follows a predictable ordered sequence of events. This sequence has been arbitrarily divided into a series of stages namely (i) an inflammatory phase; (ii) a tissue formation phase and (iii) a tissue regeneration phase. Acute wounds, which are often caused by trauma/surgery, will repair by progressing through these stages in an ordered and timely manner. In contrast, chronic wounds do not follow this ordered sequence and become 'stuck' in the inflammatory phase. This delays the healing process and means certain chronic wounds may never heal or may take years to do so (Rovee DT and Maibach HI in The Epidermis in Wound Healing
  • ECM extracellular matrix
  • fibrous elements e.g. collagen, elastin
  • link proteins e.g. f ⁇ bronectin
  • space filling molecules e.g. hyaluronan
  • ECM degradation is also essential to allow the ECM to remodel so that it can support the synthesis of new tissue.
  • the activity of ECM degrading enzymes in wounds should be reduced to allow a balance between the necessary breakdown and restructuring of existing ECM and the synthesis of new ECM.
  • the persistent activity of degrading enzymes at the site of tissue repair may explain the chronicity of wound healing.
  • studies by numerous researchers have demonstrated that the levels of enzymes that degrade ECM are considerably higher in chronic wounds than in acute wounds. Yager et al (J Invest Dermatol 1996; 107: 743-8) showed that levels of MMP-2 and MMP-9 were significantly higher in wound fluid from chronic pressure ulcers compared to acute surgical wounds.
  • the differing biochemical composition of the wound microenvironment in chronic wounds compared to acute wounds means that the methods of treating these distinct wound types is different.
  • Falanga (Wounds 2002; 14 (2): 47-57) states that using therapeutic agents and wound bed preparation methods suitable for acute wounds are not appropriate for chronic wounds. This is because chronic wounds do not follow the ordered healing stages of acute wounds.
  • Chronic wounds may occur in humans both internally and externally. Internal chronic wounds result from damage to the epithelium of the gastrointestinal tract and can occur as lesions or ulcerations in the oral cavity, throat, oesophagus, stomach, small and large intestine, colon and rectum. External chronic wounds affect the epidermis/dermis and include, for example, diabetic foot ulcers, venous stasis ulcers and pressure ulcers.
  • Gastric juice contains a series of aspartic proteases (Pepsin 1, 3a, 3b, 3c and gastricsin), which are synthesised in the gastric mucosa as an inactive precursor (pepsinogen) and, following stimulation of gastric chief cells, are released into the gastric lumen where they are activated by hydrochloric acid.
  • pepsinogen aspartic proteases
  • the primary function of pepsin is to degrade dietary proteins and peptides into amino acid fragments suitable for absorption. Pepsin does not specifically degrade dietary protein and will indiscriminately cleave any suitable protein, peptide or glycoprotein.
  • the mucus layer can, however, be degraded by pepsin and therefore a dynamic balance exists between mucus secretion and degradation. If this balance is disturbed, and the mucus barrier compromised, pepsin can digest the underlying epithelium and collagen resulting in tissue destruction and gastric injury. Similarly, if pepsin is refluxed beyond the oesophageal sphincter into the aero-digestive tract, extensive tissue damage can occur as the epithelium above this sphincter does not possess the protective mechanisms present in the stomach.
  • the reflux of gastric contents into the oesophagus and larynx may give rise to damage to the squamous epithelium of the oesophagus and larynx and may cause gastroesophageal reflux disease and extra-esophageal reflux disease as well as predisposing the mucosa to Barrett's oesophagus and oesophageal or laryngeal carcinoma.
  • Excess activity of enzymes which degrade ECM contribute to the chronicity of both internal chronic wounds, such as lesions/ulceration of the gastrointestinal tract and external chronic wounds, such as diabetic foot ulcers, venous stasis ulcers and pressure ulcers.
  • ECM including collagenase, hyaluronidase and elastase
  • the proteolytic enzyme pepsin is implicated as the causative enzyme in gastric, oesophageal and laryngeal lesions/ulceration as well as contributing to their delayed healing.
