US20060057552A1 - Method of conserving biological prostheses, conserved biological prostheses and conserving solution - Google Patents

Method of conserving biological prostheses, conserved biological prostheses and conserving solution Download PDF

Info

Publication number
US20060057552A1
US20060057552A1 US11/250,360 US25036005A US2006057552A1 US 20060057552 A1 US20060057552 A1 US 20060057552A1 US 25036005 A US25036005 A US 25036005A US 2006057552 A1 US2006057552 A1 US 2006057552A1
Authority
US
United States
Prior art keywords
heparin
solution
epoxide
biological
conserving
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Abandoned
Application number
US11/250,360
Inventor
Leonid Barbarash
Irina Jouravleva
Svetlana Novikova
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Individual
Original Assignee
Individual
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Individual filed Critical Individual
Priority to US11/250,360 priority Critical patent/US20060057552A1/en
Assigned to FREY, RAINER reassignment FREY, RAINER ASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS). Assignors: BARBARASH, LEONID, JOURAVLEVA, IRINA, NOVIKOVA, SVETLANA
Publication of US20060057552A1 publication Critical patent/US20060057552A1/en
Abandoned legal-status Critical Current

Links

Images

Classifications

    • 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
    • A61L2/00Methods or apparatus for disinfecting or sterilising materials or objects other than foodstuffs or contact lenses; Accessories therefor
    • A61L2/16Methods or apparatus for disinfecting or sterilising materials or objects other than foodstuffs or contact lenses; Accessories therefor using chemical substances
    • A61L2/18Liquid substances or solutions comprising solids or dissolved gases
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61FFILTERS IMPLANTABLE INTO BLOOD VESSELS; PROSTHESES; DEVICES PROVIDING PATENCY TO, OR PREVENTING COLLAPSING OF, TUBULAR STRUCTURES OF THE BODY, e.g. STENTS; ORTHOPAEDIC, NURSING OR CONTRACEPTIVE DEVICES; FOMENTATION; TREATMENT OR PROTECTION OF EYES OR EARS; BANDAGES, DRESSINGS OR ABSORBENT PADS; FIRST-AID KITS
    • A61F2/00Filters implantable into blood vessels; Prostheses, i.e. artificial substitutes or replacements for parts of the body; Appliances for connecting them with the body; Devices providing patency to, or preventing collapsing of, tubular structures of the body, e.g. stents
    • A61F2/02Prostheses implantable into the body
    • A61F2/24Heart valves ; Vascular valves, e.g. venous valves; Heart implants, e.g. passive devices for improving the function of the native valve or the heart muscle; Transmyocardial revascularisation [TMR] devices; Valves implantable in the body
    • A61F2/2412Heart valves ; Vascular valves, e.g. venous valves; Heart implants, e.g. passive devices for improving the function of the native valve or the heart muscle; Transmyocardial revascularisation [TMR] devices; Valves implantable in the body with soft flexible valve members, e.g. tissue valves shaped like natural valves
    • A61F2/2415Manufacturing methods

