USE OF ADENOSINE DEAMINASE AND ADENOSINEDEAMINASE MODIFIER IN PREPARATION OF MEDICAMENTFOR WOUND REPAIR IN PATIENT WITH DIABETES
20230144882 · 2023-05-11
Inventors
Cpc classification
A61K38/50
HUMAN NECESSITIES
A61P17/02
HUMAN NECESSITIES
A61K47/60
HUMAN NECESSITIES
Y02A50/30
GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
International classification
A61K38/50
HUMAN NECESSITIES
A61K47/60
HUMAN NECESSITIES
Abstract
The present disclosure provides use of adenosine deaminase (ADA) and an ADA modifier in preparation of a medicament for wound repair in a patient with diabetes. It is found for the first time that the ADA (EC 3.5.4.4) and a polyethylene glycol-modified adenosine deaminase (PEG-ADA) have a significant improvement effect on wound repair of type-2 diabetic mice, and the ADA or the ADA modifier can be developed into a medicament for treating diabetic wounds.
Claims
1. A method for wound repair in a patient with diabetes, wherein adenosine deaminase (ADA) (EC 3.5.4.4) or an ADA modifier is used in the wound repair in a patient with diabetes.
2. The method for wound repair in a patient with diabetes according to claim 1, wherein the diabetes is type 1 or type 2 diabetes.
3. The method for wound repair in a patient with diabetes according to claim 1, wherein the ADA is one selected from the group consisting of a natural ADA extracted from a biological tissue, a recombinant human-, animal- or microbe-derived ADA, and a chemically synthesized ADA.
4. The method for wound repair in a patient with diabetes according to claim 1, wherein the ADA is one selected from the group consisting of a naturally extracted bovine adenosine deaminase and an Escherichia coli-expressed murine adenosine deaminase.
5. The method for wound repair in a patient with diabetes according to claim 1, wherein the ADA modifier is an ADA modifier obtained by chemically modifying the ADA to increase stability thereof and prolong half-life thereof.
6. The method for wound repair in a patient with diabetes according to claim 1, wherein the ADA modifier is a polyethylene glycol-modified adenosine deaminase (PEG-ADA).
7. The method for wound repair in a patient with diabetes according to claim 6, wherein the PEG-ADA is one selected from the group consisting of a PEG-modified naturally extracted bovine ADA and a PEG-modified Escherichia coli-expressed murine ADA.
8. The method for wound repair in a patient with diabetes according to claim 1, wherein the medicament for wound repair in a patient with diabetes is a composition comprising one or more of the ADA or the ADA modifier, and further comprises a pharmaceutically acceptable carrier or vehicle.
9. The method for wound repair in a patient with diabetes according to claim 1, wherein the ADA and the ADA modifier have an intraperitoneal injection concentration of 0.1-8 U/g, and a topical application concentration of 1-300 U/mL.
10. The method for wound repair in a patient with diabetes according to claim 1, wherein the ADA and the ADA modifier have an intraperitoneal injection concentration of 5 U/g, and a topical application concentration of 150 U/mL.
Description
BRIEF DESCRIPTION OF THE DRAWINGS
[0014]
[0015]
[0016]
[0017]
DETAILED DESCRIPTION OF THE EMBODIMENTS
[0018] To make those skilled in the art better understand the solution of the present disclosure, the technical solution of the present disclosure will be described clearly and completely below with reference to the examples of the present disclosure and the accompanying drawings. Apparently, the described examples are only a part of, but not all of, the examples. Based on the examples of the present disclosure, all other examples obtained by those of ordinary skill in the art without creative efforts shall fall within the protection scope of the present disclosure.
[0019] All raw materials used in the following examples are commercially available products, unless otherwise specified.
[0020] The ADA (EC 3.5.4.4) or the ADA modifier involved in the present disclosure may be purchased or self-prepared.
[0021] In the examples, male diabetic mice induced by STZ+high-fat diet and adult male db/db mice are used as models of type 2 diabetes.
Example 1
[0022] Effect of naturally extracted bovine ADA on wound repair in diabetic mice:
[0023] 1. Experimental Method
[0024] 1.1 Diabetic Model Establishment:
[0025] Db/db mouse model of diabetes: Male db/db diabetic mice (aged 6 weeks) from the Model Animal Research Center, Nanjing University were used in the experiment. All mice were housed under standard raising conditions. The mice were raised under a 12 h:12 h light:dark cycle and had free access to food and water. The mice with fasting blood glucose (FBG) higher than 11.1 mmol/L were considered as type 2 diabetic mice and were selected for subsequent research.