  • enzymes which degrade ECM and structural biomolecules in skin have been implicated as a causative factor in the onset and progression of skin ageing.
  • ECM active enzymes for example aspartic proteinases, such as pepsin, matrix metalloproteinases (MMPs), such as collagenase, serine proteinases, such as elastase, and/or glycoside hydrolases, such as hyaluronidase, may be advantageous in the repair and/or maintenance of a robust ECM.
  • aspartic proteinases such as pepsin
  • MMPs matrix metalloproteinases
  • collagenase such as collagenase
  • serine proteinases such as elastase
  • glycoside hydrolases such as hyaluronidase
  • Polyphosphates are generally linear polymers of many tens or hundreds of orthophosphate residues linked by high-energy, phosphoanhydride bonds. Polyphosphate is found in a broad spectrum of living cells and one of its roles is believed to be to serve as a phosphate storage reservoir for the production of ATP (adenosine triphosphate), which provides the energy to power a cell. Recently, it has been disclosed that in bacteria, polyphosphate helps these single-celled organisms adapt to nutritional deficiencies and environmental stresses. For example, when bacteria are subjected to nutritional deficiencies or environmental stresses (e.g., heat or osmotic pressure), polyphosphate is synthesized to supply the energy necessary for the production of various proteins.
  • ATP adenosine triphosphate
  • the wound dressings are composed of a support matrix, such as cotton cellulose, and an active agent associated with the support matrix.
  • the active agent may be a protease sequestrant, in particular a sequestrant of a neutrophil-derived cationic protease such as elastase.
  • an unbound polyphosphate to promote chronic wound healing, in which the polyphosphate has at least 3 phosphate units.
  • unbound there is meant that the polyphosphate is not chemically bound to any other compound or substrate when it is in active use in wound treatment. Although it may be chemically bound as stored or even as applied, it becomes “unattached” under the treatment conditions. It may be physically bound to, for instance, a substrate carrier but, again, it is essentially behaves as free polyphosphate during treatment.
  • polyphosphates of use in the present invention may be administered, for instance, externally, topically or enterally and may be effective in inhibiting various enzymes including pepsin and those involved in the restructuring of the ECM, such as collagenase, elastase and hyaluronidase.
  • various enzymes including pepsin and those involved in the restructuring of the ECM, such as collagenase, elastase and hyaluronidase.
  • Chronic external wounds such as pressure ulcers, diabetic ulcers etc- the chronicity of these wounds result from excessive activity of collagenase (MMPs), hyaluronidase and elastase; and
  • Chronic internal wounds such as lesions/ulceration of the GI tract- enzymes that degrade
  • ECM are responsible for causing these internal wounds (pepsin) and for their chronicity
  • pepsin collagenase, hyaluronidase and elastase
  • the polyphosphate inhibits the action of at least one enzyme which contributes to the prevention or delay of wound healing. More preferably, the enzyme is one or more of pepsin, collagenase, elastase and hyaluronidase.
  • the polyphosphate may be a single chemical entity or it may be a mixture of polyphosphates with different numbers of phosphate units. Where it is a mixture, the average number of phosphate units is at least 3. Preferably, the polyphosphate has an average of from 4 to 40 phosphate units.
  • the polyphosphate has a P 2 O 5 content of at least 55% by weight, more preferably at least 60% by weight.
  • a preferred range is 60 to 75% by weight, more preferably 65 to 70% by weight.
  • the material known as sodium hexametaphosphate is a mixture of polyphosphates with an average of 12 phosphate units and a P 2 O 5 content of about 68%.
  • the polyphosphate is an alkali metal salt, more preferably a sodium or potassium salt, or a mixture thereof.
  • the present invention also provides a method of promoting chronic wound healing comprising the administration of a therapeutically effective amount of a polyphosphate having at least 3 phosphate units and/or as indicated above.
  • the amount of polyphosphate is from 300mg to 24,000mg as a daily dosage.
  • the polyphosphate is administered at a pH of from 2 to 6.