Definitions

  • the invention concerns a method of conserving biological prostheses and biological prostheses produced in accordance with that method.
  • the invention further concerns a conserving solution for conserving biological prostheses.
  • Biological prostheses can be produced from body components of human beings and animals.
  • heart valves, arteries etc of cattle or pigs are used as implants in human beings.
  • glutaraldehyde has represented the main conserving agent for cardiac-circulatory bioprostheses (biological prostheses).
  • Glutaraldehyde reacts with the amino groups of lysine and hydroxylysine. As a result of those reactions, chemical bonds are formed, which are represented in particular by Schiff's bases or pyridine bases.
  • Glutaraldehyde ensures reliable sterility and the suppression of antigenic properties of the biological material.
  • Glutaraldehyde however makes the tissue stiff and hydrophobic and the surface assumes a rough disordered relief.
  • the chemical compounds of glutaraldehyde and collagen have in their structure ligands for complex formation with calcium cations. Those complexes do in fact subsequently become centers of hydroxyapatite crystallisation. In overall terms the result of this is that the glutaraldehyde has a negative influence on the thrombosis-resistant properties of the tissue and gives rise to calcification of the biological materials.
  • a greater effect can be achieved by replacing the main conserving agent by a cross-linking agent, the structural formula of which does not contain any aldehyde group.
  • Epoxide compounds are effective cross-linking agents, guarantee strength and elasticity of the biological material, inhibit calcification of the biological prostheses and have pronounced antigen-depressive properties.
  • U.S. Pat. No. 5,165,919 discloses a method of covalent fixing of heparin on medical implants by the interaction of amino and epoxy groups. That method however was developed for polymer materials and cannot be used for biological prostheses.
  • the object of the invention is to provide a method of conserving biological prostheses which are resistant to calcification and thrombosis formation and have an enhanced level of strength and elasticity. Another object of the invention is to provide improved conserved biological prostheses.
  • the object of the invention is further attained by a biological prosthesis as set forth in claim 20 .
  • a preferred embodiment of the biological prosthesis is recited in appendant claim 21 .
  • the object is further attained by the provision of a conserving agent for biological prostheses as set forth in claim 22 .
  • Preferred developments are recited in appendant claims 23 to 27 .
  • mixtures of polymer and non-polymer epoxide compounds are used for conserving biological prostheses, wherein 2 and more epoxide groups are present in the structural formula of the epoxide compounds.
  • a solution with a mixture of at least three different epoxide compounds (components) is used.
  • the antithrombotic is selected from the group which consists of heparin, low-molecular heparin, heparinoids, hirudin and mixtures thereof.
  • the antithrombotic has antithrombotic or anti-coagulating properties. In that respect it is possible in accordance with the invention to use all substances which have a heparin-like action.
  • heparin is used in accordance with the invention.
  • the biological prostheses produced in that way can be stored in a solution of any compound which guarantees sterility.
  • epoxide compounds are used in order to avoid possible additional chemical reactions.
  • the subject-matter of the present invention is thus on the one hand a method of conserving biological material which can be used in particular for producing heart and blood vessel valve prostheses.
  • the subject-matter of the invention is the provision of the biological prostheses which are conserved in accordance with the method of the invention.
  • mixtures of polymer and non-polymer epoxide compounds with a differing number of epoxide groups (2 and more) are used.
  • the composition of the mixture can be varied in dependence on the nature of the biological material and the aims of a subsequent chemical modification.
  • the epoxide group in the epoxide compounds used is a constituent of a glycidol residue.
  • a mixture of polymer and non-polymer epoxide compounds is used for conserving heart-circulatory bioprostheses (bioprosthesis—biological prosthesis).
  • a polymer epoxide compound is used to identify an epoxide compound which is composed of at least two repetitive, directly interconnected units to which epoxy group-bearing residues such as for example glycidol or 2,3-epoxypropan-1-ol are joined.
  • the polymer epoxide compounds have a degree of polymerisation of at least two, more preferably between three and 25, still more preferably between three and 15, in particular between four and nine.
  • the degree of polymerisation relates to the polymer proportion of the epoxide compound, bearing the epoxy groups.
  • an epoxide compound with between two and three epoxide groups wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms, for example a tetramethylene group.
  • Preferably arranged between the at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least six, preferably six, carbon atoms, such as for example a hexamethylene group.
  • non-polar epoxide compound is used to identify an epoxide compound which does not have any repetitive, directly interconnected units to which epoxy group-bearing residues such as for example glycidol or 2,3-epoxypropan-1-ol are joined.
  • composition of the mixture in dependence on the association in respect of nature and tissue of the biological material. That is related to the spatial configuration and the composition of the collagens of the various tissues and the different accessibility of the reactive amino acid groups of the collagen for the conserving agents which have different structural formulae.
  • composition of the mixture depends on the purpose of the additional chemical modification; saturation of the biological material with a predetermined number of epoxide groups which are required for covalent immobilisation of biologically active substances is possible. Thus for example upon immobilisation of heparin a large number of epoxide groups is required.
  • the mixture is preferably adjusted as follows:
  • the number of reactive groups must be low as supersaturation of the tissue of the biological prosthesis with high-molecular polymers results in an impairment of the properties in respect of elasticity and deformation. Accordingly use of the epoxide mixtures of differing composition permits the amount of substance which is immobilised on the biological material to be controlled or influenced.
  • the mixture is preferably adjusted as follows:
  • a non-polymer preferably low-molecular compound, with two reaction groups, must be present in the mixture.
  • alkane diol diglycidylether such as for example butane-1,4-diol diglycidylether
  • polyalcohol diglycidylether such as for example glycerine diglycidylether
  • alkylene glycol diglycidylether such as ethylene glycol diglycidylether or mixtures thereof.
  • ethylene glycol diglycidylether is used.
  • the concentration of non-polymer epoxide compound with two epoxide groups (di-epoxide compound) in the mixture is preferably 1-95% by weight, more preferably 20-90% by weight. Very good results were obtained with a concentration of 40-80% by weight.
  • the second component in the mixture is a polymer epoxide compound which contains between two and three epoxide groups in the structural formula and/or an epoxide compound with between two and three epoxide groups, wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms.
  • polyalkylene glycol diglycidylethers such as for example polyethylene glycol diglycidylether, polytetramethylene glycol diglycidylether, polypropylene glycol diglycidylether or mixtures thereof.
  • alkane diol diglycidylethers such as for example hexane-1,6-diol diglycidylether and/or higher dicarboxylic acid diglycidylesters.
  • higher dicarboxylic acid diglycidylester is used to identify glycidol esterified with higher dicarboxylic acids (2,3-epoxypropan-1-ol), that is to say diglycidylesters of higher dicarboxylic acids.
  • Identified as higher dicarboxylic acids are those which have more than 12 carbon atoms.
  • higher dicarboxylic acid diglycidylesters which can be used are Denacol EX-1111 (mixture of two acids with a molecular weight of 398 g/mol and 454 g/mol) or Denacol EX-1112 (mixture of two acids with the same molecular weight of 450 g/mol but of differing structure) from Nagase Company Ltd, Japan.
  • polyethylene glycol diglycidylether is used.
  • the polyethylene glycol diglycidylether has a degree of polymerisation of 3-12, more preferably 4-9.
  • That component supplements cross-linking of the collagen by inter-fibrillar bonds.
  • the concentration in the mixture is preferably 1-95%, more preferably 2-40% by weight, still more preferably 5-20% by weight.
  • the third component is an epoxide compound with a number of epoxide groups of at least three, for example four, five or more.
  • polyalcohol polyglycidylethers are used such as for example sorbitol polyglycidylether, glycerine polyglycidylether and the like, polysaccharide polyglycidylether or mixtures thereof.
  • polysaccharide polyglycidylether or mixtures thereof.
  • pentaerythrol polyglycidylether is used.
  • That third component saturates the tissue with an optimum number of free epoxide groups, to which heparin can be immobilised without the use of additional reagents.
  • the concentration of the component in the mixture is preferably 1-95% by weight, more preferably 10-50% by weight. Very good results were obtained with a concentration of 15-35% by weight.
  • the method according to the invention permits an increase in the density of cross-linking of the collagen, which has an advantageous effect on the strength properties of the biological prosthesis.
  • the use of mixtures of polymer and non-polymer epoxides imparts to the biological material a higher level of resistance to calcification.
  • the epoxy group represents one of the most reactive groups in the polymers, including also in biological materials. Binding of the heparin by way of the amino group does not have a disadvantageous effect on the anti-coagulant properties thereof.
  • Reaction with the epoxy group makes it possible to implement immobilisation of heparin under ‘gentle’ conditions which exclude unwanted physical-chemical changes in the biological material. Reaction of heparin with the epoxy groups can take place in a wide pH-range of the medium (pH 2-11).
  • a pH-value of 5-8 is used, for example employing phosphate buffers, phosphate-citrate buffers and/or acetylsalicylic acid.
  • a third component that is to say a compound with a number of epoxy groups of at least 3, into the epoxide conserving agent makes it possible to increase the amount of immobilised heparin.
  • the covalently bound, that is to say immobilised heparin does not pass into the bloodstream but has an antithrombotic effect due to binding and sorption to the protein layers and smoothing of the surface of the biological prosthesis.
  • acetylsalicylic acid for setting an acid pH-value in the immobilisation of heparin surprisingly further increases the thrombosis resistance of the surface.
  • aorta complexes of a pig or pericardia of cattle it is possible to use for example aorta complexes of a pig or pericardia of cattle.
  • arteriosclerosis for example damaged arteries can be replaced by the internal thoracic artery or the head artery of cattle.
  • Allogenous or heterologous mitral valves or tricuspidal valves can be used for the orthotopic replacement of heart valves.
  • pericardia from cattle, the allogenous hard meninges or body-specific pericardia.
  • Valves, membrane-like tissues and vessels, for example arteries, veins, artery segments, vein segments and so forth can be taken from any biological genuses of mammals, for example cattle, pigs, sheep, human beings and so forth, insofar as they are suitable in respect of their anatomical features for replacement of one element or another of the heart-circulation system.
  • the conserving solution was replaced by an identical but freshly produced solution.
  • the valve vela were rinsed with sterile 0.9% by weight NaCl solution and incubated in a heparin solution (100 IU/ml, IU: International Unit) pH 5.0, in which case the pH-value was adjusted by the addition of aqueous acetylsalicylic acid solution, for a period of 3 hours at a temperature of 20° C.
  • the ratio of heparin:acetylsalicylic acid in the heparin solution, in relation to weight, is about 1.3-16:1.
  • the precise ratio of heparin:acetylsalicylic acid depends on the respective activity (in IU/weight) of the heparin used.
  • a heparin solution which is suitable for the invention can be produced by the addition of about 7-10 mg/ml of acetylsalicylic acid to a heparin solution with about 75-100 IU/ml.
  • acetylsalicylic acid is added to the heparin solution until the pH-value of the solution is between about 5 and 6.
  • the concentration of the heparin solution is at least 75 IU/ml, preferably 100 IU/ml. It will be appreciated that it is also possible to use solutions with higher heparin concentrations.
  • the comparative samples were incubated for 28 days in 0.6250% by weight glutaraldehyde (GA), and 50 mM phosphate buffer pH 7.4 at ambient temperature (between 20° C. and 25° C.).
  • the GA-solution was changed four times, that is to say after the 1st, 3rd, 7th and 21st days.
  • the conserving solution was removed.
  • the comparative sample was washed at ambient temperature for one hour without agitation in 0.9% common salt solution.
  • the common salt solution was changed in that procedure after every 20 minutes (a total of three washing steps).
  • the comparative sample was incubated for 21 days in 5% by weight ethylene glycol diglycidylether (DEE) and 50 mM phosphate buffer pH 7.4 at ambient temperature (20° C.-25° C.).
  • the DEE solution was changed after three days without a washing step.
  • the conserving solution was then removed.
  • the comparative sample was then washed at ambient temperature for one hour without agitation in 0.9% common salt solution.
  • the common salt solution was changed after every 20 minutes (a total of three washing steps).
  • the heparin treatment was effected with 100 IU/ml at 37° C. for 8-16 hours.
  • the unbound heparin was removed by washing with 0.9% by weight common salt solution for one hour at ambient temperature (20-25° C.).
  • the density of transverse cross-linking was assessed in accordance with the reduction in the number of free amino acid residues in the biological material, in which respect they were determined by an amino acid analysis method.
  • dumbbell shape dumbbell test bodies
  • That blade is of a standard shape and size and has sharpened edges.
  • samples of a standardised size are cut out of the biological material. Ten samples were investigated in each case.
  • the average thickness h of the samples (mm) was determined using a micrometer eyepiece.
  • the width of the sample was set to 0.25 cm using the above-mentioned blade.
  • the samples were of an initial length of 11 mm.
  • the amount of immobilised heparin was determined by means of elementary analysis in accordance with the difference in the content of sulfur in unmodified (control sample) and modified sample portions (modified sample).
  • the method is based on determining the difference in the level of sulfur concentration in test samples (modified sample) and control samples.
  • the sulfur content in heparin is high and low in collagen.
  • ⁇ [S] heparin [S] mod. sample ⁇ [S] control sample, wherein [S] is the sulfur concentration in [ ⁇ g/g] dry weight.
  • Y ⁇ [S]/S 1 , wherein Y is the heparin content in the biological material (biological prosthesis) in [mg/g], S 1 is the sulfur content in [ ⁇ g] in 1 mg of heparin.
  • any quantitative determination method can be used for determining the concentration of the sulfur content.
  • the sample material (at least 20 g) is firstly cut up with a pair of shears until a thin pulpy consistency is attained. Each sample has 10 ml of distilled water poured thereover. The sample is frozen at ⁇ 55° C. and lyophilised with a stepwise increase in temperature to +60° C. until dry. The dried sample material obtained in that way is finely ground in an agate mortar until a fine powder is produced.
  • the amount of immobilised heparin can also be determined in another fashion. For example, it is possible to implement quantification of immobilised heparin using toluidine blue which binds to immobilised heparin.
  • Example 1 shows the relative content of free amino acid residues (related to 1000 amino acid residues) in pig aortic valve vela
  • Example of the Amino acid Native tissue GA DEE + heparin invention THR 27.3 ⁇ 0.2 27.6 ⁇ 0.6 24.5 ⁇ 0.3 23.3 ⁇ 0.5 SER 45.3 ⁇ 0.4 46.7 ⁇ 1.1 41.6 ⁇ 0.4 39.6 ⁇ 0.4
  • GLY 238.2 ⁇ 1.2 252.1 ⁇ 4.1 261.1 ⁇ 2.4 272.7 ⁇ 3.2 ALA 124.3 ⁇ 0.9 127.7 ⁇ 0.8 122.3 ⁇
  • the density of transverse cross-linking is greater than when using the individual substance—ethylene glycol diglycidylether. That can be seen in particular from a reduction in the relative content of the amino acids methionine, tyrosine, lysine and hydroxylysine.
  • Table 2 shows the physical-mechanical parameters of pig aortic valve vela conserved with various methods.
  • Table 3 shows the amount of calcium (mg/g of dry tissue) in valve vela portions implanted under the skin of rats at various periods after implantation.
  • the sample produced in accordance with the example of the invention has an extremely low degree of calcification.
  • Table 4 shows the amount of immobilised heparin. DEE + heparin Example according to the invention 530 ⁇ 20 ⁇ g/g dry tissue 2340 ⁇ 120 ⁇ g/g dry tissue
  • the sample produced in accordance with the example of the invention has a very high content of immobilised heparin.
  • the conserving solution was replaced by an identical but freshly produced solution.
  • the segments were rinsed with sterile 0.9% by weight NaCl solution and incubated in a heparin solution (100 IU/ml) pH 5.0, wherein the pH-value was adjusted by the addition of aqueous acetylsalicylic acid solution (production, see Example 1 according to the invention), for a period of 4 hours at a temperature of 20° C. Production of the heparin solution was effected as described in Example 1.
  • the comparative samples used Were segments of the internal thoracic artery of a pig, which were treated with 0.625% by weight glutaraldehyde in 50 mM phosphate buffer pH 7.4 (GA) and with 5% by weight ethylene glycol diglycidylether and 100 IU/ml heparin in 50 mM phosphate buffer pH-value 7.4 (DEE+heparin) (see RU 2 008 767).
  • Production of the comparative samples was effected in accordance with the description set forth in relation to comparative Examples 1.
  • Example 1 The operation of determining the density of transverse cross-linking, the degree of calcification and the amount of immobilised heparin was effected as described hereinbefore in relation to Example 1.
  • the results contained in Example 1 and comparative Examples 1 are confirmed by the results obtained in the present case.
  • the resistance to thrombosis formation was assessed after the implantation of vessel segments which were conserved in accordance with the method according to the invention (example according to the invention) or for comparison purposes using glutaraldehyde (GA) or ethylene glycol diglycidylether and heparin (DEE+heparin), into the carotid artery of dogs.
  • G glutaraldehyde
  • DEE+heparin ethylene glycol diglycidylether and heparin
  • the vessel segments were between about 3 mm and 3.5 mm in diameter and between about 5 and 7 cm in length and were implanted in the neck artery (carotid) of 24 non-thoroughbred dogs which weighed between 10 and 15 kg.
  • the dogs were previously anesthetized by the intravenous administration of sodium thiopental and mechanically ventilated.
  • a carotid artery segment of between 5 and 7 cm in length was removed from the dogs and the bioprosthesis was implanted in place thereof using 6-0 polypropylene suture material.
  • Actuarial analysis is a standardised statistical procedure which is based on the probability of analysed complications, in the present case thrombosis, in which respect events which have already occurred are taken into consideration. Evaluation of the results was effected with the program STATISTICA for Windows (StatSoft, Inc, 1995).
  • Table 6 shows the relative content of free methionine, tyrosine, lysine and hydroxylysine residues (related to 1000 amino acid residues) in samples of the internal thoracic artery of a pig.
  • Native Ex. of the Amino acid tissue GA DEE + heparin inv. MET 7.5 ⁇ 0.5 7.3 ⁇ 0.4 6.3 ⁇ 0.2 — TYR 10.0 ⁇ 0.6 11.0 ⁇ 0.4 — 3.4 ⁇ 0.5 OHLYS 7.0 ⁇ 0.5 1.0 0.2 0.9 ⁇ 0.2 — LYS 24.1 ⁇ 1.9 3.5 ⁇ 0.5 — —
  • Table 7 shows the amount of immobilised heparin.
  • DEE + heparin Example according to the invention 190 ⁇ 10 ⁇ g/g dry tissue 1005 ⁇ 90 ⁇ g/g dry tissue
  • Table 8 shows the amount of calcium (mg/g of dry tissue) in samples implanted under the skin of rats of the internal thoracic artery of a pig at various periods after implantation.
  • pericardium was rinsed three times with an excess of 0.9% by weight NaCl solution and put into a 5% by weight ethylene glycol diglycidylether solution, where it was stored until further use.
  • the comparative samples used were pig pericardium portions which were treated with 0.625% by weight glutaraldehyde in 50 mM phosphate buffer pH 7.4 (GA) or with 5% by weight ethylene glycol diglycidylether (DEE) and 100 IU/ml heparin in 50 mM phosphate buffer pH-value 7.4 (DEE+heparin) (see RU 2 008 767).
  • Production of the comparative samples was effected in accordance with the description set forth in relation to comparative Examples 1.
  • Example 1 The operation of determining the density of transverse cross-linking, the properties in respect of elasticity and deformation and the amount of immobilised heparin was effected as described in Example 1. The results obtained in Example 1 and comparative Examples 1 are confirmed by the results obtained in the present case.
  • Example 3 According to the Invention/Comparative Examples 3 TABLE 9 Table 9 shows the relative content of free methionine, tyrosine, lysine and hydroxylysine residues (related to 1000 amino acid residues) in pig pericardia. Ex. of the Amino acid native tissue GA DEE + heparin inv.
  • Table 10 shows the amount of immobilised heparin.
  • DEE + heparin Example according to the invention 760 ⁇ 10 ⁇ g/g dry tissue 2640 ⁇ 85 ⁇ g/g dry tissue
  • Table 11 shows the physical-mechanical parameters of pig pericardium portions conserved with various methods.
  • Conserving agent ⁇ [kg/cm 2 ] ⁇ [%] h [cm] Glutaradehyde 119.8 ⁇ 6.2 48.5 ⁇ 5.8 0.046 ⁇ 0.003 DEE + heparin 123.3 ⁇ 11.4 58.4 ⁇ 3.5 0.044 ⁇ 0.004 Ex. of the inv. 125.5 ⁇ 12.3 57.0 ⁇ 3.6 0.045 ⁇ 0.005

