METHOD FOR PRODUCING COLLAGEN VITRIGEL, METHOD FOR PRODUCING PURIFIED COLLAGEN VITRIGEL, AND COLLAGEN VITRIGEL AND PURIFIED COLLAGEN VITRIGEL PRODUCED BY SAID METHODS

Abstract

An object is to produce a collagen vitrigel, which has a high film strength even without performing a crosslinking treatment, and is easily produced and processed industrially and mechanically, and is also easy to handle and is highly safe, from collagen, and a purified product thereof. In order to achieve the object, it is directed to a method for producing a collagen vitrigel characterized by gelling collagen with a gelling agent containing an inorganic carbonate and a compound selected from the group consisting of an inorganic chloride and an inorganic phosphate, subsequently vitrifying the obtained collagen gel, and further subjecting the vitrified collagen gel to a hydration treatment; a method for producing a purified collagen vitrigel characterized by desalting, equilibrating, and further drying the collagen vitrigel; and a collagen vitrigel and a purified collagen vitrigel obtained by these methods.

Claims

1. A method for producing a collagen vitrigel, the method comprising: gelling collagen with a gelling agent comprising an inorganic carbonate and a compound selected from the group consisting of an inorganic chloride and an inorganic phosphate, to obtain a collagen gel; vitrifying the collagen gel, to obtain a vitrified collagen gel; and subjecting the vitrified collagen gel to a hydration treatment, to obtain the collagen vitrigel.

2. The method for producing a collagen vitrigel according to claim 1, wherein the collagen is porcine skin-derived atelocollagen.

3. The method for producing a collagen vitrigel according to claim 1, wherein a pH at 25 C. of a mixture of the collagen and the gelling agent is 6.2 to 9.8.

4. The method for producing a collagen vitrigel according to claim 3, wherein an ionic strength of a compound contained in the mixture of the collagen and the gelling agent is 0.07 to 0.22.

5. The method for producing a collagen vitrigel according to claim 1, wherein the inorganic carbonate is an inorganic carbonate or an inorganic bicarbonate.

6. The method for producing a collagen vitrigel according to claim 5, wherein the inorganic carbonate is sodium carbonate or potassium carbonate.

7. The method for producing a collagen vitrigel according to claim 5, wherein the inorganic bicarbonate is sodium bicarbonate or potassium bicarbonate.

8. The method for producing a collagen vitrigel according to claim 1, wherein the compound is at least one inorganic chloride selected from the group consisting of sodium chloride, potassium chloride, magnesium chloride, and calcium chloride.

9. The method for producing a collagen vitrigel according to claim 1, wherein the compound is at least one inorganic phosphate selected from the group consisting of sodium phosphate, potassium phosphate, disodium hydrogen phosphate, dipotassium hydrogen phosphate, sodium dihydrogen phosphate, potassium dihydrogen phosphate, and calcium dihydrogen phosphate.

10. The method for producing a collagen vitrigel according to claim 1, wherein the gelling agent does not contain an organic component derived from a medium component and an organic buffer component.

11. A method for producing a purified collagen vitrigel hydrated body, the method comprising desalting and equilibrating a collagen vitrigel prepared by the method of claim 1.

12. A method for producing a purified collagen vitrigel dried body, the method comprising further drying and revitrifying a purified collagen vitrigel hydrated body prepared by the method of claim 11.

13. A method for producing a purified collagen vitrigel hydrated body, the method comprising further rehydrating a purified collagen vitrigel dried body prepared by the method of claim 12.

14. A collagen vitrigel obtained by the method of claim 1.

15. A biological graft material, comprising the collagen vitrigel of claim 14.

16. The biological graft material according to claim 15, wherein the collagen vitrigel does not contain cells.

17. A medical artificial skin, comprising the collagen vitrigel of claim 14.

18. A purified collagen vitrigel hydrated body obtained by the method of claim 11.

19. A biological graft material, comprising the purified collagen vitrigel hydrated body of claim 18.

20. The biological graft material according to claim 19, wherein the purified collagen vitrigel hydrated body does not contain cells.

21. A medical artificial skin, comprising the purified collagen vitrigel hydrated body of claim 18.

22. A purified collagen vitrigel dried body obtained by the method of claim 12.

23. A biological graft material, comprising the purified collagen vitrigel dried body of claim 22.

24. The biological graft material according to claim 23, wherein the purified collagen vitrigel dried body does not contain cells.

25. A medical artificial skin, comprising the purified collagen vitrigel dried body according to claim 22.

26. A collagen gel dried body obtained by gelling collagen with a gelling agent comprising an inorganic carbonate and a compound selected from the group consisting of an inorganic chloride and an inorganic phosphate, and subsequently vitrifying an obtained collagen gel.

Description

BRIEF DESCRIPTION OF DRAWINGS

[0028] FIG. 1 is a view simply showing a production method for a collagen vitrigel and a purified collagen vitrigel of the present invention, a relationship thereof, etc.

