This application claims the priority of Chinese Patent Application No. 202010643578.4 filed at the Chinese Patent Office on Jul. 6, 2020, titled with “USE OF COMPOUND OR PHARMACEUTICALLY ACCEPTABLE SALT, DIMER OR TRIMER THEREOF IN MANUFACTURE OF MEDICAMENT FOR TREATING CANCER”, the entire content of which is incorporated herein by reference.
The present disclosure relates to the field of medicine technology, and in particular to use of a compound or a pharmaceutically acceptable salt, dimer or trimer thereof in the manufacture of a medicament for treating cancer.
Non-communicable diseases are the main cause of death in the world, and cancer is the disease with the highest fatality rate among non-communicable diseases, bringing a heavy burden to the social health and medical system. Traditional cancer treatment is mainly surgery, radiotherapy and chemotherapy, and chemotherapy is the main treatment for advanced cancer.
Classical chemotherapy has serious side effects due to poor targeting. The emergence of targeted chemotherapy drug such as Gleevec has greatly reduced the pain caused by chemotherapy to patients. Targeted drugs are designed based on the different growth characteristics and expression of cancer cells compared with normal cells. For example, Gleevec specifically targets the constitutively activated tyrosine kinases in chronic myelogenous leukemia to achieve a good therapeutic effect (Flynn and Gerriets, 2020). Another distinguishing feature of cancer cells compared with normal cells is the change in metabolism. In order to meet the needs of cell components for rapid proliferation and maintain the energy supply needed for survival, cancer cells prefer to use glucose by aerobic glycolysis, which is called the Warburg effect (Warburg, 1956). Aerobic glycolysis cannot fully oxidize glucose to produce ATP, but can produce a large amount of intermediate metabolites for DNA and protein synthesis to promote cancer cell proliferation. Therefore, it is feasible to target the sugar metabolism of tumor cells to inhibit the proliferation of cancer cells (Kroemer and Pouyssegur, 2008).
Cancer cells absorb glucose from the external environment mainly through glucose transporters. Glucose transporters are divided into two major families, one of which is the GLUT family that transports glucose along the glucose concentration gradient by assisting diffusion, and the other is the sodium-glucose co-transporter SGLT family that co-transports sodium ions for glucose absorption and actively transports glucose from the external for cell consumption by consuming ATP (Navale and Paranjape, 2016). The two main members of the SGLT family are SGLT1 and SGLT2. SGLT2 is mainly distributed at the front end of the proximal convoluted tubule of the kidney, and reabsorbs more than 97% of the glucose from the original urine into the blood through active transport, while SGLT1 is mainly distributed in the epithelial cells of the small intestine chorion and the distal end of the proximal convoluted tubules of the kidney, and through active transport absorbs glucose from food in the intestine and the remaining 3% glucose in the original urine after the absorption by SGLT2 (Dominguez Rieg and Rieg, 2019). Due to the important role of SGLT1 and SGLT2 in sugar absorption and reabsorption, they have become ideal targets for diabetes treatment. Currently Empagliflozin, Canagliflozin and Dapagliflozin targeting SGLT2 have shown good therapeutic effects in the treatment of type 2 diabetes, and the effect of reducing cardiovascular disease. Migliflozin, which targets SGLT1 alone, has entered the clinical research phase. Sotagliflozin, which targets both SGLT1 and SGLT2, has been approved for marketing in the EU.
There is now no report on the use of Sotagliflozin in the treatment of cancer.
In view of this, the technical problem to be solved by the present disclosure is to provide the use of Sotagliflozin in the manufacture of a medicament for treating cancer.