Abstract

The invention concerns a method of conserving biological prostheses, wherein the method includes the following steps: (a) treating biological prostheses with a solution which contains a mixture of epoxide compounds which are at least in part of different lengths; (b) treating the biological prosthesis treated in accordance with step (a) with an antithrombotic-bearing solution; and (c) possibly storing the prosthesis treated in accordance with step (b) in a sterilising solution. The invention further concerns a biological prosthesis produced in accordance with the method of the invention and a conserving agent.

Description

  • The invention concerns a method of conserving biological prostheses and biological prostheses produced in accordance with that method. The invention further concerns a conserving solution for conserving biological prostheses.
  • Biological prostheses can be produced from body components of human beings and animals. For example heart valves, arteries etc of cattle or pigs are used as implants in human beings.
  • It will be appreciated that the biological prostheses must be chemically treated prior to implantation in the organism of the human being. The treatment method must ensure:
      • 1) the absence of immunogenity (that applies equally to heterologous and allogenous tissue);
      • 2) sterility of the implant;
      • 3) high strength, elasticity and deformation properties of the biological material; and
      • 4) high biocompatibility whose main parameter, in relation to the biological prostheses, is the absence of calcification and thromboses in the event of long-term use in the recipient organism.
  • For more than 30 years now glutaraldehyde has represented the main conserving agent for cardiac-circulatory bioprostheses (biological prostheses). Glutaraldehyde reacts with the amino groups of lysine and hydroxylysine. As a result of those reactions, chemical bonds are formed, which are represented in particular by Schiff's bases or pyridine bases. Glutaraldehyde ensures reliable sterility and the suppression of antigenic properties of the biological material.
  • Glutaraldehyde however makes the tissue stiff and hydrophobic and the surface assumes a rough disordered relief. In addition the chemical compounds of glutaraldehyde and collagen have in their structure ligands for complex formation with calcium cations. Those complexes do in fact subsequently become centers of hydroxyapatite crystallisation. In overall terms the result of this is that the glutaraldehyde has a negative influence on the thrombosis-resistant properties of the tissue and gives rise to calcification of the biological materials.
  • In order to eliminate the negative influence of glutaldehyde on the biological material, methods have been developed for the additional chemical modification of biological prostheses.
  • For increasing thrombosis resistance use was made for example of heparin (U.S. Pat. No. 3,988,782) while aminodiphosphonates were used for the prophylaxis of calcification (U.S. Pat. No. 4,553,974). However those methods do not have the expected effect as the negative influence of the glutaraldehyde as a main conserving agent on the tissue is excessively great.
  • A greater effect can be achieved by replacing the main conserving agent by a cross-linking agent, the structural formula of which does not contain any aldehyde group.
  • Methods are known for conserving biological prostheses using individual polymer (U.S. Pat. No. 4,806,595 and U.S. Pat. No. 5,080,670) and non-polymer (U.S. Pat. No. 5,880,242 and RU 2 008 767) epoxide compounds.
  • Epoxide compounds are effective cross-linking agents, guarantee strength and elasticity of the biological material, inhibit calcification of the biological prostheses and have pronounced antigen-depressive properties.
  • To improve the thrombosis resistance of the tissue, it is possible to implement an additional modification with heparin (U.S. Pat. No. 4,806,595 and RU 2 008 767). The disadvantages of those methods are as follows:
      • 1) A masking effect which is characteristic of non-polymer or polymer di-epoxides when one of the epoxy groups reacts with collagen but the other remains without a bond, that is to say it does not react. On the one hand those unbound, that is to say free epoxy groups exhibit a cytotoxic effect, on the other hand they result in insufficient density in terms of transverse cross-linking, which has a negative influence on the strength properties of the tissue.
      • 2) The use of individual polymer epoxides, in the structural formula of which there are contained more than two epoxide groups, reduces the masking effect but it detrimentally affects transverse cross-linking and increases the content of free epoxide groups in the tissue. Without an additional modification which is targeted at closing or converting those groups, on the one hand the cytotoxic effect is increased. On the other hand the number of such epoxide groups is too low for saturation of the biological material with substances which impart additional properties to the biological prostheses (heparin, anti-bacterial agents and so forth).
  • The method known from U.S. Pat. No. 4,806,595 for heparin treatment of epoxy-conserved biological prostheses includes the use of protamine which is firmly bound to the collagen by an epoxide bond. The procedure involves in turn fixing on the protamine heparin which, lifting off the surface, exerts an anti-coagulant function.
  • The effectiveness of such a method is however limited in respect of time and requires the use of an intermediate reagent, namely protamine. The possibility of bonding protamine to the collagen—if this is involves collagen from the bonding tissue of the biological prosthesis—is in turn limited by the number of free reactive groups of the conserving agent as the main proportion of those groups is required for the cross-linking effect.
  • U.S. Pat. No. 5,165,919 discloses a method of covalent fixing of heparin on medical implants by the interaction of amino and epoxy groups. That method however was developed for polymer materials and cannot be used for biological prostheses.
  • The object of the invention is to provide a method of conserving biological prostheses which are resistant to calcification and thrombosis formation and have an enhanced level of strength and elasticity. Another object of the invention is to provide improved conserved biological prostheses.
  • The object of the invention is attained by a method having the features of claim 1. Preferred developments are recited in appendant claims 2 to 19.
  • The object of the invention is further attained by a biological prosthesis as set forth in claim 20. A preferred embodiment of the biological prosthesis is recited in appendant claim 21.
  • The object is further attained by the provision of a conserving agent for biological prostheses as set forth in claim 22. Preferred developments are recited in appendant claims 23 to 27.
  • In accordance with the invention preferably mixtures of polymer and non-polymer epoxide compounds are used for conserving biological prostheses, wherein 2 and more epoxide groups are present in the structural formula of the epoxide compounds.
  • Preferably a solution with a mixture of at least three different epoxide compounds (components) is used.
  • In a further preferred feature the antithrombotic is selected from the group which consists of heparin, low-molecular heparin, heparinoids, hirudin and mixtures thereof.
  • It is essential in accordance with the invention that the antithrombotic has antithrombotic or anti-coagulating properties. In that respect it is possible in accordance with the invention to use all substances which have a heparin-like action.
  • Thus it is also possible to use chemically, mechanically and/or enzymatically modified heparin, truncated heparin, recombinant heparin or mixtures thereof insofar as the correspondingly modified heparin has antithrombotic properties.
  • Preferably heparin is used in accordance with the invention.
  • It was surprisingly found that:
      • 1) the strength of the biological prosthesis is increased by transverse connections as the accessibility of reactive groups of collagen in the biological prosthesis for an interaction with various conserving agents which have various molecule lengths is guaranteed. That enhances the strength of the biological material and ensures a better antigen depression effect;
      • 2) the use of compounds with more than 2 epoxide groups in the mixture of epoxide compounds permits the production of biological material with a predetermined number of free epoxy groups;
      • 3) subsequently heparin can be immobilised on those groups to impart thrombosis resistance. Immobilisation of heparin in the complex with acetylsalicylic acid strengthens the thrombosis-resistance effect.
  • After conservation and modification with heparin the biological prostheses produced in that way can be stored in a solution of any compound which guarantees sterility. Preferably epoxide compounds are used in order to avoid possible additional chemical reactions.
  • The subject-matter of the present invention is thus on the one hand a method of conserving biological material which can be used in particular for producing heart and blood vessel valve prostheses. On the other hand the subject-matter of the invention is the provision of the biological prostheses which are conserved in accordance with the method of the invention.
  • In accordance with the invention, preferably to provide the conserving effect instead of individual epoxide conserving agents, mixtures of polymer and non-polymer epoxide compounds with a differing number of epoxide groups (2 and more) are used. The composition of the mixture can be varied in dependence on the nature of the biological material and the aims of a subsequent chemical modification.
  • Preferably the epoxide group in the epoxide compounds used is a constituent of a glycidol residue.
  • In order at the same time to improve the thrombosis-resistance properties and to close, that is to say transform, the free epoxide groups which have not bound to the collagen in the conservation procedure subsequent treatment of the biological material with heparin and acetylsalicylic acid is implemented.
  • Preferably a mixture of polymer and non-polymer epoxide compounds is used for conserving heart-circulatory bioprostheses (bioprosthesis—biological prosthesis).
  • In accordance with the invention the term a polymer epoxide compound is used to identify an epoxide compound which is composed of at least two repetitive, directly interconnected units to which epoxy group-bearing residues such as for example glycidol or 2,3-epoxypropan-1-ol are joined.
  • Preferably the polymer epoxide compounds have a degree of polymerisation of at least two, more preferably between three and 25, still more preferably between three and 15, in particular between four and nine. In this respect the degree of polymerisation relates to the polymer proportion of the epoxide compound, bearing the epoxy groups.
  • Instead of a polymer epoxide compound it is also possible to use an epoxide compound with between two and three epoxide groups, wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms, for example a tetramethylene group. Preferably arranged between the at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least six, preferably six, carbon atoms, such as for example a hexamethylene group.
  • In accordance with the invention the term non-polar epoxide compound is used to identify an epoxide compound which does not have any repetitive, directly interconnected units to which epoxy group-bearing residues such as for example glycidol or 2,3-epoxypropan-1-ol are joined.
  • It may be advantageous to vary the composition of the mixture in dependence on the association in respect of nature and tissue of the biological material. That is related to the spatial configuration and the composition of the collagens of the various tissues and the different accessibility of the reactive amino acid groups of the collagen for the conserving agents which have different structural formulae.