  • the present invention further provides a pharmaceutical composition
  • a pharmaceutical composition comprising a therapeutically effective amount of a polyphosphate having at least 3 phosphate units in admixture with a pharmaceutically acceptable adjuvant, diluent or carrier.
  • polyphosphates of use in the present invention are trimetaphosphate (P 3 ) and hexametaphosphate (ostensibly P 6 although in practice about P 12 ).
  • the polyphosphate may be, for instance, an alkali metal salt (as mentioned above), an alkaline earth metal salt, such as a calcium salt, or an ammonium salt. Preferably, it is a soluble salt.
  • the enzyme subject to inhibition by the polyphosphate may include an ECM active enzyme selected from the group consisting of a Matrix Metalloproteinase (MMP), a serine proteinase and a glycoside hydrolase.
  • MMP Matrix Metalloproteinase
  • the MMP may be, for instance, collagenase
  • the serine proteinase may be, for instance, elastase
  • the glycoside hydrolase may be, for instance, hyaluronidase.
  • the one or more enzymes may be active in the upper digestive tract. They include an aspartyl proteinase, for instance, pepsin, and an extracellular matrix (ECM) enzyme, for instance, selected from the group consisting of a Matrix Metalloproteinase (MMP), a serine proteinase and a glycoside hydrolase. Examples are collagenase, elastase and a hyaluronidase.
  • MMP Matrix Metalloproteinase
  • serine proteinase a glycoside hydrolase
  • glycoside hydrolase examples are collagenase, elastase and a hyaluronidase.
  • the polyphosphate may be used in the manufacture of a medicament for the inhibition of an ECM or digestive tract active enzyme in a mammal.
  • the therapeutically effective amount of the polyphosphate may be from 0.1 to 500 mM and preferred ranges include 0.1 to 200 mM and 0.1 to 100 mM.
  • the polyphosphate may be administered at a pH, for instance, in the range of from 4 to 10.
  • a preferred range includes 6 to 8 and a more preferred range is 6 to 7.
  • the method may be a method of reduction of scar formation and/or wound healing.
  • the method may be for the prevention, alleviation or treatment of gastric lesions caused by pepsin activity in a mammal.
  • the therapeutically effective amount of the polyphosphate may be, for instance, from 0.1 to 500 mM or from 0.1 to 10 mM.
  • the pH of administration may be in one of the ranges 2 to 8, 2 to 6 and 3 to 5.
  • the pharmaceutical composition may be in any suitable form including a dry powder, a gel or paste or as a liquid.
  • the polyphosphate may be present in an amount of, for instance, 0.1 to 12.0% weight/volume.
  • the composition may be in any suitable structure such as a spray, roll-on, patch, suspension, implant, sub-dermal depot, injection, lipstick / balm style applicator, suture / stitches or surgical glue.
  • the wound dressing for delivering a therapeutically effective amount of polyphosphate/ trimetaphosphate to the wound site will contain a wound contacting material.
  • the wound contacting material (incorporating the polyphosphate/ trimetaphosphate) may take a number of forms. These include, without limitation, foams, fibers, fabrics, films, alginates, hydrogels, and hydrocolloids.
  • Foam generally refers to a cellular polymeric structure, and preferably an open cell structure.
  • Suitable foams include such synthetic organic polymers as polyurethane, carboxylated butadiene styrene rubber, polyester, polyacrylate and non-synthetic/semi-synthetic polymers such as polysaccharides and there derivatives. It is generally desirable that the foam is hydrophilic; however, hydrophobic foams having a hydrophilic coating on them may be used.
  • Hydrophilic foams include cellular polyurethane foam formed from isocyanates, polyether/ polyester polyols and water, catalysts, stabilizers and other substances. Fabric may be formed from fibers such as synthetic fibers, natural fibers, or combinations thereof.
  • Synthetic fibers include, for example, polyester, acrylic, polyamide, polyolefin, polyaramid, polyurethane, regenerated cellulose, and blends thereof. More specifically, polyester includes, for example, polyethylene terephthalate, polytriphenylene terephthalate, polybutylene terephthalate, polylactic acid, and combinations thereof.