The present disclosure provides use of a compound of formula I
wherein:
R1 is hydrogen, or C1-10-alkyl, C1-5-cycloalkyl or 5-membered heterocyclic ring optionally substituted with one or more R1A;
each R1A is independently amino, ester, amide, thiol, carboxylic acid, cyano, halogen, hydroxyl, or C1-4-alkoxy, C1-5-cycloalkyl or 5-membered heterocyclic ring optionally substituted with one or more R1B; each R1B is independently C1-4-alkyl, halogen or hydroxy; n is 0, 1 or 2;
each R2 is independently F or OR2A, wherein each R2A is independently hydrogen, C1-4-alkyl or acyl;
each R3 is independently halogen, hydroxy, or C1-10-alkyl or C1-10-alkoxy optionally substituted with one or more R3A;
each R3A is independently amino, ester, amide, thiol, carboxylic acid, cyano, halogen, hydroxyl, or C1-4-alkoxy, C1-5-cycloalkyl or 5-membered heterocyclic ring optionally substituted with one or more R3B; each R3B is independently C1-4-alkyl, amino, cyano, halogen or hydroxyl; p is 0, 1 or 2;
each R4 is independently R4A, —N(R4A)(R4B), —OR4A, —SR4A, —S(O)R4A or —S(O)2R4A;
R4A is C4-20-alkyl or 4-20 membered heteroalkyl optionally substituted with one or more R4C and optionally attached to another R4A to provide a dimer or trimer; R4B is hydrogen or R4A; each R4C is independently amino, aminoacyl, azo, carbonyl, carboxyl, cyano, formyl, guanidino, halogen, hydroxyl, iminoacyl, imino, isothiocyanate, nitrile, nitro, nitroso, nitroxyl, oxy, alkylthio, sulfinyl, sulfonyl, thioaldehyde, thiocyanate, thioketone, thiourea, urea or X1, X1-L1-X2 or X1-L1-X2-L2-X3, wherein each of X1, X2 and X3 is independently C1-4-alkyl, C1-6-cycloalkyl, 5- or 6-membered heterocyclic or aryl optionally substituted with one or more R4D, and each of L1 and L2 is independently C1-6-alkyl or 1-10 membered heteroalkyl optionally substituted with one or more R4E; each R4D is independently R4E, or C1-6-alkyl optionally substituted with one or more R4E; each R4E is independently amino, aminoacyl, azo, carbonyl, carboxyl, cyano, formyl, guanidino, halogen, hydroxyl, iminoacyl, imino, isothiocyanate, nitrile, nitro, nitroso, nitroxyl, oxo, alkylthio, sulfinyl, sulfonyl, thioaldehyde, thiocyanate, thioketone or urea; and m is 1, 2 or 3;
or a pharmaceutically acceptable salt, dimer or trimer thereof in the manufacture of a medicament for treating cancer.
In the present disclosure, the cancer treated by the compound of formula I or a pharmaceutically acceptable salt, dimer or trimer thereof includes bladder cancer, blood cancer, bone cancer, brain cancer, breast cancer, central nervous system cancer, cervical cancer, colon cancer, endometrial cancer, esophageal cancer, gallbladder cancer, gastrointestinal cancer, external genital cancer, urogenital cancer, head cancer, kidney cancer, laryngeal cancer, liver cancer, muscle tissue cancer, neck cancer, oral or nasal mucosal cancer, ovarian cancer, prostate cancer, skin cancer, spleen cancer, small bowel cancer, large bowel cancer, stomach cancer, testicular cancer and/or thyroid cancer.
In an embodiment, R1 is methyl, n=0; each R2 is —OH; p=1, R3 is Cl; m=1, and R4 is ethoxy.
In some embodiments, the compound of Formula I is Sotagliflozin with the structure as shown in Formula II.
In the present disclosure, the treatment includes inhibiting tumor cell proliferation and/or inhibiting tumor volume. In some examples, lung cancer A549 cells, liver cancer HepG2 cells, prostate cancer DU145 cells, breast cancer MCF-7 cells, esophageal cancer KYSE30 cells, gastric cancer HGC-27 cells, cholangiocarcinoma RBE cells, ovarian cancer SKOV3 cells, and cervical cancer HeLa cells were used to verify the inhibitory effect of Sotagliflozin on tumor cells, and the cell experiments showed that Sotagliflozin had a certain inhibitory effect on tumor cells, with an IC50 of 71.57 μM, 115.7 μM, 40.77 μM, 64.84 μM, 82.27 μM, 48.54 μM, 182.5 μM, 84.49 μM and 82.11 μM, respectively. In animal experiments, Sotagliflozin showed a good inhibitory effect on tumor volume, which was very significantly different from that of the solvent control group, p<0.05.