[0026] 1.2 Establishment of a Mouse Wound Model
[0027] Animals in each group were anesthetized with pentobarbital sodium (1%), the back was shaved, and a full-thickness wound with a diameter of 8 mm was cut with scissors at the top of the back. Photographs were taken to record the wound healing of mice after administration, and 1 cm.sup.2 was used as a scale to analyze the wound healing of the mice in each group.
[0028] 1.3 Grouping and Administration Method
[0029] Blank control group: A mouse wound model was established and treated with the corresponding drug vehicle (phosphate buffered saline, PBS).
[0030] Diabetic model group: A mouse model of type 2 diabetes and a mouse wound model were established. The mice were treated with the corresponding drug vehicle (PBS).
[0031] Diabetic ADA (injection) treatment group: A mouse model of type 2 diabetes and a mouse wound model were established. Naturally extracted bovine ADA (0.1 U/g, 0.2 U/g, 0.4 U/g, 0.8 U/g, 1.5 U/g, 3 U/g, 5 U/g, and 8 U/g) was intraperitoneally injected daily.
[0032] Diabetic ADA (dripping) treatment group: A mouse model of type 2 diabetes and a mouse wound model were established, and bovine ADA (1 U/mL, 2 U/mL, 4 U/mL, 10 U/mL, 30 U/mL, 80 U/mL, 150 U/mL, and 300 U/mL) was dipped on the wound every day.
[0033] 2. Experimental Results
[0034] 2.1 Effect of ADA on Wound Healing in Diabetic Mice
[0035] The results are shown in
[0036] Compared with the blank control group, the wound healing rate of the mice in the diabetic model group was slower, and the wound area was 30±0.5% after 14 days (the percentage represents the wound area at this time point/original wound area, the same below).
[0037] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (injection) treatment group.
[0038] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (dripping) treatment group.
[0039] The results showed that the naturally extracted bovine ADA could effectively accelerate the wound healing rate of diabetic mice, and the administration by injection was as effective as the administration by dripping.
[0040] And, the injection concentration was effective in the range of 0.1 to 8 U/g, and the therapeutic effect was first strong and then weak with the increase of the concentration within the effective concentration range; the optimum concentration was 5 U/g, but the concentration lower than 0.1 U/g or higher than 8 U/g was ineffective. The application and dripping concentration was effective in the range of 1 to 300 U/mL, and the therapeutic effect became stronger at first and then weakened with the increase of the effective concentration within the effective concentration range; the optimum concentration was 150 U/mL, and the concentration lower than 1 U/mL or higher than 300 U/mL was ineffective.
Example 2
[0041] Effect of PEG-modified naturally extracted bovine ADA on wound repair in diabetic mice:
[0042] 1. Experimental Method
[0043] 1.1 Preparation of PEG-ADA
[0044] ADA was diluted to 500 U/mL with 1 mL of sterile PBS (10 mmol/L, pH 9.0). Subsequently, methoxy polyethylene glycol succinimidyl propionate (mPEG-SPA) with a molecular weight of 20 kDa was added to obtain a final concentration of 100 mg/mL, and the mixture was mixed at room temperature for 5 h to obtain PEG-ADA. Finally, the PEG-ADA was diluted to a final concentration of 150 U/mL with PBS (10 mmol/L, pH 7.4).
[0045] 1.2 Establishment of a Mouse Model of Diabetes
[0046] Db/db mouse model of diabetes: Male db/db diabetic mice (aged 6 weeks) from the Model Animal Research Center, Nanjing University were used in the experiment. All mice were housed under standard raising conditions. The mice were raised under a 12 h:12 h light:dark cycle and had free access to food and water. The mice with FBG higher than 11.1 mmol/L were considered as type 2 diabetic mice and were selected for subsequent research.
[0047] 1.3 Establishment of a Mouse Wound Model
[0048] Animals in each group were anesthetized with pentobarbital sodium (1%), the back was shaved, and a full-thickness wound with a diameter of 8 mm was cut with scissors at the top of the back. Photographs were taken to record the wound healing of mice after administration, and 1 cm.sup.2 was used as a scale to analyze the wound healing of the mice in each group.
[0049] 1.4 Grouping and Administration Method
[0050] Blank control group: A mouse wound model was established. The mice were treated with the corresponding drug vehicle (PBS).
[0051] Diabetic model group: A mouse model of type 2 diabetes and a mouse wound model were established. The mice were treated with the corresponding drug vehicle (PBS).
[0052] Diabetic ADA (injection) treatment group: A mouse model of type 2 diabetes and a mouse wound model were established. PEG-modified naturally extracted bovine ADA (0.1 U/g, 0.2 U/g, 0.4 U/g, 0.8 U/g, 1.5 U/g, 3 U/g, 5 U/g, and 8 U/g) was intraperitoneally injected weekly.
