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ChEMBL ligand: CHEMBL4107297 |
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DB | Assay description | Assay Type | Standard value | Standard parameter | Original value | Original units | Original parameter | Reference |
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Sodium/glucose cotransporter 1 in Human (target type: SINGLE PROTEIN) [ChEMBL: CHEMBL4979] [GtoPdb: 915] [UniProtKB: P13866] | ||||||||
ChEMBL | In Vitro Assay: Human SGLT-2 and SGLT-1 sequences were stably expressed in the CHO cells. The cell culture was conducted in a 96-well plate for 12 hr. The plate was washed with KRHâ¿¿Na+(Buffer A) or KRH-NMG (Buffer A−) buffering solution for three times, 2004/well. Then the plate was added with a buffering solution containing Buffer A or Buffer A− plus [14C]-AMG (10 μCi/mL), 100 μL/well. The cell culture was conducted at 37 °C. for 1 hr. Then, 100 μL of an ice pre-cooled buffering solution (Buffer D) was added to terminate the assay. The plate was washed for five times. Then an ice pre-cooled lytic buffering solution (100 mM NaOH solution) was added, 20 μL/well, and the centrifugation at 600 rpm was conducted for 5 mins. Then Microscint 40 solution was added, 80 μl/well, and the centrifugation at 600 rpm was conducted for 5 mins. Finally, the radioactivity of [14C]-AMG was detected with MicroBeta Trilux (purchased from PerkinElmer Co. Ltd.) according to the scintillation counting method, and the half-inhibition concentration IC50 was calculated. | B | 4.76 | pIC50 | 17217.33 | nM | IC50 | US-9315438-B2. Optically pure benzyl-4-chlorophenyl-C-glucoside derivative (2016) |
Sodium/glucose cotransporter 2 in Human (target type: SINGLE PROTEIN) [ChEMBL: CHEMBL3884] [GtoPdb: 916] [UniProtKB: P31639] | ||||||||
GtoPdb | Determined in CHO cells stably expressing human SGLT2 | - | 8.6 | pIC50 | 2.5 | nM | IC50 | US9315438B2. Optically pure benzyl-4-chlorophenyl-C-glucoside derivative (2016) |
ChEMBL | In Vitro Assay: Human SGLT-2 and SGLT-1 sequences were stably expressed in the CHO cells. The cell culture was conducted in a 96-well plate for 12 hr. The plate was washed with KRHâ¿¿Na+(Buffer A) or KRH-NMG (Buffer A−) buffering solution for three times, 2004/well. Then the plate was added with a buffering solution containing Buffer A or Buffer A− plus [14C]-AMG (10 μCi/mL), 100 μL/well. The cell culture was conducted at 37 °C. for 1 hr. Then, 100 μL of an ice pre-cooled buffering solution (Buffer D) was added to terminate the assay. The plate was washed for five times. Then an ice pre-cooled lytic buffering solution (100 mM NaOH solution) was added, 20 μL/well, and the centrifugation at 600 rpm was conducted for 5 mins. Then Microscint 40 solution was added, 80 μl/well, and the centrifugation at 600 rpm was conducted for 5 mins. Finally, the radioactivity of [14C]-AMG was detected with MicroBeta Trilux (purchased from PerkinElmer Co. Ltd.) according to the scintillation counting method, and the half-inhibition concentration IC50 was calculated. | B | 8.6 | pIC50 | 2.5 | nM | IC50 | US-9315438-B2. Optically pure benzyl-4-chlorophenyl-C-glucoside derivative (2016) |
ChEMBL data shown on this page come from version 35:
Zdrazil B, Felix E, Hunter F, Manners EJ, Blackshaw J, Corbett S, de Veij M, Ioannidis H, Lopez DM, Mosquera JF, Magarinos MP, Bosc N, Arcila R, Kizilören T, Gaulton A, Bento AP, Adasme MF, Monecke P, Landrum GA, Leach AR. (2024). The ChEMBL Database in 2023: a drug discovery platform spanning multiple bioactivity data types and time periods. Nucleic Acids Res., 52(D1). DOI: 10.1093/nar/gkad1004. [EPMCID:10767899] [PMID:37933841]
Davies M, Nowotka M, Papadatos G, Dedman N, Gaulton A, Atkinson F, Bellis L, Overington JP. (2015) 'ChEMBL web services: streamlining access to drug discovery data and utilities.' Nucleic Acids Res., 43(W1). DOI: 10.1093/nar/gkv352. [EPMCID:25883136]