  • In addition the composition of the mixture depends on the purpose of the additional chemical modification; saturation of the biological material with a predetermined number of epoxide groups which are required for covalent immobilisation of biologically active substances is possible. Thus for example upon immobilisation of heparin a large number of epoxide groups is required.
  • For that purpose the mixture is preferably adjusted as follows:
  • 40-80% by weight, more preferably 50-70% by weight, of at least one non-polymer epoxide compound with two epoxide groups;
  • 5-20% by weight, more preferably 10-15% by weight, of at least one polymer epoxide compound with between two and three epoxide groups and/or at least one epoxide compound with between two and three epoxide groups, wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms; and
  • 15-45% by weight, more preferably 20-35% by weight, of at least one epoxide compound with at least three epoxide groups;
  • wherein the total amount is 100% by weight. The foregoing percentage details of the respective epoxide compound in percent by weight relate in each case to the total amount of epoxide compounds used.
  • In a modification of high-molecular polymer substances in contrast the number of reactive groups must be low as supersaturation of the tissue of the biological prosthesis with high-molecular polymers results in an impairment of the properties in respect of elasticity and deformation. Accordingly use of the epoxide mixtures of differing composition permits the amount of substance which is immobilised on the biological material to be controlled or influenced.
  • For that purpose the mixture is preferably adjusted as follows:
  • 70-90% by weight, more preferably 75-85% by weight, of at least one non-polymer epoxide compound with two epoxide groups;
  • 5-20% by weight, more preferably 10-15% by weight, of at least one polymer epoxide compound with between two and three epoxide groups and/or at least one epoxide compound with between two and three epoxide groups, wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms; and
  • up to 5% by weight, more preferably 1-2% by weight, of at least one epoxide compound with at least three epoxide groups;
  • wherein the total amount is 100% by weight. The foregoing percentage details of the respective epoxide compound in percent by weight relate in each case to the total amount of epoxide compounds used.
  • In the case of the above-specified mixtures a non-polymer, preferably low-molecular compound, with two reaction groups, must be present in the mixture. For example it is possible to use alkane diol diglycidylether such as for example butane-1,4-diol diglycidylether, polyalcohol diglycidylether such as for example glycerine diglycidylether, alkylene glycol diglycidylether such as ethylene glycol diglycidylether or mixtures thereof. Preferably ethylene glycol diglycidylether is used.
  • Those compounds ensure intermolecular transverse cross-linking of the collagen and intramolecular cross-linking of proteoglycans and proteins of the cell elements which represent the most active antigenic determinants.
  • The concentration of non-polymer epoxide compound with two epoxide groups (di-epoxide compound) in the mixture is preferably 1-95% by weight, more preferably 20-90% by weight. Very good results were obtained with a concentration of 40-80% by weight.
  • The second component in the mixture is a polymer epoxide compound which contains between two and three epoxide groups in the structural formula and/or an epoxide compound with between two and three epoxide groups, wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms.
  • For example it is possible to use polyalkylene glycol diglycidylethers such as for example polyethylene glycol diglycidylether, polytetramethylene glycol diglycidylether, polypropylene glycol diglycidylether or mixtures thereof.
  • Instead of or in addition to the above-noted polymer epoxide compound it is also possible to use alkane diol diglycidylethers such as for example hexane-1,6-diol diglycidylether and/or higher dicarboxylic acid diglycidylesters.
  • In accordance with the invention the term higher dicarboxylic acid diglycidylester is used to identify glycidol esterified with higher dicarboxylic acids (2,3-epoxypropan-1-ol), that is to say diglycidylesters of higher dicarboxylic acids. Identified as higher dicarboxylic acids are those which have more than 12 carbon atoms.
  • By way of example higher dicarboxylic acid diglycidylesters which can be used are Denacol EX-1111 (mixture of two acids with a molecular weight of 398 g/mol and 454 g/mol) or Denacol EX-1112 (mixture of two acids with the same molecular weight of 450 g/mol but of differing structure) from Nagase Company Ltd, Japan.
  • Preferably polyethylene glycol diglycidylether is used. Preferably the polyethylene glycol diglycidylether has a degree of polymerisation of 3-12, more preferably 4-9.
  • That component supplements cross-linking of the collagen by inter-fibrillar bonds. The concentration in the mixture is preferably 1-95%, more preferably 2-40% by weight, still more preferably 5-20% by weight.
  • The third component is an epoxide compound with a number of epoxide groups of at least three, for example four, five or more.
  • Preferably in that respect polyalcohol polyglycidylethers are used such as for example sorbitol polyglycidylether, glycerine polyglycidylether and the like, polysaccharide polyglycidylether or mixtures thereof. Preferably pentaerythrol polyglycidylether is used.
  • That third component saturates the tissue with an optimum number of free epoxide groups, to which heparin can be immobilised without the use of additional reagents. The concentration of the component in the mixture is preferably 1-95% by weight, more preferably 10-50% by weight. Very good results were obtained with a concentration of 15-35% by weight.
  • The foregoing percentage details of the respective epoxide compound in percent by weight relate respectively to the total amount of epoxide compounds used.
  • The method according to the invention permits an increase in the density of cross-linking of the collagen, which has an advantageous effect on the strength properties of the biological prosthesis. The use of mixtures of polymer and non-polymer epoxides imparts to the biological material a higher level of resistance to calcification.
  • Saturation of the tissue with free epoxide groups makes it possible to implement covalent immobilisation of heparin on the biological prosthesis when pre-treated in that way.
  • In relation to the functional groups of the heparin, the epoxy group represents one of the most reactive groups in the polymers, including also in biological materials. Binding of the heparin by way of the amino group does not have a disadvantageous effect on the anti-coagulant properties thereof.
  • Reaction with the epoxy group makes it possible to implement immobilisation of heparin under ‘gentle’ conditions which exclude unwanted physical-chemical changes in the biological material. Reaction of heparin with the epoxy groups can take place in a wide pH-range of the medium (pH 2-11).
  • In terms of modification of the biological tissue, preferably a pH-value of 5-8 is used, for example employing phosphate buffers, phosphate-citrate buffers and/or acetylsalicylic acid.
  • Such an operating procedure makes it possible on the one hand to achieve an improvement in the thrombosis-resistant properties and on the other hand to neutralise the free epoxy groups which are always present in the biological material as a result of the masking effect.
  • The introduction of a third component, that is to say a compound with a number of epoxy groups of at least 3, into the epoxide conserving agent makes it possible to increase the amount of immobilised heparin. The covalently bound, that is to say immobilised heparin does not pass into the bloodstream but has an antithrombotic effect due to binding and sorption to the protein layers and smoothing of the surface of the biological prosthesis.
  • The use of acetylsalicylic acid for setting an acid pH-value in the immobilisation of heparin surprisingly further increases the thrombosis resistance of the surface.
  • To produce a conserved biological prosthesis according to the invention for heart-circulation surgery, such as for example biological heart valve prostheses, it is possible to use for example aorta complexes of a pig or pericardia of cattle. In the case of arteriosclerosis for example damaged arteries can be replaced by the internal thoracic artery or the head artery of cattle.
  • Allogenous or heterologous mitral valves or tricuspidal valves can be used for the orthotopic replacement of heart valves. For intracardial plastic surgery and angioplastic surgery it is possible to use pericardia from cattle, the allogenous hard meninges or body-specific pericardia. Valves, membrane-like tissues and vessels, for example arteries, veins, artery segments, vein segments and so forth can be taken from any biological genuses of mammals, for example cattle, pigs, sheep, human beings and so forth, insofar as they are suitable in respect of their anatomical features for replacement of one element or another of the heart-circulation system.
  • Examples 1 through 3 according to the invention which are set out hereinafter serve only to further illustrate the invention and in no way limit the scope of protection thereof.
  • In the examples according to the invention a mixture of ethylene glycol diglycidylether (DEE), pentaerythrol polyglycidylether and polyethylene glycol diglycidylether were used in the respectively specified quantitative ratios for conservation of the respective biological prosthesis used.
  • In that respect the examples were all implemented at ambient temperature, that is to say at between about 20° C. and about 25° C. It is also possible to use higher temperatures, but not more than 37° C. In all incubation steps, the solutions were not agitated. It will be appreciated however that the solutions can also be agitated.
    • EXAMPLE 1 ACCORDING TO THE INVENTION
  • Aortic valve vela of a pig (15 g of moist tissue) were rinsed with 0.90% by weight NaCl solution and put into 200 ml of a conserving solution according to the invention, which is produced from 50 mM phosphate buffer pH 7.4 and contains 6 g of ethylene glycol diglycidylether, 1 g of polyethylene glycol diglycidylether (n=5) and 3 g of pentaerythrol polyglycidylether (number of glycidylether units per molecule: 4).
  • After 48 hours the conserving solution was replaced by an identical but freshly produced solution. After 12 days the valve vela were rinsed with sterile 0.9% by weight NaCl solution and incubated in a heparin solution (100 IU/ml, IU: International Unit) pH 5.0, in which case the pH-value was adjusted by the addition of aqueous acetylsalicylic acid solution, for a period of 3 hours at a temperature of 20° C.
  • Thereafter rinsing was effected five times with an excess of 0.90% by weight NaCl solution and the treated valve vela were put into 5% by weight ethylene glycol diglycidylether solution where they were stored until further use.
  • Production of the Heparin Solution
  • The ratio of heparin:acetylsalicylic acid in the heparin solution, in relation to weight, is about 1.3-16:1. The precise ratio of heparin:acetylsalicylic acid depends on the respective activity (in IU/weight) of the heparin used.
  • By way of example a heparin solution which is suitable for the invention can be produced by the addition of about 7-10 mg/ml of acetylsalicylic acid to a heparin solution with about 75-100 IU/ml. In that case acetylsalicylic acid is added to the heparin solution until the pH-value of the solution is between about 5 and 6. The concentration of the heparin solution is at least 75 IU/ml, preferably 100 IU/ml. It will be appreciated that it is also possible to use solutions with higher heparin concentrations.