[0053] Diabetic ADA (dripping) treatment group: A mouse model of type 2 diabetes and a mouse wound model were established, and bovine ADA (1 U/mL, 2 U/mL, 4 U/mL, 10 U/mL, 30 U/mL, 80 U/mL, 150 U/mL, and 300 U/mL) was dipped on the wound every day.
[0054] 2. Experimental Results
[0055] 2.1 Effect of ADA on Wound Healing in Diabetic Mice
[0056] The results are shown in
[0057] Compared with the blank control group, the wound healing rate of the mice in the diabetic model group was slower, and the wound area was 30±0.5% after 14 days.
[0058] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (injection) treatment group.
[0059] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (dripping) treatment group.
[0060] The results showed that the PEG-modified naturally extracted bovine ADA could effectively accelerate the wound healing rate of diabetic mice, and the administration by injection was as effective as the administration by dripping.
[0061] And, the injection concentration was effective in the range of 0.1 to 8 U/g, and the therapeutic effect was first strong and then weak with the increase of the concentration within the effective concentration range; the optimum concentration was 1.5 U/g, but the concentration lower than 0.1 U/g or higher than 8 U/g was ineffective. The application and dripping concentration was effective in the range of 1 to 300 U/mL, and the therapeutic effect became stronger at first and then weakened with the increase of the effective concentration within the effective concentration range; the optimum concentration was 150 U/mL, and the concentration lower than 1 U/mL or higher than 300 U/mL was ineffective.
Example 3
[0062] Effects of E. coli-expressed murine ADA on wound repair in diabetic mice:
[0063] 1. Experimental Method
[0064] 1.1 For the preparation of E. coli-expressed murine ADA, refer to the corresponding literature [Kim D, Ku S. Bacillus Cellulase Molecular Cloning, Expression, and Surface Display on the Outer Membrane of Escherichia coli. Molecules. 2018;23(2):503. Published 2018 Feb. 24. doi: 10.3390/molecules23020503].
[0065] 1.2 Establishment of a Mouse Model of Diabetes
[0066] Type 2 diabetic model induced by STZ+high-fat diet: Male C57BL/6 mice (aged 8-10 weeks) from the Model Animal Research Center, Nanjing University were used in the experiment. All mice were housed under standard raising conditions. The mice were raised under a 12 h:12 h light:dark cycle and had free access to food and water. After four-week feeding, intraperitoneal injection was induced with 30 mg/kg STZ for three consecutive days. The mice with FBG higher than 11.1 mmol/L were considered as type 2 diabetic mice and were selected for subsequent research.
[0067] 1.3 Establishment of a Mouse Wound Model
[0068] Animals in each group were anesthetized with pentobarbital sodium (1%), the back was shaved, and a full-thickness wound with a diameter of 8 mm was cut with scissors at the top of the back. Photographs were taken to record the wound healing of mice after administration, and 1 cm.sup.2 was used as a scale to analyze the wound healing of the mice in each group.
[0069] 1.4 Grouping and Administration Method
[0070] Blank control group: A mouse wound model was established. The mice were treated with the corresponding drug vehicle (PBS).
[0071] Diabetic model group: A type 2 diabetic mouse wound model was established. The mice were treated with the corresponding drug vehicle (PBS).
[0072] Diabetic ADA (injection) treatment group: A mouse model of type 2 diabetes and a mouse wound model were established. Murine ADA (0.1 U/g, 0.2 U/g, 0.4 U/g, 0.8 U/g, 1.5 U/g, 3 U/g, 5 U/g, and 8 U/g) was intraperitoneally injected weekly.
[0073] Diabetic ADA (dripping) treatment group: A mouse model of type 2 diabetes and a mouse wound model were established, and murine ADA (1 U/mL, 2 U/mL, 4 U/mL, 10 U/mL, 30 U/mL, 80 U/mL, 150 U/mL, and 300 U/mL) was dipped on the wound every day.
[0074] 2. Experimental Results
[0075] 2.1 Effect of ADA on Wound Healing in Diabetic Mice
[0076] The results are shown in
[0077] Compared with the blank control group, the wound healing rate of the mice in the diabetic model group was slower, and the wound area was still 30±0.5% after 14 days.
[0078] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (injection) treatment group.
[0079] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (dripping) treatment group.
[0080] The results showed that the E. coli-expressed murine ADA could effectively accelerate the wound healing rate of diabetic mice, and the administration by injection was as effective as the administration by dripping.