DESCRIPTION OF EMBODIMENTS

[0029] In the present description, the collagen vitrigel means a material obtained by rehydrating a collagen gel dried body (collagen xerogel) resulting from vitrification of a collagen gel by drying as shown in FIG. 1. Further, the purified collagen vitrigel means a material obtained by equilibrating the collagen vitrigel after a desalting treatment, a material obtained by revitrification by further drying the equilibrated collagen vitrigel, and a rehydrated material thereof.

[0030] The collagen vitrigel of the present invention is obtained by mixing collagen with an aqueous solution containing an inorganic carbonate and a compound (inorganic salt) selected from the group consisting of an inorganic chloride and an inorganic phosphate, thereby preparing a collagen gel, subsequently vitrifying the obtained collagen gel by drying, thereby obtaining a collagen gel dried body, and further hydrating the collagen gel dried body.

[0031] More specifically, the collagen vitrigel is produced in the following manner. That is, first, a collagen solution and an aqueous solution containing the above-mentioned inorganic carbonate and a compound selected from the group consisting of an inorganic chloride and an inorganic phosphate (hereinafter sometimes abbreviated as gelling agent), thereby forming a collagen sol, and the collagen sol is heated to cause fibril formation, whereby a collagen gel is formed. Subsequently, a collagen gel dried body obtained by drying and vitrifying the collagen gel is subjected to a hydration treatment, whereby a collagen vitrigel is obtained.

[0032] Further, the purified collagen vitrigel is obtained by further desalting (washing) and equilibrating a collagen vitrigel obtained as described above, and further drying and revitrifying the equilibrated collagen vitrigel, followed by rehydration as needed.

[0033] In order to prepare a collagen vitrigel by the method of the present invention, first, it is necessary to prepare a collagen gel by mixing collagen with a gelling agent.

[0034] The collagen to be used in the present invention is not particularly limited with respect to an animal species from which it is derived, and various species can be used. For example, as its origin, mammalian-derived collagen (for example, bovine-derived collagen, porcine-derived collagen, goat-derived collagen, sheep-derived collagen, or monkey-derived collagen), avian-derived collagen (for example, chicken-derived collagen, goose-derived collagen, duck-derived collagen, or ostrich-derived collagen), fish-derived collagen (for example, salmon-derived collagen, sea bream-derived collagen, tuna-derived collagen, tilapia-derived collagen, or shark-derived collagen), reptil-derived collagen (for example, crocodile-derived collagen), amphibian-derived collagen (for example, frog-derived collagen), or invertebrate-derived collagen (for example, jellyfish-derived collagen) can be used. Further, a site from which the collagen is derived is not particularly limited, and for example, a skin, a bone, a cartilage, a muscle, or a scale can be exemplified.

[0035] In the present invention, the collagen to be preferably used is collagen that is stable without denaturation at a temperature not higher than 37 C. that is the human body temperature. The denaturation temperature of collagen is associated with the habitat of an organism from which it is derived, and collagen of an aquatic organism such as a fish has a denaturation temperature in a lower temperature range than that of a human. Therefore, collagen derived from a terrestrial organism having a denaturation temperature close to that of a human is preferred, and it is preferred to obtain collagen from a livestock animal from the viewpoint of industrial stable supply. Examples of the livestock animal include cattle and swine, however, there is a risk that cattle may have a pathogen of BSE (bovine spongiform encephalopathy) or the like, and therefore, cattle is not preferred, and swine is preferred.

[0036] Further, the collagen to be used in the present invention is not limited also with respect to its molecular structure as long as it is fibrous collagen, and examples of a molecular species (type) include type I collagen, type II collagen, type III collagen, and type V collagen. In particular, collagen constituted by type I collagen or type III collagen as a main component is produced in an industrially high yield and can be supplied relatively inexpensively and stably, and thus is preferred. Further, a non-helical structure region (telopeptide) present at the end of a collagen molecule has antigenicity, and therefore, it is more preferred to use atelocollagen obtained by removing the telopeptide by an enzymatic treatment (conversion into atelocollagen).

[0037] The collagen is preferably used in a state of a solution in which the collagen is dissolved in a solvent such as water at the time of gelling, and is more preferably an acid-soluble collagen solution at a pH of 2.0 to 6.0. When the pH is lower than 2.0, a collagen molecule may be hydrolyzed, and when the pH is higher than 6.0, collagen may not be sufficiently solubilized, and therefore both pH ranges are not preferred.

[0038] Further, the collagen concentration in the collagen solution at the time of gelling is not limited as long as the solubility of collagen and the viscosity of the collagen solution do not hinder the production of the collagen gel, and the physical properties of the obtained collagen vitrigel are sufficient for its application, however, the final concentration after mixing with the gelling agent is preferably within a range of 0.05 w/v % to 5.0 w/v %, and more preferably within a range of 0.2 w/v % to 2.0 w/v %.

[0039] On the other hand, the gelling agent to be used in the gelling of collagen is an aqueous solution containing an inorganic carbonate (an inorganic carbonate or an inorganic bicarbonate) and a compound selected from the group consisting of an inorganic chloride and an inorganic phosphate (hereinafter sometimes abbreviated as inorganic salt) as described above.