    • COMPARATIVE EXAMPLES 1
  • Comparative samples involved using aortic valve vela of a pig, which were treated with 0.6250% by weight glutaraldehyde (GA) in 50 mM phosphate buffer pH 7.4 or with 5% by weight ethylene glycol diglycidylether (DEE) and 100 IU/ml heparin in 50 mM phosphate buffer pH 7.4 (DEE+heparin) (see RU 2 008 767).
  • a) Treatment of Samples with Glutaraldehyde
  • The comparative samples were incubated for 28 days in 0.6250% by weight glutaraldehyde (GA), and 50 mM phosphate buffer pH 7.4 at ambient temperature (between 20° C. and 25° C.). The GA-solution was changed four times, that is to say after the 1st, 3rd, 7th and 21st days. Prior to further use (analysis or implantation) the conserving solution was removed. Subsequently the comparative sample was washed at ambient temperature for one hour without agitation in 0.9% common salt solution. The common salt solution was changed in that procedure after every 20 minutes (a total of three washing steps).
  • b) Treatment of Samples with DEE and Heparin
  • The comparative sample was incubated for 21 days in 5% by weight ethylene glycol diglycidylether (DEE) and 50 mM phosphate buffer pH 7.4 at ambient temperature (20° C.-25° C.). The DEE solution was changed after three days without a washing step. The conserving solution was then removed. The comparative sample was then washed at ambient temperature for one hour without agitation in 0.9% common salt solution. In that procedure the common salt solution was changed after every 20 minutes (a total of three washing steps). The heparin treatment was effected with 100 IU/ml at 37° C. for 8-16 hours. The unbound heparin was removed by washing with 0.9% by weight common salt solution for one hour at ambient temperature (20-25° C.). During the washing operation the common salt solution was not agitated and not changed. The comparative sample was stored in 2-5% by weight DEE solution. The conserving solution was removed prior to further use (analysis or implantation). The comparative example was then washed at ambient temperature for one hour without agitation in 0.9% common salt solution. In that procedure the common salt solution was changed after every 20 minutes (a total of three washing steps).
  • Comparison of Examples According to the Invention and Comparative Examples
  • The improvement in the properties of biological prostheses conserved using the method according to the invention (Examples 1 through 3 according to the invention) is clearly shown by comparison of biological prostheses conserved with conventional conservation methods (comparative Examples 1 through 3). In that respect the density of transverse cross-linking of amino acids in the respective biological prostheses used, the properties in respect of elasticity and deformation, the degree of calcification and the amount of immobilised heparin were determined and compared to each other.
  • The above-indicated parameters were determined in that respect in the following fashion.
  • Determining Transverse Cross-Linking
  • The density of transverse cross-linking was assessed in accordance with the reduction in the number of free amino acid residues in the biological material, in which respect they were determined by an amino acid analysis method.
  • For the amino acid analysis procedure, five samples were taken in each case and washed with distilled water which was renewed twice in one hour. The samples were then lyophilised for three hours (temperature of the sample: between −55° C. and +60° C.). Between 1.5 and 2 mg of dry tissue was put into between 0.15 ml and 2 ml of 6 N HCl and incubated in sealed vacuum flasks for 24 hours at 110° C. Thereafter the acid was evaporated and the residue was diluted in 2.5 ml of lithium citrate buffer and centrifuged. The supernatant substance was subjected to an amino acid analysis operation in an amino acid analyser (CL 5001 BIOTRONIC, Germany) with computer-aided data evaluation (CR-3A, SHIMADZU Integrator, Japan).
  • Determining the Properties in Respect of Elasticity and Deformation
  • The samples were cut out in dumbbell shape (dumbbell test bodies) using an especially shaped blade. That blade is of a standard shape and size and has sharpened edges. Using that blade, samples of a standardised size are cut out of the biological material. Ten samples were investigated in each case.
  • The properties in respect of elasticity and deformation were determined on the tensile strength testing machine ‘Instron-1122’ (manufacturer: INSTRON, England).
  • All the materials investigated were loaded to investigate the breaking/tearing strength at a constant speed (50 mm/min).
  • The average thickness h of the samples (mm) was determined using a micrometer eyepiece.
  • The data were calculated as follows:
  • a) Maximum Tensile Strength (Tensile Stress) σ (kg/cm2)
    σ=P max /S, wherein Pmax is the breaking load (kg) and S is the cross-sectional area of the sample (cm2),
    S=h×b 0, wherein h (cm) is the thickness of the sample and b0 (cm) is the width of the sample.
  • In the present case the width of the sample was set to 0.25 cm using the above-mentioned blade.
  • b) Maximum Stretch εmax (%)
    εmax=(Δl max /l 0)×100,
    Δmax =l max −l 0, wherein ‘lmax’ is the final length and ‘l0’ is the initial length of the sample.
  • In the present case the samples were of an initial length of 11 mm.
  • Determining Calcification
  • Resistance to calcification was investigated by subcutaneous implantation of conserved biological prostheses under the skin of 3-week male rats (diameter of the samples: 7 mm).
  • Three samples, in each case one of the biological samples conserved using GA, DEE+heparin and the conserving solution according to the invention, were each implanted into a respective one of male Vistar rats (n=33), weight 48.64±3.5 g, under ether anesthesia. The implants were removed from 11 animals in each case after a respective period of 30, 60 and 90 days.
  • After removal of the samples they were cleaned of the surrounding tissue, washed with 0.9% NaCl solution and dried at 56° C. for a day. Then each of the samples was hydrolysed in concentrated chloric acid. The samples were then quantitatively investigated for calcium by means of atom absorption spectroscopy.
  • Determining the Amount of Immobilised Heparin
  • The amount of immobilised heparin was determined by means of elementary analysis in accordance with the difference in the content of sulfur in unmodified (control sample) and modified sample portions (modified sample).
  • The method is based on determining the difference in the level of sulfur concentration in test samples (modified sample) and control samples. The sulfur content in heparin is high and low in collagen. A rise in the sulfur content after modification of the biological prosthesis accordingly permits calculation of the amount of heparin immobilised to the biological prosthesis.
    Δ[S] heparin=[S] mod. sample−[S] control sample,
    wherein [S] is the sulfur concentration in [μg/g] dry weight.
  • In that respect calculation of the heparin content in the sample is effected in accordance with the following formula:
  • Y=Δ[S]/S1, wherein Y is the heparin content in the biological material (biological prosthesis) in [mg/g], S1 is the sulfur content in [μg] in 1 mg of heparin.
  • Basically any quantitative determination method can be used for determining the concentration of the sulfur content.
  • In the present case the determination procedure was effected as follows:
  • The method of determining the concentration of the sulfur—which is contained in the range of between 0.2 and 100% in organic samples—is based on the titration of an aqueous-organic medium after combustion of the sample in an oxygen-bearing flask.
  • The sample material (at least 20 g) is firstly cut up with a pair of shears until a thin pulpy consistency is attained. Each sample has 10 ml of distilled water poured thereover. The sample is frozen at −55° C. and lyophilised with a stepwise increase in temperature to +60° C. until dry. The dried sample material obtained in that way is finely ground in an agate mortar until a fine powder is produced.
  • 5 mg of the sample material is weighed out on an analytical balance with a graduation of 0.0001 g. The weighed sample is burnt in a flask which is filled with gaseous oxygen and contains 10 ml of 6% H2O2 solution. After the burning operation the combustion products are rinsed with 5 ml of water and cooled. Added to that solution are 0.25 ml of 2 N HCl, 25 ml of acetone and 2 drops of indicator (0.2% aqueous chlorophosphonazo-III solution (bis-(4-chloro-2-phophonobenzolazo)-2,7-chromotropic acid, Fluka Chemie AG, CH-9471 Buchs, Switzerland). Titration is effected with 0.02 N Ba(NO3)2 solution until there is a transition from a violet-rose coloration to a light blue coloration. For control purposes a blind test is carried out under analysis conditions including combustion and titration.
  • The sulfur content X is calculated as follows: X = ( V - V 0 ) × K A × 1000 ,
    wherein:
      • V is the volume of 0.02 N Ba(NO3)2 solution in [ml], which is used for the titration procedure,
      • V0 is the volume of 0.02 N Ba(NO3)2 solution in [ml], which is used for the titration procedure in the blind test,
      • K is the conversion factor which reproduces the titer of the Ba(NO3)2 solution for the sulfur equivalent in [mg/ml], and
      • A is the weight of the sample in [mg].
  • It will be appreciated that the amount of immobilised heparin can also be determined in another fashion. For example, it is possible to implement quantification of immobilised heparin using toluidine blue which binds to immobilised heparin.
  • Both methods lead to the same result.
  • Result of Example 1/Comparative Examples 1
    TABLE 1
    Table 1 shows the relative content of free amino acid residues
    (related to 1000 amino acid residues) in pig aortic valve vela
    Example
    of the
    Amino acid Native tissue GA DEE + heparin invention
    THR 27.3 ± 0.2 27.6 ± 0.6 24.5 ± 0.3 23.3 ± 0.5
    SER 45.3 ± 0.4 46.7 ± 1.1 41.6 ± 0.4 39.6 ± 0.4
    GLU 97.7 ± 0.0 103.0 ± 0.5  89.1 ± 0.7 88.2 ± 1.2
    OHPRO 110.4 ± 1.2  117.6 ± 1.2  115.6 ± 3.9  110.8 ± 1.8 
    PRO 25.7 ± 0.5 28.6 ± 0.4 65.6 ± 0.6 64.8 ± 1.7
    GLY 238.2 ± 1.2  252.1 ± 4.1  261.1 ± 2.4  272.7 ± 3.2 
    ALA 124.3 ± 0.9  127.7 ± 0.8  122.3 ± 0.5  132.2 ± 3.1 
    VAL 44.3 ± 0.8 41.9 ± 1.2 42.0 ± 1.7 37.1 ± 1.4
    MET 10.7 ± 0.3 10.6 ± 0.2
    ILE 19.9 ± 0.3 20.2 ± 0.3 16.0 ± 0.3 16.7 ± 0.5
    LEU 42.4 ± 0.3 42.6 ± 0.6 36.2 ± 0.3 36.1 ± 0.5
    TYR 10.4 ± 0.3  9.4 ± 0.2  8.7 ± 0.2  1.9 ± 0.5
    PHE 21.9 ± 0.4 20.9 ± 0.4 22.6 ± 0.7 19.7 ± 1.4
    HIS 12.9 ± 0.2 15.8 ± 0.3 35.6 ± 0.4 39.2 ± 0.6
    OHLYS 11.0 ± 0.2  1.4 ± 0.2  2.3 ± 0.2
    LYS 34.0 ± 0.3  3.3 ± 0.2  7.4 ± 0.2
    ASP 66.5 ± 0.5 70.0 ± 0.5 61.2 ± 0.5 60.1 ± 0.9
    ARG 57.1 ± 0.8 63.1 ± 1.2 47.8 ± 0.9 56.3 ± 1.3
  • It is known that epoxide compounds react with methionine, tyrosine, lysine and hydroxylysine of the biological material, whereas glutaraldehyde reacts only with the last two amino acids. The results demonstrated confirm this.
  • In this respect when using the conserving agent according to the invention the density of transverse cross-linking is greater than when using the individual substance—ethylene glycol diglycidylether. That can be seen in particular from a reduction in the relative content of the amino acids methionine, tyrosine, lysine and hydroxylysine.
    TABLE 2
    Table 2 shows the physical-mechanical parameters of pig aortic valve
    vela conserved with various methods.
    Conserving agent σ[kg/cm2] ε[%] h[cm]
    Glutaraldehyde (GA) 59.2 ± 4.6 38.7 ± 1.9 0.059 ± 0.003
    DEE + heparin 69.9 ± 5.9 38.7 ± 1.8 0.046 ± 0.002
    Example of the inv. 93.5 ± 8.0 35.9 ± 1.6 0.041 ± 0.002