  • Polyamide includes, for example, nylon 6, nylon 6,6, and combinations thereof.
  • Polyolefin includes, for example, polypropylene, polyethylene, and combinations thereof.
  • Polyaramid includes, for example, poly-p-phenyleneteraphthalamid (i.e., Kevlar®), poly-m-phenyleneteraphthalamid (i.e., Nomex®), and combinations thereof.
  • Natural fibers include, for example, wool, cotton, flax, and blends thereof.
  • the fabric may be of any variety, including but not limited to, woven fabric, knitted fabric, nonwoven fabric, or combinations thereof.
  • the film may include thermoplastic materials, thermoset materials, or combinations thereof.
  • Thermoplastic or thermoset materials may include polyolefin, polyester, polyamide, polyurethane, acrylic, silicone, melamine compounds, polyvinyl acetate, polyvinyl alcohol, nitrile rubber, ionomers, polyvinyl chloride, polyvinylidene chloride, chloroisoprene, or combinations thereof.
  • the polyolefin may be polyethylene, polypropylene, ethylvinyl acetate, ethylmethyl acetate, or combinations thereof.
  • Polyethylene may include low density or high density polyethylene.
  • the film may have a thickness of between about 1 and about 500 microns, or more preferably between about 1 and about 250 microns, or even more preferable between about 1 and about 100 microns.
  • Alginate is a natural polysaccharide that exists widely in many brown seaweeds. Sodium alginates are well known for their ability to form a gel in contact with most multivalent cations. Alginate fibers may be formed from alginate by extruding or spinning an alginate aqueous solution into a coagulating bath containing a multivalent cation (such as calcium) to cross-link and gel the alginate solution. The alginate fibers are then typically processed and incorporated into a wound care dressing.
  • a multivalent cation such as calcium
  • Hydrogels generally consist of high-molecular molecules that form a coherent matrix for enclosing smaller molecules and aqueous solutions. Hydrogels can be described as a two- component system of water and a three-dimensional network polymer. Examples of hydrogels include starch, pectin, gelatin, other natural gums and insoluble cross-linked polymers such as polyethylene oxide. Hydrocolloids are hydrophilic polymers, of vegetable, animal, microbial or synthetic origin, that generally contain many hydroxyl groups and may be polyelectrolytes. They are naturally present or added to control the functional properties of a material such as viscosity, including thickening and gelling, and water binding.
  • hydrocolloids include carbowax, vinyl polymers (such as polyvinyl alcohol, polyvinyl pyrrolidone, and polyvinylacetate), cellulose derivatives (such as ethyl cellulose, methyl cellulose, and carboxymethyl cellulose), and natural gums (such as guar, acacia, and pectins).
  • Azocoll is a commercially available azo dye labelled collagen Type I substrate derived from bovine hide. In the presence of certain enzymes the red azo dye is liberated from the collagen and the resulting colour change can be measured and correlated with collagenolytic activity.
  • the Azocoll assay was used to determine the inhibitory effect of polyphosphates on the action of pepsin, collagenase, snake venom metalloprotease, human gastric juice and human chronic wound fluid against azo-labelled collagen substrate.
  • Human chronic Human chronic wound fluid was extracted from primary wound wound fluid dressing by soaking a single dressing overnight in 5ml phosphate buffered saline. pH 4.0 - 6.0 5OmM sodium acetate adjusted to relevant pH with glacial acetic buffer acid pH 7.0 - 8.0 0.2 M Tris(hydroxymethyl)aminomethane (Tris) corrected to buffer relevant pH using 0.2M hydrochloric acid
  • Azocoll solution 0.30% w/v solution of Azocoll substrate (azo-dye labelled Type I collagen (Calbiochem, UK)) prepared in buffer
  • Table 1 Reagents and buffers used in the Azocoll assay. (All reagents were purchased from standard laboratory suppliers, unless otherwise indicated)
  • test solutions containing between 0-122mg/ml of the proposed inhibitor were prepared. 100 ⁇ l of this test solution was then thoroughly mixed with 100 ⁇ l of the relevant enzyme solution on a vortex mixer before lOOO ⁇ l of buffered Azocoll solution was added and mixed. The inhibitor:enzyme:Azocoll sample was then incubated in a heated water bath for 3 hours at 37°C and inverted every 30 minutes during this incubation time. Samples were then removed from the incubator, placed in iced water to cool and centrifuged (Fisher Scientific, accuSpin Model 400 Benchtop Centrifuge) at 4000rpm for 5 minutes.