[0040] In the present invention, the inorganic carbonate to be used as a component of the gelling agent is not limited with respect to its molecular structure as long as it is easily soluble in water, and for example, an inorganic carbonate such as sodium carbonate or potassium carbonate or an inorganic bicarbonate such as sodium bicarbonate or potassium bicarbonate can be used.

[0041] Further, as the inorganic salt to be used as another component of the gelling agent is not limited with respect to its molecular structure as long as it belongs to an inorganic chloride or an inorganic phosphate, and is easily soluble in water, and for example, an inorganic chloride such as sodium chloride, potassium chloride, magnesium chloride, or calcium chloride, or an inorganic phosphate such as sodium phosphate, potassium phosphate, disodium hydrogen phosphate, dipotassium hydrogen phosphate, sodium dihydrogen phosphate, potassium dihydrogen phosphate, or calcium dihydrogen phosphate can be used.

[0042] The types of the inorganic carbonate and the inorganic salt (the inorganic chloride or the inorganic phosphate) and the combination thereof in the gelling agent are not particularly limited as long as fibril formation (self-assembly) of collagen can be caused when mixing the collagen solution therewith, however, it is necessary to contain at least one inorganic carbonate and at least one compound of an inorganic chloride and an inorganic phosphate.

[0043] Further, the pH at 25 C. of the solution (collagen sol) after mixing the gelling agent and the collagen solution is preferably within a range of 6.2 to 9.8, and more preferably within a range of 6.8 to 9.0. In addition, as the concentrations of the inorganic carbonate and the inorganic salt in the gelling agent, the ionic strength in the collagen sol is preferably within a range of 0.07 to 0.22, and more preferably within a range of 0.07 to 0.18.

[0044] In the present invention, the collagen sol prepared by mixing the gelling agent and the collagen solution is heated to cause fibril formation of collagen, whereby a collagen gel is formed, however, the temperature at that time is preferably determined based on the denaturation temperature of the collagen to be used. The fibril formation of collagen is caused at a temperature in the vicinity of the denaturation temperature of the collagen, and fibril formation is not caused at a temperature much lower than the denaturation temperature. That is, the temperature is preferably within a range that is 20 C. or higher with respect to the denaturation temperature and the denaturation temperature or lower. For example, the denaturation temperature of porcine-derived collagen is 41 C., and therefore, the temperature is preferably within a range of 21 C. to 41 C.

[0045] The collagen gel obtained as described above is subsequently subjected to drying and vitrification, thereby forming a collagen gel dried body (collagen xerogel). The vitrification means, for example, a phenomenon in which a hydrogel of a thermally denatured protein such as a hen egg protein (egg white) is dried to sufficiently remove water, thereby converting it into a glass-like material that is hard and has high transparency (Takushi Eisei, Edible eyeballs from fish, Nature, 1990, Vol. 345, pp. 298-299).

[0046] In the method of the present invention, as a drying method for vitrification of the collagen gel, it is preferred to use air drying, and further, the temperature in the air drying is preferably the denaturation temperature of the collagen or lower.

[0047] More specifically, preferably, in the air drying, a constant temperature and humidity machine is used, and for example, it is preferred to perform the vitrification of the collagen gel by leaving the collagen gel to stand under the temperature and humidity conditions of about 10 C. and 40% RH for 2 days.

[0048] The thus obtained collagen gel dried body is subsequently rehydrated, whereby a collagen vitrigel can be formed. As a solution to be used for the rehydration of the collagen gel dried body, an aqueous solution in a neutral pH range (for example, about pH 6.0 to 8.0) such as physiological saline, a phosphate buffer solution, or purified water containing the components to be contained in the gelling agent of the present invention can be exemplified. The solution to be used for the rehydration does not need to have the same composition and concentration as those of the gelling agent when producing the collagen gel, and is not limited thereto.

[0049] In the rehydration, it is preferred to hydrate the collagen gel dried body by immersing it in the above D-PBS() in an amount of 1 mL or more per 10 mg of the collagen gel dried body for 30 minutes or more. The temperature of the aqueous solution to be used for the hydration is preferably a temperature much lower than the denaturation temperature of the collagen to be used, and is preferably 20 C. or lower with respect to the denaturation temperature.

[0050] The collagen vitrigel as a hydrated material is prepared as described above. The collagen vitrigel has a high strength itself, and is easily produced and processed industrially and mechanically, and is easy to handle. Then, in the collagen vitrigel, only inorganic compounds such as an inorganic carbonate, an inorganic chloride, or an inorganic phosphate are used as a component of a gelling agent or a rehydrating agent to be used in the production step, and medium components or organic materials that are conventionally used are not used, and therefore, the collagen vitrigel can be used, for example, as a biologically highly safe collagen vitrigel for medical purposes.

[0051] Note that by further subjecting the collagen vitrigel to a desalting treatment and an equilibration treatment, followed by drying, a purified collagen vitrigel (dried body) can be formed.