The present disclosure also provides use of a compound of formula I or a pharmaceutically acceptable salt, dimer or trimer thereof in the manufacture of a preparation for reversing the resistance to an anti-tumor drug. In some specific embodiments, the present disclosure provides use of Sotagliflozin in the manufacture of a preparation for reversing the resistance to an anti-tumor drug.
The present disclosure also provides a method for reversing the resistance to an anti-tumor drug, comprising administering a compound of formula I or a pharmaceutically acceptable salt, dimer or trimer thereof. In some specific embodiments, the present disclosure also provides a method for reversing the resistance to an anti-tumor drug, comprising administering Sotagliflozin.
In the present disclosure, the compound of formula I or a pharmaceutically acceptable salt, dimer or trimer thereof is capable of reversing the resistance to an anti-tumor drug, and the anti-tumor drug is a tyrosine kinase activity inhibitor.
In the present disclosure, the tyrosine kinase activity inhibitor includes: EGFR inhibitor, c-Kit, c-Met, c-Ret, Raf, PDGFR, BTK, PKA/C, FGFR inhibitor or VEGFR inhibitor.
In some embodiments, the EGFR inhibitor includes: Gefitinib, Erlotinib, Afatinib, Lapatinib ditosylate, Genistein, Lapatinib, Saputinib, Daphnetin, DacOlmutinib, Varlitinib, Icotinib, Lidocaine hydrochloride, Osimertinib mesylate, Osimertinib, Poziotinib, Nazartinib, AZD3759, Olmutinib, Avitinib, Neratinib, Lazertinib;
The c-Met inhibitor includes: Cabozantinib;
The PKA/C inhibitor includes: Daphnetin;
The BTK inhibitor includes: Olmutinib;
The c-Ret inhibitor includes: Regorafenib monohydrate and Regorafenib;
The Raf inhibitor includes: Regorafenib monohydrate;
The FGFR inhibitor includes: 4-[(1E)-2-[5-[(1R)-1-(3,5-dichloro-4-pyridyl)ethoxy]-1H-indazol-3-yl]vinyl]-1H-pyrazole-1-ethanol(LY2874455); Nintedanib, Nintedanib Ethanesulfonate, Ponatinib, Brivanib, Brivanib Alaninate;
The c-Kit inhibitor includes: Axitinib, Pazopanib, Pazopanib HCl, Regorafenib Monohydrate, Sunitinib Malate, Sunitinib, Sitravatinib, Telatinib;
The PDGFR inhibitor includes: Axitinib, Tivozanib, Telatinib, Nintedanib, Nintedanib Ethanesulfonate Salt, Pazopanib, Pazopanib HCl, Ponatinib;
The VEGFR inhibitors include: Apatinib, Axitinib, Nintedanib, Cediranib, Pazopanib HCl, Sunitinib Malate, Brivanib, Cabozantinib, Brivanib Alaninate, Lenvatinib, Regorafenib, ENMD-2076, ENMD-2076 L-(+)-Tartaric acid, Tivozanib, Ponatinib, Fruquintinib, Telatinib, Taxifolin, Pazopanib, Cabozantinib malate, Vitamin E, Regorafenib Monohydrate, Nintedanib Ethanesulfonate Salt, Lenvatinib Mesylate, Cediranib Maleate, LY2874455, Sunitinib, Sitravatinib, Anlotinib, Sorafenib, Vandetanib and Bevacizumab and other monoclonal antibodies targeting VEGFR.