  • the absorbance of the supernatant was measured at 540 nm (Labsystems Multiskan Ascent 354, ThermoFisher Scientific, Horsham, Westshire, UK) using deionised water as a blank.
  • TCA Tricholoroacetic Acid
  • the TCA assay is based on the method described by M.L. Anson (1938). J General Physiol, 22, 79-89.
  • the substrate bovine haemoglobin
  • the substrate bovine haemoglobin
  • Any remaining undigested haemoglobin is then precipitated with TCA to yield a supernatant which contains only products of digested haemoglobin.
  • the concentration of haemoglobin breakdown products in the supernatant is measured spectrophotometrically and provides an indication of proteinase activity.
  • the TCA precipitation assay was used to determine the inhibitory effect of polyphosphates and trimetaphosphate on the action of pepsin against haemoglobin.
  • Pepsin solution 20 ⁇ g/ml of pepsin (from porcine gastric mucosa lyophilized powder, 3,200-4,500 units/mg protein :Sigma-Aldrich Ltd, UK) prepared in a buffered solution (pH 2-4 as desired) pH 2.0 buffer 0.2 M glycine and 0.1 M sodium chloride solution
  • test solutions containing between 0-306 mg/ml of the proposed inhibitor were prepared. 100 ⁇ l of this test solution was then thoroughly mixed with 100 ⁇ l of pepsin solution on a vortex mixer before 1500 ⁇ l of buffered bovine haemoglobin solution was added and mixed. The inhibitor:enzyme:haemoglobin sample was then incubated in a heated water bath for 30 minutes at 37 0 C. The samples was then removed from the incubator, mixed with 2.0ml TCA solution and left to stand for 30 minutes in iced water. The sample was then centrifuged (Fisher Scientific, accuSpin Model 400 Benchtop Centrifuge) at 4000rpm for 5 minutes.
  • the absorbance of the supernatant was measured at 280 nm (Labsystems Multiskan Ascent 354, ThermoFisher Scientific, Horsham, West Wales, UK) using deionised water as a blank.
  • the percentage inhibition of pepsin activity was calculated by comparing the absorbance intensity of test samples containing inhibitor with samples containing 0 ⁇ g/ml of inhibitor according to the equation below:
  • Elastin Congo red is a commercially available elastin substrate impregnated with the chromophore Congo red. In the presence of elastase the Congo red dye is liberated from the elastin and the resulting colour change can be measured and correlated with elastolytic activity.
  • the elastin Congo red assay was used to determine the inhibitory effect of polyphosphates and trimetaphosphate on the elastase against the elastin Congo red substrate.
  • test solutions containing between 0-306 mg/ml of the proposed inhibitor were prepared. 100 ⁇ l of this test solution was then thoroughly mixed with 100 ⁇ l of elastase solution on a vortex mixer. 1 OOO ⁇ l of buffered Elastin Congo red solution was then added and mixed. The inhibitor:enzyme:Elastin Congo red sample was then incubated overnight in a heated water bath at 37°C. Samples were then removed from the water bath and placed in iced water to cool for 30 minutes before being centrifuged (Fisher Scientific, accuSpin Model 400 Benchtop Centrifuge) at 13000rpm for 5 minutes.
  • the absorbance of the supernatant was measured at 540 nm (Labsystems Multiskan Ascent 354, ThermoFisher Scientific, Horsham, West Wales, UK) using deionised water as a blank.
