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No effect of CYP450 and P-glycoprotein on hydroxyurea in vitro metabolism

机译:CYP450和P-糖蛋白对羟基脲体外代谢无影响

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Our objectives were (1) to study the HU metabolism via human cytochromes and (2) to test if HU is a substrate of P-gp. HU metabolism was investigated by determining the appearance of urea and HU decreasing upon incubation with human liver microsomes. Quantification was determined using HPLC coupled with UV-detection at 449 nm. Our method was linear between 5 and 1000 mum, precise (coefficients of variation ranging from 1.7 to 9.9%), accurate (97.7-103.9%). The limit of quantification was 7 mum. The ATPase activity of human P-gp membranes was determined by measuring inorganic phosphate liberation. HU and urea measurements in microsomes were not different between 0 and 60 min whatever HU concentration used from 30 to 300 mum. The presence of NADPH in the medium has no effect on HU and urea measurements. In the absence of verapamil, the ATPase activity was unaffected by HU at concentrations of 10, 30, 100 and 300 mum. HU is unlikely to cause clinically relevant drug interactions with the substrates of these enzymes/transporters. However, it will be necessary to validate these in vitro data in patients with sickle cell anemia to evaluate the impact of genetic polymorphisms of these enzymes in a black population.
机译:我们的目标是(1)研究人类细胞色素对HU的代谢作用,以及(2)测试HU是否是P-gp的底物。通过测定与人肝微粒体温育后尿素和HU的减少来研究HU代谢。使用HPLC结合449 nm处的UV检测确定定量。我们的方法在5至1000微米之间是线性的,精确的(变异系数在1.7%至9.9%之间),精确的(97.7-103.9%)。定量限为7μm。通过测量无机磷酸盐的释放来测定人P-gp膜的ATPase活性。无论使用30到300微米的HU浓度,微粒体中的HU和尿素测量值在0到60分钟之间都没有差异。培养基中NADPH的存在对HU和尿素测量没有影响。在没有维拉帕米的情况下,浓度为10、30、100和300毫米的HU不会影响ATPase的活性。 HU不太可能引起与这些酶/转运蛋白的底物在临床上相关的药物相互作用。但是,有必要在镰状细胞性贫血患者中验证这些体外数据,以评估这些酶的遗传多态性对黑人人群的影响。

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