In the present disclosure, the anti-tumor drugs used to verify the efficacy of Sotagliflozin for reversing the resistance to an anti-tumor drug include at least one of ENMD-2076, Tivozanib, Genistein, Ponatinib, Daphnetin, DacOlmutinib, Varlitinib, Icotinib, Osimertinib mesylate, Osimertinib, Nazartinib, AZD3759, Anlotinib, Avitinib, or Lazertinib, Lidocaine hydrochloride, Y2874455, Axitinib, Nintedanib, Cediranib, Pazopanib HCl, Sunitinib Malate, Brivanib, Cabozantinib, Brivanib Alaninate, Lenvatinib, Regorafenib, ENMD-2076 L-(+)-Tartaric acid, Telatinib, Pazopanib, Cabozantinib malate, Regorafenib Monohydrate, Nintedanib Ethanesulfonate Salt, Lenvatinib Mesylate, Cediranib Maleate, Fruquintinib, Sunitinib, Olmutinib, Sitravatinib, Vandetanib, Gefitinib, Afatinib, Apatinib, Erlotinib, or Sorafenib, Taxifolin or Vitamin E.
In an example of the present disclosure, a cell line resistant to 60 μM Gefitinib was first constructed, and then a combination of 30 μM Gefitinib and Sotagliflozin was added to the Gefitinib resistant cell line obtained in the present disclosure. The cell line was effectively killed, it means that the combination of Sotagliflozin and Gefitinib reversed the resistance of tumor cells to Gefitinib.
The present disclosure also provides a medicament for treating cancer, comprising a compound of formula I or a pharmaceutically acceptable salt, dimer or trimer thereof, as well as pharmaceutically acceptable excipients.
The medicament of the present disclosure also comprises other drugs with anti-tumor effects, for example, tyrosine kinase activity inhibitors.
The medicament is administered orally, and its dosage forms include granules, pills, powders, tablets, capsules, oral solutions or syrups.
In some embodiments of the present disclosure, the capsule is a hard capsule or a soft capsule.
In some embodiments of the present disclosure, the tablet is an oral tablet or a buccal tablet.
Tablets refer to tablets for oral administration, and the active ingredients in most of such tablets are absorbed through the gastrointestinal tract to exert their effects, and active ingredients in some tablets act locally in the gastrointestinal tract. In some embodiments of the present disclosure, the tablets are ordinary compressed tablets, dispersible tablets, effervescent tablets, chewable tablets, coated tablets or sustained and controlled release tablets.
The medicament also comprises pharmaceutically acceptable auxiliary materials, including one of fruit powder, edible essence, sweetener, sour agent, filler, lubricant, preservative, suspending agent, food coloring, diluent, emulsifier, disintegrant and plasticizer, or a mixture thereof.
The present disclosure also provides a method for treating cancer, comprising administering the medicament of the present disclosure.
The present disclosure provides use of a compound of formula I or a pharmaceutically acceptable salt, dimer or trimer thereof in the manufacture of a medicament for treating cancer.
By testing the inhibitory effect on a variety of tumor cells, the results show that the compound of formula I has a certain inhibitory effect on tumor cells, with an IC50 of 40.77 μM-182.5 μM. In animal experiments using tumor-bearing mouse models produced from liver cancer cells and lung cancer cells, the compound of formula I showed a good inhibitory effect of tumor volume, which is very significantly different from that of the solvent control group, p<0.05.
The present disclosure provides use Sotagliflozin in the manufacture of a medicament for treating cancer. Those skilled in the art can learn from the content of the present disclosure and appropriately improve the process parameters. It should be particularly pointed out that all similar replacements and modifications are obvious to those skilled in the art, and are all deemed to be included in the present disclosure. The method and application of the present disclosure have been described through the preferred examples. Those skilled in the art can make changes or appropriate modifications and combinations to the methods and applications described herein without departing from the content, spirit and scope of the present disclosure, to implement and apply the technology of the present disclosure.
Unless specifically stated otherwise in the present disclosure, all technical and scientific terms involved in the present disclosure have the same meanings as commonly understood by those in the art. The technology used in the present disclosure is intended to refer to the technology generally understood in the art, including changes or equivalent replacements of the technology obvious to those skilled in the art. Although it is believed that the following terms are well understood by those skilled in the art, the following definitions are provided to better explain the present disclosure.