[0052] The above-mentioned collagen gel dried body (collagen xerogel) is obtained by drying the collagen gel, and therefore, the inorganic compounds contained in the used gelling agent is concentrated by drying and is apt to be deposited as crystals in some cases. The crystals are unevenly deposited on the surface of the collagen vitrigel dried body, and therefore, the appearance is deteriorated, and also a problem in uniformity of products may occur.

[0053] On the other hand, by subjecting the collagen vitrigel to a desalting treatment and an equilibration treatment, a purified collagen vitrigel (hydrated body) having high uniformity and good appearance can be obtained. The desalting treatment performed here is carried out by immersing the collagen vitrigel in an aqueous solution in a neutral pH range (for example, about pH 6.0 to 8.0), but is preferably carried out by immersing it in D-PBS(). Specifically, for example, the collagen gel dried body is hydrated by immersing it in D-PBS() in an amount of 1 mL or more per 10 mg of the collagen gel dried body, thereby forming a collagen vitrigel, and thereafter, D-PBS() around the collagen vitrigel is removed, and further the collagen vitrigel is immersed in D-PBS() twice of more, whereby desalting of the collagen vitrigel and equilibration thereof with D-PBS() can be carried out.

[0054] The temperature of the aqueous solution in the operation is preferably a temperature much lower than the denaturation temperature of the collagen to be used, and is preferably 20 C. or lower with respect to the denaturation temperature.

[0055] Further, in the drying for revitrification of the purified collagen vitrigel (hydrated body), it is preferred to use air drying, and further, the temperature in the air drying is preferably the denaturation temperature of the collagen or lower. More specifically, it is preferred to use a constant temperature and humidity machine in the air drying, and for example, it is preferred to perform the drying by leaving the purified collagen vitrigel (hydrated body) to stand in a constant temperature and humidity machine under the temperature and humidity conditions of 10 C. and 40% RH for 1 day.

[0056] The collagen vitrigel and the purified collagen vitrigel prepared by the method described above have a high strength per se, and are highly safe as described above, and therefore, can be used particularly as a device for medical purposes such as a cell carrier for regenerative medicine, a wound dressing, an artificial skin, or an adhesion preventive material. Further, as for its shape, it can be processed into an arbitrary shape according to its application, for example, a plate shape, a film shape, a rod shape, a thread shape, a cylindrical shape, a tubular shape, a bag shape, or the like.

EXAMPLES

[0057] Hereinafter, the present invention will be further specifically described by showing Examples, however, the present invention is not limited to the Examples, and various changes can be made within the scope being not deviated from the technical idea of the present invention.

Example 1

(Preparation of Collagen Solution)

[0058] 2 g of porcine skin-derived atelocollagen (NH Foods Ltd. #NMP collagen PS) was dissolved in 200 mL of sterile water, whereby a 1 w/v % collagen solution was prepared.

(Preparation of Gelling Agent)

[0059] To 500 mL of phosphate-buffered saline (D-PBS(), Wako Pure Chemical Industries, Ltd. #045-29795), 1.85 g of sodium bicarbonate (Wako Pure Chemical Industries, Ltd. #191-01305) was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0060] In a 50-mL conical tube (Corning #352070), 20 mL of each of the gelling agent and the 1 w/v % collagen solution was taken and uniformly mixed, and the resulting mixture was used as a collagen sol. The preparation of the collagen sol was performed under ice cooling. Subsequently, an acrylic cylindrical mold (Cosmos Vid, 38.8 mm (outer diameter)34.8 mm (inner diameter)30.0 mm (height)) was placed in a polystyrene rectangular dish (AS ONE Corporation #D210-16), and 10 mL of the collagen sol was filled in the mold. The dish was left to stand in a constant temperature machine at 37 C. for 2 hours to cause fibril formation of collagen, whereby a collagen gel was obtained.

[0061] The collagen gel was vitrified by drying in a constant temperature and humidity machine (the temperature and humidity conditions: 10 C. and 40% RH) for 2 days, whereby a collagen gel dried body was obtained. Further, the collagen gel dried body was hydrated by immersing it in D-PBS() in an amount of 1 mL per 10 mg of the collagen gel dried body, whereby a collagen vitrigel was obtained.

[0062] The collagen vitrigel was washed twice with D-PBS() to remove the excess salt, and the inside of the collagen vitrigel was equilibrated with D-PBS(), and thereafter the collagen vitrigel was dried again in a constant temperature and humidity machine (the temperature and humidity conditions: 10 C. and 40% RH) for 2 days, whereby a purified collagen vitrigel (dried body) was obtained.