  • the percentage inhibition of elastase activity was calculated by comparing the absorbance intensity of test samples containing inhibitor with samples containing 0 ⁇ g/ml of inhibitor according to the equation below:
  • the hyaluronidase activity assay is based on the methods of Bonner and Cantey (Clin. Chim. Acta, 13 (1966) 746-752) and Reissig et al. J. Biol. Chem., 217 (1955) 959-966. It relies on the fact that sodium hyaluronate is degraded in the presence of hyaluronidase into saccharides with N-acetylglucosamine (NAG) end-groups. The NAG can then be quantified by heating with alkaline tetraborate to form an intermediate which reacts with p-dimethylamino benzaldehyde in acidic medium to form a coloured product.
  • NAG N-acetylglucosamine
  • the colour change can be measured and correlated with the activity of hyaluronidase.
  • the hyaluronidase assay was used to determine the inhibitory effect of polyphosphates on the activity of hyaluronidase against the sodium hyaluronan substrate.
  • test solutions containing between 0-61.2 mg/ml of the proposed inhibitor were prepared. 100 ⁇ l of this test solution was then thoroughly mixed with 100 ⁇ l of 1 mg/ml hyaluronidase using a vortex mixer before 200 ⁇ l of 4 mg/ml buffered, sodium hyaluronate solution was added. The polymer:hyaluronidase:HA test sample was then thoroughly mixed using a vortex mixer and incubated at 37 0 C for 4 hours. The reaction was subsequently terminated by heating at 80°C for 5 min. After incubation, 60 ⁇ l of potassium tetraborate (0.8M) was added and the samples were again incubated at 80 °C for 5 minutes followed by cooling on ice for 5 minutes.
  • potassium tetraborate 0.8M
  • the lysozyme dose response assay is based on the observation that in the presence of lysozyme the optical density of a cell suspension of Micrococcus lysodeikticus decreases. The rate of this decrease in optical density can be measured and correlated with the activity of lysozyme.
  • the lysozyme assay was used to determine the inhibitory effect of sodium polyphosphate (68% P 2 O 5 ) on the action of lysosyme against the Micrococcus lysodeikticus cell suspension substrate.
  • the inhibition of lysozyme activity was calculated by comparing the maximum linear gradient of the fall in optical density over the 5 minute period for test samples containing inhibitor with samples containing 0 ⁇ g/ml of inhibitor.
  • the percentage inhibition was calculated according to the equation below:
  • Chymotrypsin dose response assay The chymotrypsin dose response assay is based on the observation that in the presence of chymotrpysin the substrate Na-benzoyl-L-tyrosine ethyl ester (BTEE) is degraded into Na- benzoyl-L-tyrosine + Ethanol. This conversion can be measured spectrophotometrically by an increase in absorbance at 253nm. The rate of change in absorbance can then be measured and correlated with the activity of chymotrypsin. The chymotrypsin assay was used to determine the inhibitory effect of sodium polyphosphate (68% P 2 O 5 ) on the action of chymotrypsin against the BTEE substrate. Materials:
  • test solution containing between 0-61.2 mg/ml of the proposed inhibitor was added to a quartz cuvette and placed in a thermostatically controlled UV spectrophotometer maintained at 25°C.
  • 1.26ml of BTEE solution and 0.07ml of calcium chloride solution were also added to the cuvette, mixed by inversion and allowed to equilibrate until the absorbance at 253nm was constant.
  • 0.09ml of chymotrypsin solution was then added to the cuvette and immediately mixed by inversion.
  • the absorbance of the inhibitor: substrate xhymotrypsin test sample was measured at 253 nm at 3 second intervals for 5 minutes (Unicam UV 500, Thermo Spectronic, Cambridge, UK). Buffer was used as a blank.
  • the inhibition of chymotrypsin activity was calculated by comparing the maximum linear gradient of the increase in absorbance at 253nm over the 5 minute period for test samples containing inhibitor with samples containing 0 ⁇ g/ml of inhibitor.