As used herein, the terms “including”, “comprising”, “having”, “containing” or “involving” and other variants thereof herein are inclusive or open-ended, and do not exclude other non-listed elements or method steps
Therefore, the present disclosure relates to use of a dual inhibitor Sotagliflozin of SGLT1 and SGLT2, the two most important members of the SGLT family highly expressed in cancer cells, and a composition comprising TKI in the manufacture of a medicament for treating cancer.
The term “treatment” as used herein means that after administration of the medicament of the present disclosure, the experimental animal suffering from a disease or condition shows partial or full relief of the symptoms, or the symptoms do not continue to worsen after treatment. Therefore, treatment includes cure.
As used herein, “therapeutic effect” refers to the effect caused by the treatment, which is manifested as cell growth inhibition rate or cell death rate at the cellular level, and changes, generally reduction or improvement of symptoms of a disease or condition, or cure of the disease or condition at the animal level. In the present disclosure, a medicament is effective if the tumor growth inhibition rate is greater than 60%, and the p-value of the statistical difference of the tumor volume or weight between the treatment group and the control group is less than 0.05.
As used herein, “cell growth inhibition rate” refers to the ratio of the average value of the absorbance of the cells stained with MTT in the treatment group to the average value of the absorbance in the control group after drug treatment. “Tumor growth inhibition rate” represents the ratio of the average tumor volume or weight of the treatment group after drug treatment to the average volume or weight of the control group.
In an embodiment, the Sotagliflozin is used to treat cancer in a subject.
The term “cancer” as used herein refers to the malignant proliferation of epithelial cells due to changes in genetic material. The cancers include: bladder cancer, blood cancer, bone cancer, brain cancer, breast cancer, central nervous system cancer, cervical cancer, colon cancer, endometrial cancer, esophageal cancer, gallbladder cancer, gastrointestinal cancer, external genital cancer, urogenital cancer, head cancer, kidney cancer, laryngeal cancer, liver cancer, muscle tissue cancer, neck cancer, oral or nasal mucosal cancer, ovarian cancer, prostate cancer, skin cancer, spleen cancer, small bowel cancer, large bowel cancer, stomach cancer, testicular cancer and/or thyroid cancer.
The test materials used in the present disclosure are all common commercially available products, and all are available in the market.
In the examples of this application, the drugs involved and their Chinese names are shown in Table 1:
The present disclosure will be now further explained with respect to the examples:
Prostate cancer DU145 cells, breast cancer MCF-7 cells, esophageal cancer KYSE30 cells, gastric cancer HGC-27 cells, cholangiocarcinoma RBE cells, ovarian cancer SKOV3 cells, and cervical cancer Hela cells were used to verify the inhibitory effect of Sotagliflozin on tumor cells. After growing to 80% density, the cells were trypsinized, passaged and plated in a 96-well plate with 5000 cells per well. After 24 hours, the medium was replaced with a medium containing the corresponding concentration of drug. After 48 hours, the absorbance at each concentration was detected by the MTT method.
The experiment included the following groups:
Control group: cells were cultured in normal culture medium without drug added.
Sotagliflozin test group: cells were treated by adding Sotagliflozin at different concentration to each culture medium.
After incubation, the cell growth inhibition rate was calculated by dividing the absorbance value at each concentration by the absorbance value of the control group. The calculated IC50 values of Sotagliflozin on various tumor cells are shown in
Sotagliflozin was purchased from Selleck Chemicals for growth inhibition test of cancer cell in vitro. Initially, test using normal human umbilical cord epithelial cells showed that Sotagliflozin produced great cytotoxicity at a concentration higher than 80 μM, and mainly exhibited cell growth inhibition effect at a concentration lower than 8 μM. Therefore, the concentrations of Sotagliflozin used in the subsequent compositions of this experiment were all lower than 80 μM to avoid affecting normal cells.
