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Measuring Drug Metabolism Kinetics and Drug-Drug Interactions Using Self-Assembled Monolayers for Matrix-Assisted Laser Desorption-Ionization Mass Spectrometry

机译:使用自组装单层基质辅助激光解吸电离质谱法测量药物代谢动力学和药物相互作用

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The competition of two drugs for the same metabolizing enzyme is a common mechanism for drug-drug interactions that can lead to altered kinetics in drug metabolism and altered elimination rates in vivo. With the prevalence of multidrug therapy, there is great potential for serious drug drug interactions and adverse drug reactions. In an effort to prevent adverse drug reactions, the FDA mandates the evaluation of the potential for metabolic inhibition by every new chemical entity. Conventional methods for assaying drug metabolism (e.g., those based on HPLC) have been established for measuring drug-drug interactions; however, they are low-throughput. Here we describe an approach to measure the catalytic activity of CYP2C9 using the high-throughput technique self-assembled monolayers for matrix-assisted laser desorption-ionization (SAMDI) mass spectrometry. We measured the kinetics of CYP450 metabolism of the substrate, screened a set of drugs for inhibition of CYP2C9 and determined the I values for inhibitors. The throughput of this platform may enable drug metabolism and drug-drug interactions to be interrogated at a scale that cannot be achieved with current methods.
机译:两种药物对同一代谢酶的竞争是药物-药物相互作用的共同机制,可导致药物代谢动力学改变和体内消除速率改变。随着多药疗法的普及,存在严重的药物相互作用和不良药物反应的巨大潜力。为了防止药物不良反应,FDA要求对每种新化学实体对代谢抑制的潜力进行评估。已经建立了用于测定药物代谢的常规方法(例如,基于HPLC的方法)以测量药物-药物相互作用。但是,它们的吞吐量低。在这里,我们描述了一种用于基质辅助激光解吸电离(SAMDI)质谱的高通量技术自组装单分子膜来测量CYP2C9催化活性的方法。我们测量了底物CYP450代谢的动力学,筛选了一组可抑制CYP2C9的药物,并确定了抑制剂的I值。该平台的通量可以使药物代谢和药物-药物相互作用以目前方法无法实现的规模进行询问。

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