  • the percentage inhibition was calculated according to the equation below:
  • Figure 1 shows that sodium polyphosphate (68% P 2 O 5 content) inhibited the proteolytic activity of pepsin in a concentration dependent manner. The inhibition occurred across a wide range of polyphosphate concentrations. Inhibition was also pH dependent and found to be greatest at pH 4. At pH 4, levels of inhibition in excess of 90% were achieved with polyphosphate concentrations greater than 4.59mg/ml.
  • Figure 2 illustrates that the potency of inhibition varied with the polymeric chain length of sodium polyphosphates (expressed as P 2 O 5 content). Sodium polyphosphates with a greater P 2 O 5 content were more effective inhibitors of pepsin.
  • Figure 3 demonstrates that the concentration dependent inhibition of pepsin using a polyphosphate was unaffected by the choice of alkali metal counterion. Potassium polyphosphate inhibited pepsin in a comparable manner to that observed with sodium polyphosphate.
  • Figure 4 shows that sodium trimetaphosphate could also inhibit pepsin across a wide concentration range; however, the potency and extent of inhibition at maximal concentrations was not as large as that observed with polyphosphates.
  • Figure 5 shows that sodium polyphosphate (68% P 2 O 5 content) inhibited the proteolytic activity of collagenase in a concentration dependent manner. The inhibition occurred across a wide range of polyphosphate concentrations. Inhibition was also pH dependent and found to be greatest at pH 7. At pH 7, levels of inhibition in excess of 70% were achieved at higher polyphosphate concentrations.
  • Figure 6 illustrates that the potency of inhibition varied with the polymeric chain length of sodium polyphosphates (expressed as P 2 O 5 content). Sodium polyphosphates with a greater P 2 O 5 content were more effective inhibitors of collagenase.
  • Figure 7 demonstrates that the concentration dependent inhibition of collagenase using a polyphosphate was relatively unaffected by the choice of alkali metal counterion. Potassium polyphosphate inhibited collagenase in a comparable manner to that observed with sodium polyphosphate.
  • Figure 8 shows that sodium polyphosphate (68% P 2 O 5 content) inhibited the digestive activity of hyaluronidase in a concentration dependent manner. The inhibition occurred across a wide range of polyphosphate concentrations. Inhibition was also pH dependent and found to be greatest at pH 4.5. At pH 4.5, levels of inhibition in excess of 90% were achieved at polyphosphate concentrations greater than 0.612mg/ml.
  • Figure 9 illustrates that the potency of inhibition varied with the polymeric chain length of sodium polyphosphates (expressed as P 2 O 5 content). Sodium polyphosphates with a greater P 2 O 5 content were more effective inhibitors of hyaluronidase.
  • Figure 10 demonstrates that the concentration dependent inhibition of hyaluronidase using a polyphosphate was unaffected by the choice of alkali metal counterion. Potassium polyphosphate inhibited hyaluronidase in a comparable manner to that observed with sodium polyphosphate.
  • Figure 12 illustrates that the potency of inhibition varied with the polymeric chain length of sodium polyphosphates (expressed as P 2 O 5 content). Although sodium polyphosphates with a P 2 O 5 content between 60-68% gave similar levels of inhibition, sodium polyphosphate containing 70% P 2 O 5 was able to inhibit 100% of elastase activity at higher concentrations.
  • Figure 13 demonstrates that the concentration dependent inhibition of elastase using a polyphosphate was not adversely affected by the choice of alkali metal counterion. Potassium polyphosphate inhibited elastase in a slightly superior manner to that observed with sodium polyphosphate.
  • Figure 14 shows that sodium trimetaphosphate could also inhibit elastase across a wide concentration range; however, the extent of inhibition at maximal concentrations was not as large as that observed with polyphosphates.
  • Figure 15 shows that polyphosphate inhibited in a concentration dependent manner the proteolytic activity of human gastric juice. At polyphosphate concentrations greater than 6.12mg/ml nearly 100% of the proteolytic activity of human gastric juice was inhibited.
