Yasgar Adam, Shultz John, Zhou Wenhui, Wang Hui, Huang Fen, Murphy Nancy, Abel Erika L, DiGiovanni John, Inglese James, Simeonov Anton
NIH Chemical Genomics Center, National Human Genome Research Institute, National Institutes of Health, Bethesda, Maryland 20892-3370, USA.
Assay Drug Dev Technol. 2010 Apr;8(2):200-11. doi: 10.1089/adt.2009.0248.
Glutathione S-transferases (GSTs) constitute a family of detoxification enzymes that catalyze the conjugation of glutathione with a variety of hydrophobic compounds, including drugs and their metabolites, to yield water-soluble derivatives that are excreted in urine or bile. Profiling the effect of small molecules on GST activity is an important component in the characterization of drug candidates and compound libraries. Additionally, specific GST isozymes have been implicated in drug resistance, especially in cancer, and thus represent potential targets for intervention. To date, there are no sensitive miniaturized high-throughput assays available for GST activity detection. A series of GST substrates containing a masked luciferin moiety have been described recently, offering the potential for configuring a sensitive screening assay via coupled luciferase reaction and standard luminescence detection. We report on the optimization and miniaturization of this homogeneous method to 1,536-well format using GSTs from 3 different species: mouse isozyme A4-4, human isozymes A1-1, M1-1, and P1-1, and the major GST from the parasitic worm Schistosoma japonicum.
谷胱甘肽S-转移酶(GSTs)是一类解毒酶,可催化谷胱甘肽与多种疏水性化合物(包括药物及其代谢产物)结合,生成水溶性衍生物,这些衍生物通过尿液或胆汁排出体外。分析小分子对GST活性的影响是药物候选物和化合物库表征的重要组成部分。此外,特定的GST同工酶与耐药性有关,尤其是在癌症中,因此是潜在的干预靶点。迄今为止,尚无用于检测GST活性的灵敏小型化高通量检测方法。最近描述了一系列含有被掩盖的荧光素部分的GST底物,为通过偶联荧光素酶反应和标准发光检测构建灵敏的筛选检测提供了可能。我们报告了使用来自3种不同物种的GSTs将这种均相方法优化并小型化为1536孔板形式的过程,这3种GSTs分别是小鼠同工酶A4-4、人同工酶A1-1、M1-1和P1-1,以及日本血吸虫的主要GST。