    Comments:

    σ: breaking stress under tensile loading,

    ε: relative stretch,

    h: tissue thickness.
  • The sample produced according to the example of the invention, with a smaller thickness, has a better tensile strength characteristic (greater breaking stress).
    TABLE 3
    Table 3 shows the amount of calcium (mg/g of dry tissue) in valve
    vela portions implanted under the skin of rats at various periods after
    implantation.
    Example
    Implantation period GA DEE + heparin of the inv.
    Without implantation  2.25 ± 0.10 2.18 ± 0.08  2.23 ± 0.11
    30 days 125.6 ± 10.2 2.5 ± 0.07 2.15 ± 0.08
    60 days 211.7 ± 12.4 2.8 ± 0.10  2.3 ± 0.07
    90 days 265.4 ± 21.3 2.5 ± 0.09  2.7 ± 0.11
  • The sample produced in accordance with the example of the invention has an extremely low degree of calcification.
    TABLE 4
    Table 4 shows the amount of immobilised heparin.
    DEE + heparin Example according to the invention
    530 ± 20 μg/g dry tissue 2340 ± 120 μg/g dry tissue
  • The sample produced in accordance with the example of the invention has a very high content of immobilised heparin.
    • EXAMPLE 2 ACCORDING TO THE INVENTION
  • Segments of the internal thoracic artery of a pig (25 g of moist tissue) were rinsed with 0.9% by weight NaCl solution and put into 200 ml of a conserving solution which is produced from 50 mM HEPES-buffer pH 7.4 and contains 8 g of ethylene glycol diglycidylether, 0.5 g of polyethylene glycol diglycidylether (n=6) and 1.5 g of pentaerythrol polyglycidylether (number of glycidylether units per molecule: 4).
  • After 48 hours the conserving solution was replaced by an identical but freshly produced solution. After 12 days the segments were rinsed with sterile 0.9% by weight NaCl solution and incubated in a heparin solution (100 IU/ml) pH 5.0, wherein the pH-value was adjusted by the addition of aqueous acetylsalicylic acid solution (production, see Example 1 according to the invention), for a period of 4 hours at a temperature of 20° C. Production of the heparin solution was effected as described in Example 1.
  • Thereafter the segments were rinsed three times with an excess of 0.9% by weight NaCl solution and put into a 5% by weight ethylene glycol diglycidylether solution, where they were stored until further use.
    • COMPARATIVE EXAMPLES 2
  • The comparative samples used Were segments of the internal thoracic artery of a pig, which were treated with 0.625% by weight glutaraldehyde in 50 mM phosphate buffer pH 7.4 (GA) and with 5% by weight ethylene glycol diglycidylether and 100 IU/ml heparin in 50 mM phosphate buffer pH-value 7.4 (DEE+heparin) (see RU 2 008 767). Production of the comparative samples was effected in accordance with the description set forth in relation to comparative Examples 1.
  • Result Example 2/Comparative Examples 2
  • The operation of determining the density of transverse cross-linking, the degree of calcification and the amount of immobilised heparin was effected as described hereinbefore in relation to Example 1. The results contained in Example 1 and comparative Examples 1 are confirmed by the results obtained in the present case.
  • The resistance to thrombosis formation was assessed after the implantation of vessel segments which were conserved in accordance with the method according to the invention (example according to the invention) or for comparison purposes using glutaraldehyde (GA) or ethylene glycol diglycidylether and heparin (DEE+heparin), into the carotid artery of dogs.
  • In that case the vessel segments were between about 3 mm and 3.5 mm in diameter and between about 5 and 7 cm in length and were implanted in the neck artery (carotid) of 24 non-thoroughbred dogs which weighed between 10 and 15 kg.
  • The dogs were previously anesthetized by the intravenous administration of sodium thiopental and mechanically ventilated. A carotid artery segment of between 5 and 7 cm in length was removed from the dogs and the bioprosthesis was implanted in place thereof using 6-0 polypropylene suture material.
  • Eight animals received a ‘GA’ bioprosthesis in the right carotid artery and a ‘DEE+heparin’ prosthesis in the left carotid artery; eight further animals received a ‘DEE+heparin’ bioprosthesis in the right carotid artery and a bioprosthesis according to the invention in the left carotid artery; eight further animals received a bioprosthesis according to the invention in the right carotid artery and a ‘GA’ prosthesis in the left carotid artery. The through-flow in the prostheses was examined prior to closure of the wound by means of pulsation palpation. The penetration capability of the bioprostheses was determined by means of angiography and ultrasound methods (Doppler echography, duplex scanning).
  • Evaluation of the data obtained was effected by means of actuarial analysis. Actuarial analysis is a standardised statistical procedure which is based on the probability of analysed complications, in the present case thrombosis, in which respect events which have already occurred are taken into consideration. Evaluation of the results was effected with the program STATISTICA for Windows (StatSoft, Inc, 1995).
  • The actuarial values in respect of penetration capability in [%] of biological prostheses implanted in the neck artery (carotid) of the dogs were determined and are set forth in Table 5. The values specified in Table 5 are shown in graph form in FIG. 1.
    TABLE 5
    Table 5 shows the actuarial values of penetration capability of
    implanted bioprostheses in [%].
    Period in months GA DEE + heparin Example of the inv.
    0 100%  100%  100% 
    1 75% 97% 98%
    2 70% 90% 98%
    3 35% 88% 95%
    4 15% 86% 90%
    5  5% 80% 88%
    6  0% 76% 86%
    7 73% 86%
    8 72% 86%
    9 70% 80%
    10 68% 80%
    11 65% 78%
    12 65% 78%
  • TABLE 6
    Table 6 shows the relative content of free methionine, tyrosine,
    lysine and hydroxylysine residues (related to 1000 amino acid
    residues) in samples of the internal thoracic artery of a pig.
    Native Ex. of the
    Amino acid tissue GA DEE + heparin inv.
    MET  7.5 ± 0.5 7.3 ± 0.4 6.3 ± 0.2
    TYR 10.0 ± 0.6 11.0 ± 0.4  3.4 ± 0.5
    OHLYS  7.0 ± 0.5 1.0 ± 0.2 0.9 ± 0.2
    LYS 24.1 ± 1.9 3.5 ± 0.5
  • TABLE 7
    Table 7 shows the amount of immobilised heparin.
    DEE + heparin Example according to the invention
    190 ± 10 μg/g dry tissue 1005 ± 90 μg/g dry tissue
  • TABLE 8
    Table 8 shows the amount of calcium (mg/g of dry tissue) in
    samples implanted under the skin of rats of the internal
    thoracic artery of a pig at various periods after implantation.
    Implantation period GA DEE + heparin Ex. of the inv.
    Without 1.39 ± 0.11 1.5 ± 0.03 1.42 ± 0.09 
    implantation
    30 days 52.6 ± 4.1  1.35 ± 0.04  1.5 ± 0.10
    60 days 74.1 ± 9.3  1.8 ± 0.07 1.9 ± 0.07
    90 days 92.0 ± 10.4 1.5 ± 0.04 1.5 ± 0.01
    • EXAMPLE 3 ACCORDING TO THE INVENTION
  • Pig pericardium (30 g of moist tissue) was mechanically cleaned of the surrounding tissue, rinsed with 0.9% by weight NaCl solution and incubated in 200 ml of a conserving solution which is produced from 50 mM HEPES-buffer pH 7.4 and contains 4.5 g of ethylene glycol diglycidylether, 1.5 g of polyethylene glycol diglycidylether (n=4) and 4 g of pentaerythrol polyglycidylether (number of the glycidylether units per molecule: 4).
  • After 48 hours the solution was replaced by an identical abut freshly produced solution. After 12 days the pericardium was rinsed with sterile 0.9% by weight NaCl solution and incubated in a heparin solution (100 IU/ml) pH 6.0, wherein the pH-value was adjusted by the addition of aqueous acetylsalicylic acid solution (production, see Example 1 according to the invention), for a period of 4 hours at a temperature of 20° C.
  • Thereafter the pericardium was rinsed three times with an excess of 0.9% by weight NaCl solution and put into a 5% by weight ethylene glycol diglycidylether solution, where it was stored until further use.
    • COMPARATIVE EXAMPLES 3
  • The comparative samples used were pig pericardium portions which were treated with 0.625% by weight glutaraldehyde in 50 mM phosphate buffer pH 7.4 (GA) or with 5% by weight ethylene glycol diglycidylether (DEE) and 100 IU/ml heparin in 50 mM phosphate buffer pH-value 7.4 (DEE+heparin) (see RU 2 008 767). Production of the comparative samples was effected in accordance with the description set forth in relation to comparative Examples 1.
  • The operation of determining the density of transverse cross-linking, the properties in respect of elasticity and deformation and the amount of immobilised heparin was effected as described in Example 1. The results obtained in Example 1 and comparative Examples 1 are confirmed by the results obtained in the present case.
  • Result of Example 3 According to the Invention/Comparative Examples 3
    TABLE 9
    Table 9 shows the relative content of free methionine, tyrosine,
    lysine and hydroxylysine residues (related to 1000 amino acid
    residues) in pig pericardia.
    Ex. of the
    Amino acid native tissue GA DEE + heparin inv.
    MET 8.8 ± 0.5 8.7 ± 0.5 4.4 ± 0.3
    TYR 8.2 ± 0.2 8.0 ± 0.4 5.0 ± 0.3
    OHLYS 9.9 ± 0.4 1.1 ± 0.1 0.7 ± 0.2 1.5 ± 0.1
    LYS 32.0 ± 1.9  2.8 ± 0.1 1.4 ± 0.3
    ARG 55.6 ± 0.8  58.6 ± 0.5  50.9 ± 0.8  12.7 ± 0.3 
  • TABLE 10
    Table 10 shows the amount of immobilised heparin.
    DEE + heparin Example according to the invention
    760 ± 10 μg/g dry tissue 2640 ± 85 μg/g dry tissue
  • TABLE 11
    Table 11 shows the physical-mechanical parameters of pig
    pericardium portions conserved with various methods.
    Conserving agent σ [kg/cm2] ε [%] h [cm]
    Glutaradehyde 119.8 ± 6.2  48.5 ± 5.8 0.046 ± 0.003
    DEE + heparin 123.3 ± 11.4 58.4 ± 3.5 0.044 ± 0.004
    Ex. of the inv. 125.5 ± 12.3 57.0 ± 3.6 0.045 ± 0.005
  • Comments: σ: breaking strain under tensile loading, ε: relative stretch, h: tissue thickness.