According to the tissue distribution characteristics of EGFR and SGLT1/2, the targets of Gefitinib and Sotagliflozin, the followings cells were selected for experimental verification: lung cancer cell line A549; colorectal cancer cell line LoVo, HT29, SW620, HCT116; cervical cancer HeLa; ovarian cancer SKOV3; gastric cancer HGC27; cholangiocarcinoma RBE; esophageal cancer KYSE30, and the like. After growing to 80% density, the cells were trypsinized, passaged and plated in a 96-well plate with 5000 cells per well. After 24 hours, the medium was replaced with a medium containing the corresponding concentration of drug. After 48 hours, the absorbance at each concentration was detected by the MTT method.
The experiment included the following groups:
Control group: cells were cultured in normal culture medium without drug added.
Gefitinib test group: cells were treated by adding Gefitinib alone at 4 different concentration, 5 μM, 10 μM, 20 μM, 30 μM, respectively, to the culture medium.
Gefitinib+Sotagliflozin combination test group: cells were treated by adding both Sotagliflozin (20 μM) and Gefitinib at 4 different concentration, 5 μM, 10 μM, 20 μM and 30 μM, respectively, to the culture medium.
After incubation, the cell growth inhibition rate was calculated by dividing the absorbance value at each concentration by the absorbance value of the control group. The results are shown in
Lung cancer cell line A549 was used as an example to verify the IC50 value of the Gefitinib+Sotagliflozin combination. The experiment included the following groups:
Gefitinib test group (
Sotagliflozin test group (
Gefitinib+Sotagliflozin combination test group 1 (
Gefitinib+Sotagliflozin combination test group 2 (
Gefitinib+Sotagliflozin combination test group 3 (
The results showed that with the combination of Sotagliflozin and Gefitinib, the inhibitory effect of Gefitinib on A549 cells was significantly enhanced, and the IC50 was reduced to less than half of that of the single agent. Therefore, the effect of the combination in the safe concentration range of Sotagliflozin is better than the effect of each single agent. The verification results of other cell lines are shown in the figures (2f-2j). It is worth mentioning that the ability of Sotagliflozin in the combination to enhance the efficacy of EGFR-targeting TKI drugs is not limited to a single drug of Gefitinib. In
After knowing that the combination of Gefitinib and Sotagliflozin significantly enhanced the effectiveness of Gefitinib from example 1, the present disclosure continues to explore whether the combination of the two drugs can reverse the resistance of tumor cells to Gefitinib. Gefitinib-resistant cells can be obtained by long-term culturing of A549 cells with a medium containing Gefitinib at increasing concentrations. After 5 months of screening, the present disclosure obtained A549 gefitinib-resistant cell line that can survive in 60 μM gefitinib for a long time.
2. Sotagliflozin Combined with Gefitinib Reverses the Resistance of Tumor Cells to Gefitinib
The Gefitinib-resistant cell line obtained by the present disclosure can be effectively killed by adding 30 μM Gefitinib and Sotagliflozin composition. It shows that the combination of Sotagliflozin and Gefitinib reverses the resistance of tumor cells to Gefitinib. The results are shown in
After obtaining the effectiveness of Gefitinib in Example 1, the present disclosure further validated another VEGFR-targeting TKI drug, Apatinib. According to the tissue distribution characteristics of VEGFR and SGLT1/2, the targets of Apatinib and Sotagliflozin, the followings cells were selected for experimental verification: liver cancer cell line HepG2; colorectal cancer cell line LoVo, HT29, SW620, SW480; cervical cancer HeLa; ovarian cancer SKOV3; gastric cancer HGC27; cholangiocarcinoma RBE; esophageal cancer KYSE3, and the like. After growing to 80% density, the cells were trypsinized, passaged and plated in a 96-well plate with 5000 cells per well. After 24 hours, the medium was replaced with a medium containing the corresponding concentration of Apatinib, Sotagliflozin, or the combination of Apatinib and Sotagliflozin. After 48 hours, the absorbance at each concentration was detected by the MTT method.
The experiment included the following groups:
Control group: cells were cultured in normal culture medium without drug added.
Apatinib test group: cells were treated by adding Apatinib alone at 4 different concentrations, 5 μM, 10 μM, 20 μM, 30 μM, respectively, to the culture medium.
Apatinib+Sotagliflozin combination test group: cells were treated by adding both Sotagliflozin (20 μM) and Apatinib at 4 different concentrations, 5μM, 10 μM, 20 μM and 30 μM, respectively, to the culture medium.
The cell growth inhibition rate was calculated by dividing the absorbance value at each concentration by the absorbance value of the control group. The results are shown in
2.1. Liver Cancer Cell Line HepG2 was Used as an Example to Verify the IC50 Value of the Apatinib+Sotagliflozin Combination. The Experiment Included the Following Groups:
Apatinib test group (
Sotagliflozin test group (
Apatinib+Sotagliflozin combination test group 1 (
Apatinib+Sotagliflozin combination test group 2 (
Apatinib+Sotagliflozin combination test group 3 (
Apatinib+Sotagliflozin combination test group 4 (
These results showed that with the combination of Sotagliflozin and Apatinib, the inhibitory effect of Apatinib on HepG2 cells was significantly enhanced, and the IC50 was reduced to less than one-fourth of that of the single agent. Therefore, the effect of the combination in the safe concentration range of Sotagliflozin is better than the effect of each single agent. The verification results of other cell lines are shown in the FIGS. (4c-4g). It is worth mentioning that the ability of Sotagliflozin in the combination to enhance the efficacy of VEGFR-targeting TKI drugs is not limited to a single drug of Apatinib. In
Other TKI drugs were further verified, proving that the TKI drugs which can be combined with Sotagliflozin are not limited to specific one or several drugs.
The selected drugs included: Axitinib (
The present disclosure preferentially selected liver cancer cell line HepG2 for experimental verification. After growing to 80% density, the cells were trypsinized, passaged and plated in a 96-well plate with 5000 cells per well. After 24 hours, the medium was replaced with a medium containing the corresponding concentration of Apatinib, Sotagliflozin, or the combination of Apatinib and Sotagliflozin. After 48 hours, the absorbance at each concentration was detected by the MTT method.
The experimental method was the same as before, and the incubation time was 1 h. The experiment included a blank control group, namely normal cultured HepG2 cells, in which the concentrations of Sotagliflozin or TKI drugs were both 0, and the survival rate of the blank control group cells was set to 100%. In other groups, the concentration of Sotagliflozin used was mol/L, and the concentrations of TKI drugs are shown in Table 2. The results are shown in the attached Figures:
The results showed that each combination administration group showed a significantly better inhibitory effect on tumor cells than the single agent control group.
Examples 1 to 4 are all tests at the cell level. In order to further verify the anti-tumor effect in vivo of the diabetes treatment drug Sotagliflozin discovered in the present disclosure and the combination thereof with TKI inhibitor drugs, lung cancer A549 cells and the Ba1bc nude mice from Charles River Laboratories were used in tumor treatment experiments. After growing to the logarithmic phase, A549 cells were collected and resuspended in serum-free DMEM medium to 5×107 cells per ml. Each mouse was inoculated with 100 μl of 5×106 cells, and the tumor size was measured 19 days later. Mice were grouped according to the tumor size, and the average tumor size in each group was the same. Mice were administered after grouping.
According to the current recommended daily dose 200-400 mg of Sotagliflozin for diabetic patients, corresponding to 22 mg to 44 mg per kilogram of body weight for mice, we finally chose a dose of 30 mg/kg of Sotagliflozin for oral administration in mice. The dose of Gefitinib was 100 mg per kilogram according to the reported dose for the treatment of A549 xenograft tumor in previous studies. The two drugs were administered by gavage, consistent with the current oral mode in clinical use. The dosing cycle was once every two days. The tumor size was measured every two days. After 40 days of administration, the test was ended, and the tumor was removed and weighed.
As shown in
The above are only the preferred embodiments of the present disclosure. It should be pointed out that for those of skilled in the art, various improvements and modifications can be made without departing from the principle of the present disclosure, and these improvements and modifications should also be considered within the scope of the present disclosure.
Number | Date | Country | Kind |
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202010643578.4 | Jul 2020 | CN | national |
Filing Document | Filing Date | Country | Kind |
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PCT/CN2020/109966 | 8/19/2020 | WO |