  • Human gastric juice contains a mixture of aspartic proteases including Pepsin 1, 3a, 3b, 3c and gastricsin. The inhibition of activity for gastric juice demonstrates that polyphosphates can inhibit other aspartic proteases in addition to pepsin.
  • Figure 16 illustrates that polyphosphate can inhibit in a concentration dependent manner snake venom metalloproteinase. This demonstrates that, in addition to collagenase, polyphosphate can inhibit other matrix metalloproteinases.
  • Figure 17 shows that polyphosphate can inhibit in a concentration dependent manner the digestive activity of lysozyme. This demonstrates that, in addition to hyaluronidase, polyphosphate can inhibit other enzymes from the glycoside hydrolase class.
  • Figure 18 shows that polyphosphate can inhibit in a concentration dependent manner the digestive activity of ⁇ -chymotrypsin. This demonstrates that, in addition to elastase, polyphosphate can inhibit other enzymes from the serine protease class.
  • Figure 19 shows that polyphosphate can inhibit in a concentration dependent manner the proteolytic activity of fluid extracted from human chronic wounds.

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  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)
PCT/GB2009/000504 2008-02-22 2009-02-23 Chronic wound treatment Ceased WO2009104005A1 (en)

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US12/918,826 US20110117208A1 (en) 2008-02-22 2009-02-23 Chronic wound treatment
EP09712875A EP2254585A1 (en) 2008-02-22 2009-02-23 Chronic wound treatment
JP2010547251A JP2011512394A (ja) 2008-02-22 2009-02-23 慢性創傷の治療

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GB0803284A GB0803284D0 (en) 2008-02-22 2008-02-22 Enzyme inhibition
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WO2011125619A1 (ja) * 2010-04-08 2011-10-13 国立大学法人旭川医科大学 腸管保護剤
CN103687582A (zh) * 2011-07-19 2014-03-26 露珍细胞再生株式会社 含有从酵母菌中提取出的多聚磷酸、多聚磷酸的盐或多聚磷酸的溶剂化物的多聚磷酸组合物及其制作方法
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JP5901021B2 (ja) 2010-01-20 2016-04-06 ケーシーアイ ライセンシング インク 流体潅流および/または陰圧閉鎖創傷療法のための、親水性フォーム状創傷挿入材を用いた漏出防止包帯システムおよび方法
DE102013222223A1 (de) * 2013-10-31 2015-04-30 Bk Giulini Gmbh Blutstillendes Mittel enthaltend kristallines Polyphosphat
GB2561262B (en) * 2017-07-13 2019-03-20 Dentmed Ltd A targeted drug delivery pad

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WO2011125619A1 (ja) * 2010-04-08 2011-10-13 国立大学法人旭川医科大学 腸管保護剤
EP2559437A4 (en) * 2010-04-08 2013-08-21 Nat University Corp Asahikawa Medical University Intestinal protectant
JP5660508B2 (ja) * 2010-04-08 2015-01-28 国立大学法人旭川医科大学 腸管保護剤
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US11752180B2 (en) 2010-04-08 2023-09-12 National University Corporation Asahikawa Medical University Intestinal protectant
CN103687582A (zh) * 2011-07-19 2014-03-26 露珍细胞再生株式会社 含有从酵母菌中提取出的多聚磷酸、多聚磷酸的盐或多聚磷酸的溶剂化物的多聚磷酸组合物及其制作方法
CN103687582B (zh) * 2011-07-19 2016-03-30 露珍细胞再生株式会社 含有从酵母菌中提取出的多聚磷酸、多聚磷酸的盐或多聚磷酸的溶剂化物的多聚磷酸组合物及其制作方法
WO2020039070A1 (en) * 2018-08-23 2020-02-27 Fibrothelium Gmbh Preparation of fibroin and therapeutic products made thereof
US12447240B2 (en) 2018-08-23 2025-10-21 Fibrothelium Gmbh Preparation of fibroin and therapeutic products made thereof
US12214103B2 (en) 2018-12-20 2025-02-04 Bk Giulini Gmbh Products for treating bleeding wounds

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