Claims (3)

1-20. (canceled)
21. A conserved biological prosthesis produced in accordance with a method comprising the following steps: (a) treating a biological prosthesis with a solution which contains a mixture of epoxide compounds which are at least in part of different lengths, wherein the mixture of epoxide compounds includes at least one polymer epoxide compound with two or three epoxide groups and/or an epoxide compound with two or three epoxide groups, wherein arranged between at least two epoxide groups is a straight-chain or branched hydrocarbon chain with at least four carbon atoms: (b) treating the biological prosthesis treated in accordance with step (a) with a solution containing an antithrombotic, wherein the antithrombotic is a mixture of heparin and acetylsalicylic acid; and (c) optionally storing the prosthesis treated in accordance with step (b) in a sterilizing solution.
22. A conserved biological prosthesis produced in accordance with a method comprising the following steps:
(a) treating a biological prosthesis with a solution which contains a mixture of epoxide compounds which are at least in part of different lengths, wherein said mixture of epoxide compounds includes at least one epoxide compound with at least three epoxide groups;
(b) treating the biological prosthesis treated in accordance with step (a) with a solution containing an antithrombotic, wherein the antithrombotic is a mixture of heparin and acetylsalicylic acid; and
(c) optionally storing the prosthesis treated in accordance with step (b) in a sterilizing solution.
US11/250,360 2000-12-06 2005-10-14 Method of conserving biological prostheses, conserved biological prostheses and conserving solution Abandoned US20060057552A1 (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
US11/250,360 US20060057552A1 (en) 2000-12-06 2005-10-14 Method of conserving biological prostheses, conserved biological prostheses and conserving solution

Applications Claiming Priority (5)

Application Number Priority Date Filing Date Title
DE10060660.1 2000-12-06
DE10060660A DE10060660A1 (en) 2000-12-06 2000-12-06 Preservation of biological prostheses comprises treating the prosthesis with a solution containing a mixture of epoxy compounds of different lengths and then with a solution containing an antithrombotic agent
US10/433,872 US7014655B2 (en) 2000-12-06 2001-12-03 Method for conserving biological prostheses, conserved biological prostheses and conserving solutions
PCT/DE2001/004494 WO2002058745A1 (en) 2000-12-06 2001-12-03 Method for conserving biological protheses, conserved biological protheses and conserving solutions
US11/250,360 US20060057552A1 (en) 2000-12-06 2005-10-14 Method of conserving biological prostheses, conserved biological prostheses and conserving solution

Related Parent Applications (2)

Application Number Title Priority Date Filing Date
US10/433,872 Continuation US7014655B2 (en) 2000-12-06 2001-12-03 Method for conserving biological prostheses, conserved biological prostheses and conserving solutions
PCT/DE2001/004494 Continuation WO2002058745A1 (en) 2000-12-06 2001-12-03 Method for conserving biological protheses, conserved biological protheses and conserving solutions

Publications (1)

Publication Number Publication Date
US20060057552A1 true US20060057552A1 (en) 2006-03-16

Family

ID=7666021

Family Applications (2)

Application Number Title Priority Date Filing Date
US10/433,872 Expired - Fee Related US7014655B2 (en) 2000-12-06 2001-12-03 Method for conserving biological prostheses, conserved biological prostheses and conserving solutions
US11/250,360 Abandoned US20060057552A1 (en) 2000-12-06 2005-10-14 Method of conserving biological prostheses, conserved biological prostheses and conserving solution

Family Applications Before (1)

Application Number Title Priority Date Filing Date
US10/433,872 Expired - Fee Related US7014655B2 (en) 2000-12-06 2001-12-03 Method for conserving biological prostheses, conserved biological prostheses and conserving solutions

Country Status (6)

Country Link
US (2) US7014655B2 (en)
EP (1) EP1347785B1 (en)
AT (1) ATE270900T1 (en)
CA (1) CA2429603A1 (en)
DE (2) DE10060660A1 (en)
WO (1) WO2002058745A1 (en)