[0081] And, the injection concentration was effective in the range of 0.1 to 8 U/g, and the therapeutic effect was first strong and then weak with the increase of the concentration within the effective concentration range; the optimum concentration was 5 U/g, but the concentration lower than 0.1 U/g or higher than 8 U/g was ineffective. The application and dripping concentration was effective in the range of 1 to 300 U/mL, and the therapeutic effect became stronger at first and then weakened with the increase of the effective concentration within the effective concentration range; the optimum concentration was 150 U/mL, and the concentration lower than 1 U/mL or higher than 300 U/mL was ineffective.
Example 4
[0082] Effect of PEG-modified E. coli-expressed murine ADA on wound repair in diabetic mice:
[0083] 1. Experimental Method
[0084] 1.1 For the preparation of E. coli-expressed murine ADA, refer to the corresponding literature [Kim D, Ku S. Bacillus Cellulase Molecular Cloning, Expression, and Surface Display on the Outer Membrane of Escherichia coli. Molecules. 2018;23(2):503. Published 2018 Feb. 24. doi: 10.3390/molecules23020503].
[0085] 1.2 Preparation of PEG-Modified ADA
[0086] ADA was diluted to 500 U/mL with 1 mL of sterile PBS (10 mmol/L, pH 9.0). Subsequently, mPEG-SPA with a molecular weight of 20 kDa was added to obtain a final concentration of 100 mg/mL, and the mixture was mixed at room temperature for 5 h. Finally, the PEG-ADA was diluted to a final concentration of 150 U/mL with PBS (10 mmol/L, pH 7.4).
[0087] 1.3 Establishment of a Mouse Model of Diabetes
[0088] Type 2 diabetic model induced by STZ+high-fat diet: Male C57BL/6 mice (aged 8-10 weeks) from the Model Animal Research Center, Nanjing University were used in the experiment. All mice were housed under standard raising conditions. The mice were raised under a 12 h:12 h light:dark cycle and had free access to food and water. After four-week feeding, intraperitoneal injection was induced with 30 mg/kg STZ for three consecutive days. The mice with FBG higher than 11.1 mmol/L were considered as type 2 diabetic mice and were selected for subsequent research.
[0089] 1.4 Establishment of a Mouse Wound Model
[0090] Animals in each group were anesthetized with pentobarbital sodium (1%), the back was shaved, and a full-thickness wound with a diameter of 8 mm was cut with scissors at the top of the back. Photographs were taken to record the wound healing of mice after administration, and 1 cm.sup.2 was used as a scale to analyze the wound healing of the mice in each group.
[0091] 1.5 Grouping and Administration Method
[0092] Blank control group: A mouse wound model was established. The mice were treated with the corresponding drug vehicle (PBS).
[0093] Diabetic model group: A type 2 diabetic mouse wound model was established. The mice were treated with the corresponding drug vehicle (PBS).
[0094] Diabetic ADA (injection) treatment group: A mouse model of diabetes and a mouse wound model were established. E. coli-expressed murine ADA (0.1 U/g, 0.2 U/g, 0.4 U/g, 0.8 U/g, 1.5 U/g, 3 U/g, 5 U/g, and 8 U/g) was intraperitoneally injected weekly.
[0095] Diabetic ADA (dripping) treatment group: A db/db mouse model of diabetes and a mouse wound model were established, and PEG-modified murine ADA (1 U/mL, 2 U/mL, 4 U/mL, 10 U/mL, 30 U/mL, 80 U/mL, 150 U/mL, and 300 U/mL) was dipped on the wound every day.
[0096] 2. Experimental Results
[0097] 2.1 Effect of ADA on Wound Healing in Diabetic Mice
[0098] The results are shown in
[0099] Compared with the blank control group, the wound healing rate of the mice in the diabetic model group was slower, and the wound area was still 30±0.5% after 14 days.
[0100] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (injection) treatment group.
[0101] Compared with the diabetic model group, the wound healing rate was significantly accelerated and the wound area at 14 days was 10±0.5% in the diabetic ADA (dripping) treatment group.
[0102] The results showed that the PEG-modified E. coli-expressed murine ADA could effectively accelerate the wound healing rate of diabetic mice, and the administration by injection was as effective as the administration by dripping.
[0103] And, the injection concentration was effective in the range of 0.1 to 8 U/g, and the therapeutic effect was first strong and then weak with the increase of the concentration within the effective concentration range; the optimum concentration was 1.5 U/g, but the concentration lower than 0.1 U/g or higher than 8 U/g was ineffective. The application and dripping concentration was effective in the range of 1 to 300 U/mL, and the therapeutic effect became stronger at first and then weakened with the increase of the effective concentration within the effective concentration range; the optimum concentration was 150 U/mL, and the concentration lower than 1 U/mL or higher than 300 U/mL was ineffective.