Example 2

(Preparation of Gelling Agent)

[0063] 3.21 g of sodium chloride (Wako Pure Chemical Industries, Ltd. #191-01665), 3.40 g of potassium dihydrogen phosphate (Wako Pure Chemical Industries, Ltd. #169-04245), and 1.85 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0064] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 3

(Preparation of Gelling Agent)

[0065] 3.21 g of sodium chloride and 1.85 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0066] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 4

(Preparation of Gelling Agent)

[0067] To 500 mL of phosphate-buffered saline, 0.42 g of sodium bicarbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0068] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 5

(Preparation of Gelling Agent)

[0069] To 500 mL of phosphate-buffered saline, 0.84 g of sodium bicarbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0070] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 6

(Preparation of Gelling Agent)

[0071] To 500 mL of phosphate-buffered saline, 2.27 g of sodium bicarbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0072] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 7

(Preparation of Gelling Agent)

[0073] To 500 mL of phosphate-buffered saline, 0.42 g of sodium bicarbonate and 0.53 g of sodium carbonate (Wako Pure Chemical Industries, Ltd. #196-01595) were added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0074] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 8

(Preparation of Gelling Agent)

[0075] To 500 mL of phosphate-buffered saline, 1.85 g of sodium bicarbonate and 0.53 g of sodium carbonate were added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0076] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 9

(Preparation of Gelling Agent)

[0077] To 500 mL of phosphate-buffered saline, 2.94 g of sodium bicarbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0078] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 10

(Preparation of Gelling Agent)

[0079] 3.21 g of sodium chloride and 0.46 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0080] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 11

(Preparation of Gelling Agent)

[0081] 3.21 g of sodium chloride and 0.84 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0082] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 12

(Preparation of Gelling Agent)

[0083] 3.21 g of sodium chloride and 2.52 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0084] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 13

(Preparation of Gelling Agent)

[0085] 3.21 g of sodium chloride and 2.94 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0086] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 14

(Preparation of Gelling Agent)

[0087] 3.21 g of sodium chloride and 3.36 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0088] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 15

(Preparation of Gelling Agent)

[0089] 3.21 g of sodium chloride, 0.10 g of potassium chloride (Wako Pure Chemical Industries, Ltd. #163-03545), 0.10 g of calcium chloride (Wako Pure Chemical Industries, Ltd. #039-00475), 0.07 g of sodium dihydrogen phosphate monohydrate (Millipore #10049-21-5), 0.42 g of sodium bicarbonate, and 0.53 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0090] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 16

(Preparation of Gelling Agent)

[0091] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, 1.85 g of sodium bicarbonate, and 1.59 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0092] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 17

(Preparation of Gelling Agent)

[0093] 1.17 g of sodium chloride and 4.62 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0094] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 18

(Preparation of Gelling Agent)

[0095] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 0.42 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0096] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 19

(Preparation of Gelling Agent)

[0097] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 0.84 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0098] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 20

(Preparation of Gelling Agent)

[0099] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 1.68 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0100] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 21

(Preparation of Gelling Agent)

[0101] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 2.52 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0102] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 22

(Preparation of Gelling Agent)

[0103] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 3.36 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0104] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 23

(Preparation of Gelling Agent)

[0105] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 4.20 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0106] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 24

(Preparation of Gelling Agent)

[0107] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 0.53 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0108] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 25

(Preparation of Gelling Agent)

[0109] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 1.06 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0110] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 26

(Preparation of Gelling Agent)

[0111] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, 0.84 g of sodium bicarbonate, and 0.27 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0112] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 27

(Preparation of Gelling Agent)

[0113] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, 0.84 g of sodium bicarbonate, and 0.53 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0114] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 28

(Preparation of Gelling Agent)

[0115] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, 0.84 g of sodium bicarbonate, and 1.06 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0116] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 29

(Preparation of Gelling Agent)

[0117] To 500 mL of phosphate-buffered saline, 0.21 g of sodium bicarbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0118] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 30

(Preparation of Gelling Agent)

[0119] To 500 mL of a Hanks' Balanced salt solution (HBSS(), Wako Pure Chemical Industries, Ltd. #085-09355), 0.85 g of sodium carbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0120] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Example 31

(Preparation of Gelling Agent)

[0121] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 0.27 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel and Purified Collagen Vitrigel)

[0122] A collagen vitrigel and a purified collagen vitrigel (dried body) were prepared in the same manner as in Example 1 except that the gelling agent was changed to the above-prepared gelling agent.

Comparative Example 1

(Preparation of Gelling Agent)

[0123] To 490 mL of Dulbecco's modified Eagle's medium (DMEM), 10 mL of 1 mol/L HEPES (4-(2-hydroxyethyl)-1-piperazine ethanesulfonic acid), Thermo Fisher Scientific #15630-080) was added and uniformly mixed therein, and the resulting mixture was used as a gelling agent.

(Preparation of Collagen Vitrigel and Collagen Vitrigel Dried body)

[0124] In a 50-mL conical tube, 20 mL each of the above-prepared gelling agent and the 1 w/v % collagen solution of Example 1 was taken and uniformly mixed, and the resulting mixture was used as a collagen sol. The preparation of the collagen sol was performed under ice cooling. Subsequently, an acrylic cylindrical mold was placed in a polystyrene rectangular dish, and 10 mL of the collagen sol was filled in the mold. The dish was left to stand in a carbon dioxide gas incubator (CO.sub.2 5%) at 37 C. for 2 hours to cause fibril formation of collagen, whereby a collagen gel was obtained.

[0125] The collagen gel was dried and vitrified in a constant temperature and humidity machine, whereby a collagen gel dried body was obtained. Further, the collagen gel dried body was hydrated by immersing it in D-PBS() in an amount of 1 mL per 10 mg of the collagen gel dried body, whereby a collagen vitrigel was obtained. The collagen vitrigel was washed twice with D-PBS() to remove the excess salt and other components, and the inside of the collagen vitrigel was equilibrated with D-PBS(), followed by drying again, whereby a corresponding dried body of the collagen vitrigel was obtained.

Comparative Example 2

(Preparation of Collagen Vitrigel)

[0126] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to D-PBS(). However, the once gelled collagen gel was dissolved and transformed into a sol in the subsequent step, and therefore, the material could not be recovered as a collagen gel dried body, and a collagen vitrigel could not be obtained.

Comparative Example 3

(Preparation of Gelling Agent)

[0127] 8.77 g of sodium chloride was taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel)

[0128] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, the once gelled collagen gel was dissolved and transformed into a sol in the subsequent step, and therefore, the material could not be recovered as a collagen gel dried body, and a collagen vitrigel could not be obtained.

Comparative Example 4

(Preparation of Gelling Agent)

[0129] 1.75 g of sodium chloride, 0.14 g of sodium dihydrogen phosphate monohydrate, and 1.35 g of disodium hydrogen phosphate (Wako Pure Chemical Industries, Ltd. #197-02865) were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel)

[0130] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, the once gelled collagen gel was dissolved and transformed into a sol in the subsequent step, and therefore, the material could not be recovered as a collagen gel dried body, and a collagen vitrigel could not be obtained.

Comparative Example 5

(Preparation of Collagen Vitrigel)

[0131] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to HBSS(). However, collagen was not gelled, and therefore, a collagen gel could not be obtained, so that a collagen vitrigel could not be obtained.

Comparative Example 6

(Preparation of Gelling Agent)

[0132] To 500 mL of HBSS(), 2.12 g of sodium carbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel)

[0133] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, collagen was not gelled, and therefore, a collagen gel could not be obtained, so that a collagen vitrigel could not be obtained.

Comparative Example 7

(Preparation of Gelling Agent)

[0134] To 500 mL of HBSS(), 4.24 g of sodium carbonate was added and dissolved therein, whereby a gelling agent was prepared.

(Preparation of Collagen Vitrigel)

[0135] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, collagen was not gelled, and therefore, a collagen gel could not be obtained, so that a collagen vitrigel could not be obtained.

Comparative Example 8

(Preparation of Gelling Agent)

[0136] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, and 0.07 g of sodium dihydrogen phosphate monohydrate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel)

[0137] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, collagen was not gelled, and therefore, a collagen gel could not be obtained, so that a collagen vitrigel could not be obtained.

Comparative Example 9

(Preparation of Gelling Agent)

[0138] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 0.21 g of sodium bicarbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel)

[0139] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, collagen was not gelled, and therefore, a collagen gel could not be obtained, so that a collagen vitrigel could not be obtained.

Comparative Example 10

(Preparation of Gelling Agent)

[0140] 3.21 g of sodium chloride, 0.10 g of potassium chloride, 0.10 g of calcium chloride, 0.07 g of sodium dihydrogen phosphate monohydrate, and 2.12 g of sodium carbonate were taken and dissolved in 500 mL of sterile water, and the resulting solution was used as a gelling agent.

(Preparation of Collagen Vitrigel)

[0141] Preparation of a collagen vitrigel was attempted by the method of Example 1 except that the gelling agent was changed to the above-prepared gelling agent. However, collagen was not gelled, and therefore, a collagen gel could not be obtained, so that a collagen vitrigel could not be obtained.

Test Example 1

Measurement of Physical Properties:

[0142] The concentrations of the inorganic compounds contained in the collagen sols of Examples 1 to 31 and Comparative Examples 1 to 10, and the ionic strengths and pH thereof, and the film strengths of the purified collagen vitrigels (hydrated bodies) of Examples 1 to 3, Example 8, Example 10, Example 12, Example 18, Examples 23 to 25, Example 27, Examples 29 to 31, and Comparative Example 1 were measured by the following methods. The results are shown in Table 1 to Table 7.

(pH Measurement)

[0143] The pH was measured for the collagen sols before gelling of Examples 1 to 29 and Comparative Examples 1 to 10. The pH measurement was performed by placing 0.5 mL of each collagen sol in a measurement electrode dish of a pH meter (HORIBA, Ltd. #LAQUAtwin AS-712) and measuring the pH.

(Calculation of Ionic Strength)

[0144] When the molar concentrations (mol/L)of ion species A, B, C, . . . of the compounds (except for collagen) contained in a collagen sol are represented by m.sub.A, m.sub.B, m.sub.C, . . . , respectively, and the charge numbers thereof are represented by Z.sub.A, Z.sub.B, Z.sub.C, . . . , respectively, the ionic strength I of the collagen sol is defined by the following formula.

[00001] $\begin{matrix} I = \frac{1}{2} .Math. \underset{i}{.Math.} .Math. m_{i} .Math. Z_{i}^{2} .Math. .Math. (i = A, B, C .Math. .Math. .Math.) & Formula .Math. .Math. 1 \end{matrix}$

(Measurement of Film Strength)

[0145] The film strengths of the purified collagen vitrigels (hydrated bodies) of Examples 1 to 3, Example 8, Example 10, Example 12, Example 18, Examples 23 to 25, Example 27, Examples 29 to 31, and Comparative Example 1 were measured. The film strengths of the purified collagen vitrigels (hydrated bodies) were measured by the following method. That is, the purified collagen vitrigel (dried body) having a diameter of 34.8 mm was rehydrated by immersing it in 8 mL of D-PBS() for 1 hour. The purified collagen vitrigel (hydrated body) obtained by hydration was fixed by being sandwiched between two acrylic plates with a diameter of 50 mm having a hole with a diameter of 5 mm at the center. The fixed film exposed from the hole with a diameter of 5 mm was vertically pierced with a needle made of stainless steel with a diameter of 1.0 mm at a rate of 3.0 mm/min, and the maximum stress (N) before the needle penetrated through the purified collagen vitrigel (hydrated body) was measured using a small desktop testing machine (Shimadzu Corporation #EZ-SX, load cell maximum load 5 N). The measurement was performed at three sites per purified collagen vitrigel (hydrated body), and the average was taken as the maximum stress (N). The operation was performed for three purified collagen vitrigels (hydrated bodies), and the average of the three maximum stresses was taken as the membrane strength (N).

TABLE-US-00001 TABLE 1 Example 1 Example 2 Example 3 Example 4 Example 5 Example 6 Concentration NaCl 68 55 55 68 68 68 (mmol/L) KCl 1.4 1.4 1.4 1.4 CaCl.sub.2 MgSO.sub.4 NaH.sub.2PO.sub.4 KH.sub.2PO.sub.4 0.8 5 0.8 0.8 0.8 Na.sub.2HPO.sub.4 4 4 4 4 NaHCO.sub.3 22 22 22 5 10 27 Na.sub.2CO.sub.3 Components other than Absence Absence Absence Absence Absence Absence inorganic salts Ionic strength 0.165 0.151 0.121 0.113 0.128 0.179 pH 7.5 7.3 7.4 7.2 7.2 7.4 Film strength (N) 0.021 0.002 0.025 0.002 0.028 0.003 No data No data No data (average standard deviation) Remarks

TABLE-US-00002 TABLE 2 Example Example Example Example 7 Example 8 Example 9 10 11 12 Concentration NaCl 68 68 68 55 55 55 (mmol/L) KCl 1.4 1.4 1.4 CaCl.sub.2 MgSO.sub.4 NaH.sub.2PO.sub.4 KH.sub.2PO.sub.4 0.8 0.8 0.8 Na.sub.2HPO.sub.4 4 4 4 NaHCO.sub.3 5 22 35 5.5 10 30 Na.sub.2CO.sub.3 5 5 Components other than Absence Absence Absence Absence Absence Absence inorganic salts Ionic strength 0.128 0.179 0.203 0.072 0.085 0.145 pH 9.0 8.6 7.7 7.0 7.0 7.4 Film strength (N) No data 0.067 0.013 No data 0.024 0.003 No data 0.025 0.004 (average standard deviation) Remarks

TABLE-US-00003 TABLE 3 Example Example Example Example Example Example 13 14 15 16 17 18 Concentration NaCl 55 55 55 55 20 55 (mmol/L) KCl 2.6 2.6 2.6 CaCl.sub.2 0.9 0.9 0.9 MgSO.sub.4 NaH.sub.2PO.sub.4 0.5 0.5 0.5 KH.sub.2PO.sub.4 Na.sub.2HPO.sub.4 NaHCO.sub.3 35 40 5 22 55 5 Na.sub.2CO.sub.3 5 15 Components other than Absence Absence Absence Absence Absence Absence inorganic salts Ionic strength 0.160 0.175 0.093 0.174 0.185 0.078 pH 7.5 7.7 9.0 9.4 7.9 6.3 Film strength (N) No data No data No data No data No data 0.019 0.002 (average standard deviation) Remarks

TABLE-US-00004 TABLE 4 Example Example Example Example Example Example 19 20 21 22 23 24 Concentration NaCl 55 55 55 55 55 55 (mmol/L) KCl 2.6 2.6 2.6 2.6 2.6 2.6 CaCl.sub.2 0.9 0.9 0.9 0.9 0.9 0.9 MgSO.sub.4 NaH.sub.2PO.sub.4 0.5 0.5 0.5 0.5 0.5 0.5 KH.sub.2PO.sub.4 Na.sub.2HPO.sub.4 NaHCO.sub.3 10 20 30 40 50 Na.sub.2CO.sub.3 5 Components other than Absence Absence Absence Absence Absence Absence inorganic salts Ionic strength 0.093 0.123 0.153 0.183 0.213 0.078 pH 6.7 7.1 7.2 7.8 8.5 9.3 Film strength (N) No data No data No data No data 0.033 0.005 0.042 0.005 (average standard deviation) Remarks