Families Citing this family (43)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6254564B1 (en) 1998-09-10 2001-07-03 Percardia, Inc. Left ventricular conduit with blood vessel graft
DE10010073B4 (en) 2000-02-28 2005-12-22 Fraunhofer-Gesellschaft zur Förderung der angewandten Forschung e.V. Anchoring for implantable heart valve prostheses
DE10010074B4 (en) 2000-02-28 2005-04-14 Fraunhofer-Gesellschaft zur Förderung der angewandten Forschung e.V. Device for fastening and anchoring heart valve prostheses
FR2828263B1 (en) 2001-08-03 2007-05-11 Philipp Bonhoeffer DEVICE FOR IMPLANTATION OF AN IMPLANT AND METHOD FOR IMPLANTATION OF THE DEVICE
DE102004047247B3 (en) * 2004-09-22 2006-03-16 Auto Tissue Gmbh Sterilization process for the production of implantable or transplantable biological material
DE102005003632A1 (en) 2005-01-20 2006-08-17 Fraunhofer-Gesellschaft zur Förderung der angewandten Forschung e.V. Catheter for the transvascular implantation of heart valve prostheses
DE102005051849B4 (en) 2005-10-28 2010-01-21 JenaValve Technology Inc., Wilmington Device for implantation and attachment of heart valve prostheses
DE102005052628B4 (en) 2005-11-04 2014-06-05 Jenavalve Technology Inc. Self-expanding, flexible wire mesh with integrated valvular prosthesis for the transvascular heart valve replacement and a system with such a device and a delivery catheter
US20070213813A1 (en) 2005-12-22 2007-09-13 Symetis Sa Stent-valves for valve replacement and associated methods and systems for surgery
WO2008138584A1 (en) * 2007-05-15 2008-11-20 Jenavalve Technology Inc. Handle for manipulating a catheter tip, catheter system and medical insertion system for inserting a self-expandable heart valve stent
US7896915B2 (en) 2007-04-13 2011-03-01 Jenavalve Technology, Inc. Medical device for treating a heart valve insufficiency
US9138315B2 (en) 2007-04-13 2015-09-22 Jenavalve Technology Gmbh Medical device for treating a heart valve insufficiency or stenosis
ES2903231T3 (en) 2008-02-26 2022-03-31 Jenavalve Tech Inc Stent for positioning and anchoring a valve prosthesis at an implantation site in a patient's heart
US8317858B2 (en) * 2008-02-26 2012-11-27 Jenavalve Technology, Inc. Stent for the positioning and anchoring of a valvular prosthesis in an implantation site in the heart of a patient
US8465540B2 (en) 2008-02-26 2013-06-18 Jenavalve Technology, Inc. Stent for the positioning and anchoring of a valvular prosthesis
US8398704B2 (en) 2008-02-26 2013-03-19 Jenavalve Technology, Inc. Stent for the positioning and anchoring of a valvular prosthesis in an implantation site in the heart of a patient
US9044318B2 (en) * 2008-02-26 2015-06-02 Jenavalve Technology Gmbh Stent for the positioning and anchoring of a valvular prosthesis
US9168130B2 (en) 2008-02-26 2015-10-27 Jenavalve Technology Gmbh Stent for the positioning and anchoring of a valvular prosthesis in an implantation site in the heart of a patient
US8468667B2 (en) * 2009-05-15 2013-06-25 Jenavalve Technology, Inc. Device for compressing a stent
FR2951549B1 (en) 2009-10-15 2013-08-23 Olivier Schussler PROCESS FOR OBTAINING IMPLANTABLE MEDICAL BIOPROTHESES
US8579964B2 (en) 2010-05-05 2013-11-12 Neovasc Inc. Transcatheter mitral valve prosthesis
US11278406B2 (en) 2010-05-20 2022-03-22 Jenavalve Technology, Inc. Catheter system for introducing an expandable heart valve stent into the body of a patient, insertion system with a catheter system and medical device for treatment of a heart valve defect
US10856978B2 (en) 2010-05-20 2020-12-08 Jenavalve Technology, Inc. Catheter system
JP2013526388A (en) 2010-05-25 2013-06-24 イエナバルブ テクノロジー インク Artificial heart valve, and transcatheter delivery prosthesis comprising an artificial heart valve and a stent
US9308087B2 (en) 2011-04-28 2016-04-12 Neovasc Tiara Inc. Sequentially deployed transcatheter mitral valve prosthesis
US9554897B2 (en) 2011-04-28 2017-01-31 Neovasc Tiara Inc. Methods and apparatus for engaging a valve prosthesis with tissue
WO2013016571A1 (en) 2011-07-28 2013-01-31 Harbor Medtech, Inc. Crosslinked human or animal tissue products and their methods of manufacture and use
CN104159543B (en) 2011-10-21 2016-10-12 耶拿阀门科技公司 For expansible heart valve bracket is introduced conduit system in the patient
JP6227632B2 (en) 2012-05-16 2017-11-08 イェーナヴァルヴ テクノロジー ゲゼルシャフト ミット ベシュレンクテル ハフツング Catheter delivery system for introducing expandable heart substitute valve and medical device for treatment of heart valve defects
US9345573B2 (en) 2012-05-30 2016-05-24 Neovasc Tiara Inc. Methods and apparatus for loading a prosthesis onto a delivery system
US9572665B2 (en) 2013-04-04 2017-02-21 Neovasc Tiara Inc. Methods and apparatus for delivering a prosthetic valve to a beating heart
JP6563394B2 (en) 2013-08-30 2019-08-21 イェーナヴァルヴ テクノロジー インコーポレイテッド Radially foldable frame for an artificial valve and method for manufacturing the frame
US10709555B2 (en) 2015-05-01 2020-07-14 Jenavalve Technology, Inc. Device and method with reduced pacemaker rate in heart valve replacement
DE202017007326U1 (en) 2016-01-29 2020-10-20 Neovasc Tiara Inc. Valve prosthesis to prevent flow obstruction
EP3454795B1 (en) 2016-05-13 2023-01-11 JenaValve Technology, Inc. Heart valve prosthesis delivery system for delivery of heart valve prosthesis with introducer sheath and loading system
CN109996581B (en) 2016-11-21 2021-10-15 内奥瓦斯克迪亚拉公司 Methods and systems for rapid retrieval of transcatheter heart valve delivery systems
JP7094965B2 (en) 2017-01-27 2022-07-04 イエナバルブ テクノロジー インク Heart valve imitation
CN111263622A (en) 2017-08-25 2020-06-09 内奥瓦斯克迪亚拉公司 Sequentially deployed transcatheter mitral valve prosthesis
EP3876870B1 (en) 2018-11-08 2023-12-20 Neovasc Tiara Inc. Ventricular deployment of a transcatheter mitral valve prosthesis
JP7438236B2 (en) 2019-04-01 2024-02-26 ニオバスク ティアラ インコーポレイテッド Controllably deployable prosthetic valve
CA3136334A1 (en) 2019-04-10 2020-10-15 Neovasc Tiara Inc. Prosthetic valve with natural blood flow
AU2020279750B2 (en) 2019-05-20 2023-07-13 Neovasc Tiara Inc. Introducer with hemostasis mechanism
AU2020295566B2 (en) 2019-06-20 2023-07-20 Neovasc Tiara Inc. Low profile prosthetic mitral valve

Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4838888A (en) * 1987-04-17 1989-06-13 Baxter Travenol Laboratories, Inc. Calcification mitigation of implantable bioprostheses
US5880242A (en) * 1996-03-04 1999-03-09 Baxter International Inc. Nonpolymeric epoxy compounds for cross linking biological tissue and bioprosthetic grafts prepared thereby

Family Cites Families (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CA1034252A (en) * 1973-09-26 1978-07-04 Ppg Industries, Inc. Antenna windshield
JPS6238172A (en) * 1985-08-12 1987-02-19 株式会社 高研 Production of anti-thrombotic medical material
JP2529112B2 (en) * 1987-08-31 1996-08-28 株式会社 高研 Biological valve
JP2561309B2 (en) * 1988-03-28 1996-12-04 テルモ株式会社 Medical material and manufacturing method thereof
JPH06503018A (en) 1990-11-28 1994-04-07 バクスター インターナショナル インコーポレーテッド Liquid sterilization method
RU2122321C1 (en) 1996-03-06 1998-11-27 Журавлева Ирина Юрьевна Method of treating biological prosthetic means for cardiovascular surgery
US5891196A (en) 1997-04-16 1999-04-06 Baxter International Inc. Method for actively binding heparin to crosslinked biological tissues

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4838888A (en) * 1987-04-17 1989-06-13 Baxter Travenol Laboratories, Inc. Calcification mitigation of implantable bioprostheses
US5880242A (en) * 1996-03-04 1999-03-09 Baxter International Inc. Nonpolymeric epoxy compounds for cross linking biological tissue and bioprosthetic grafts prepared thereby

Also Published As

Publication number Publication date
CA2429603A1 (en) 2002-08-01
US7014655B2 (en) 2006-03-21
DE50102887D1 (en) 2004-08-19
US20040136965A1 (en) 2004-07-15
EP1347785A1 (en) 2003-10-01
DE10060660A1 (en) 2002-06-20
EP1347785B1 (en) 2004-07-14
ATE270900T1 (en) 2004-07-15
WO2002058745A1 (en) 2002-08-01

Similar Documents

Publication Publication Date Title
US7014655B2 (en) Method for conserving biological prostheses, conserved biological prostheses and conserving solutions
EP1139911B1 (en) Method for tissue fixation using epoxides
ES2251178T3 (en) CLACIFICATION RESISTANT MEDICAL ITEMS.
JP2529112B2 (en) Biological valve
CA2183263C (en) Improved process for fixation of calcification-resistant biological tissue
US6132986A (en) Tissue crosslinking for bioprostheses using activated difunctional or polyfunctional acids
US5509932A (en) Fixed tissue medical devices comprising albumin-binding dyes
US5882850A (en) Method for reducing calcification of biological tissue used implantable bioprostheses
Park et al. Novel anti-calcification treatment of biological tissues by grafting of sulphonated poly (ethylene oxide)
Bemacca et al. Chemical modification of bovine pericardium and its effect on calcification in the rat subdermal model
Noishiki et al. Development and evaluation of a pliable biological valved conduit. Part I: preparation, biochemical properties, and histological findings
US20080171906A1 (en) Tissue performance via hydrolysis and cross-linking
US20220001078A1 (en) The system of an element used for the creation of heart valve, the method of manufacturing of modified bacterial cellulose (bc), the set and the element used in cardio surgery
Smith Jr et al. Evaluation of glutaraldehyde-treated tendon xenograft
Smith Jr et al. Bioprosthesis in hand surgery
KR20010038098A (en) Calcification-resistant Heparinized Bioprosthetic Tissue Implants And Preparation Thereof
Kim et al. Negative cilia model for biocompatibility: Sulfonated peo‐grafted polymers and tissues
RU2809478C2 (en) Method of preventing decomposition and degeneration of tissue used in bioprosthesis
Raghavan ECM stabilization strategies for bioprosthetic heart valves for improved durability
Noishiki et al. Polyepoxy compound fixation
WELZ et al. Experimental evaluation of the dialdehyde starch preserved bovine internal mammary artery as a small diameter arterial substitute
RU2008767C1 (en) Method for conservation of biological tissues for prosthetics of heart and vessel valves
Zeeman et al. Cross-linking and calcification of collagen-based materials
US20030219711A1 (en) Process for treatment of biological tissues
Friebe Neomycin enhances glutaraldehyde crosslinking and glycosaminoglycan stability in bioprosthetic heart valves

Legal Events

Date Code Title Description
AS Assignment

Owner name: FREY, RAINER, GERMANY

Free format text: ASSIGNMENT OF ASSIGNORS INTEREST;ASSIGNORS:BARBARASH, LEONID;JOURAVLEVA, IRINA;NOVIKOVA, SVETLANA;REEL/FRAME:017112/0872

Effective date: 20030728

STCB Information on status: application discontinuation

Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION