Zielinska Agnieszka, Lichti Cheryl F, Bratton Stacie, Mitchell Neil C, Gallus-Zawada Anna, Le Vi-Huyen, Finel Moshe, Miller Grover P, Radominska-Pandya Anna, Moran Jeffery H
Arkansas Public Health Laboratory, Arkansas Department of Health, 201 South Monroe Street, Little Rock, AR 72205, USA.
J Pharmacol Exp Ther. 2008 Jan;324(1):139-48. doi: 10.1124/jpet.107.129858. Epub 2007 Oct 5.
Our understanding of human phase II metabolic pathways which facilitate detoxification and excretion of warfarin (Coumadin) is limited. The goal of this study was to test the hypothesis that there are specific human hepatic and extrahepatic UDP-glucuronosyltransferase (UGT) isozymes, which are responsible for conjugating warfarin and hydroxylated metabolites of warfarin. Glucuronidation activity of human liver microsomes (HLMs) and eight human recombinant UGTs toward (R)- and (S)-warfarin, racemic warfarin, and major cytochrome P450 metabolites of warfarin (4'-, 6-, 7-, 8-, and 10-hydroxywarfarin) has been assessed. HLMs, UGT1A1, 1A8, 1A9, and 1A10 showed glucuronidation activity toward 4'-, 6-, 7-, and/or 8-hydroxywarfarin with K(m) values ranging from 59 to 480 microM and V(max) values ranging from 0.03 to 0.78 microM/min/mg protein. Tandem mass spectrometry studies and structure comparisons suggested glucuronidation was occurring at the C4'-, C6-, C7-, and C8-positions. Of the hepatic UGT isozymes tested, UGT1A9 exclusively metabolized 8-hydroxywarfarin, whereas UGT1A1 metabolized 6-, 7-, and 8-hydroxywarfarin. Studies with extrahepatic UGT isoforms showed that UGT1A8 metabolized 7- and 8-hydroxywarfarin and that UGT1A10 glucuronidated 4'-, 6-, 7-, and 8-hydroxywarfarin. UGT1A4, 1A6, 1A7, and 2B7 did not have activity with any substrate, and none of the UGT isozymes evaluated catalyzed reactions with (R)- and (S)-warfarin, racemic warfarin, or 10-hydroxywarfarin. This is the first study identifying and characterizing specific human UGT isozymes, which glucuronidate major cytochrome P450 metabolites of warfarin with similar metabolic rates known to be associated with warfarin metabolism. Continued characterization of these pathways may enhance our ability to reduce life-threatening and costly complications associated with warfarin therapy.
我们对促进华法林(香豆素)解毒和排泄的人类Ⅱ相代谢途径的了解有限。本研究的目的是检验以下假设:存在特定的人类肝脏和肝外尿苷二磷酸葡萄糖醛酸基转移酶(UGT)同工酶,它们负责使华法林及其羟基化代谢产物结合。已评估了人肝微粒体(HLM)和8种人类重组UGT对(R)-和(S)-华法林、消旋华法林以及华法林的主要细胞色素P450代谢产物(4'-、6-、7-、8-和10-羟基华法林)的葡萄糖醛酸化活性。HLM、UGT1A1、1A8、1A9和1A10对4'-、6-、7-和/或8-羟基华法林表现出葡萄糖醛酸化活性,K(m)值范围为59至480微摩尔,V(max)值范围为0.03至0.78微摩尔/分钟/毫克蛋白质。串联质谱研究和结构比较表明葡萄糖醛酸化发生在C4'-、C6-、C7-和C8-位。在所测试的肝脏UGT同工酶中,UGT1A9专门代谢8-羟基华法林,而UGT1A1代谢6-、7-和8-羟基华法林。对肝外UGT同工型的研究表明,UGT1A8代谢7-和8-羟基华法林,UGT1A10使4'-、6-、7-和8-羟基华法林葡萄糖醛酸化。UGT1A4、1A6、1A7和2B7对任何底物均无活性,所评估的UGT同工酶均未催化与(R)-和(S)-华法林、消旋华法林或