TABLE-US-00005 TABLE 5 Example Example Example Example Example Example 25 26 27 28 29 30 Concentration NaCl 55 55 55 55 68 68.5 (mmol/L) KCl 2.6 2.6 2.6 2.6 1.4 2.7 CaCl.sub.2 0.9 0.9 0.9 0.9 MgSO.sub.4 NaH.sub.2PO.sub.4 0.5 0.5 0.5 0.5 KH.sub.2PO.sub.4 0.8 0.2 Na.sub.2HPO.sub.4 4 0.2 NaHCO.sub.3 10 10 10 2.5 2.1 Na.sub.2CO.sub.3 10 2.5 5 10 8.0 Components other than Absence Absence Absence Absence Absence Absence inorganic salts Ionic strength 0.093 0.101 0.108 0.123 0.106 0.104 pH 9.8 8.1 8.6 9.3 6.6 9.6 Film strength (N) 0.053 0.008 No data 0.053 0.005 No data 0.011 0.002 0.054 0.005 (average standard deviation) Remarks

TABLE-US-00006 TABLE 6 Example Comparative Comparative Comparative Comparative Comparative 31 Example 1 Example 2 Example 3 Example 4 Example 5 Concentration NaCl 55 55 68 150 30 68.5 (mmol/L) KCl 2.6 2.6 1.4 2.7 CaCl.sub.2 0.9 0.9 MgSO.sub.4 0.4 NaH.sub.2PO.sub.4 0.5 0.5 1 KH.sub.2PO.sub.4 0.8 0.2 Na.sub.2HPO.sub.4 4 19 0.2 NaHCO.sub.3 22 2.1 Na.sub.2CO.sub.3 2.5 Components other than Absence Presence Absence Absence Absence Absence inorganic salts (a total of 27 components such as amino acids, vitamins, sugars, HEPES, etc.) Ionic strength 0.071 0.131 0.098 0.150 0.150 0.080 pH 6.7 7.0 5.1 3.1 7.4 4.3 Film strength (N) 0.024 0.002 0.022 0.001 (average standard deviation) Remarks Could not be Could not be Could not be Could not be produced produced produced produced

TABLE-US-00007 TABLE 7 Comparative Comparative Comparative Comparative Comparative Example 6 Example 7 Example 8 Example 9 Example 10 Concentration NaCl 68.5 68.5 55 55 55 (mmol/L) KCl 2.7 2.7 2.6 2.6 2.6 CaCl.sub.2 0.9 0.9 0.9 MgSO.sub.4 NaH.sub.2PO.sub.4 0.5 0.5 0.5 KH.sub.2PO.sub.4 0.2 0.2 Na.sub.2HPO.sub.4 0.2 0.2 NaHCO.sub.3 2.1 2.1 2.5 Na.sub.2CO.sub.3 20 40 20 Components other than Absence Absence Absence Absence Absence inorganic salts Ionic strength 0.140 0.200 0.063 0.071 0.123 pH 10.0 10.5 3.2 4.4 10.2 Film strength (N) (average standard deviation) Remarks Could not be Could not be Could not be Could not be Could not be produced produced produced produced produced

[0146] As apparent from Table 1 to Table 6, the purified collagen vitrigels obtained according to the method of the present invention had a sufficient film strength, and also did not substantially contain residual components other than the inorganic salts, were biologically highly safe, and were of practical use.

INDUSTRIAL APPLICABILITY

[0147] As described above, according to the production methods of the present invention, a collagen vitrigel and a purified product thereof that are biologically highly safe are obtained easily at low cost.

[0148] Moreover, the obtained collagen vitrigel and purified collagen vitrigel have a sufficient film strength, are easily produced and processed industrially and mechanically, are easy to handle, and are highly safe, and therefore, are useful as various biological graft materials, for example, a cell carrier for regenerative medicine, a wound dressing, an artificial skin, an adhesion preventive material, and the like.

METHOD FOR PRODUCING COLLAGEN VITRIGEL, METHOD FOR PRODUCING PURIFIED COLLAGEN VITRIGEL, AND COLLAGEN VITRIGEL AND PURIFIED COLLAGEN VITRIGEL PRODUCED BY SAID METHODS

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Cpc classification

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A61L27/02

HUMAN NECESSITIES

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C07K14/78

CHEMISTRY; METALLURGY

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A61L27/3604

HUMAN NECESSITIES

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A61L27/24

HUMAN NECESSITIES

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A61L27/52

HUMAN NECESSITIES

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A61L27/26

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A61L27/60

HUMAN NECESSITIES

International classification

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A61L27/24

HUMAN NECESSITIES

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A61L27/02

HUMAN NECESSITIES

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A61L27/26

HUMAN NECESSITIES

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A61L27/52

HUMAN NECESSITIES

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A61L27/60

HUMAN NECESSITIES

Abstract

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