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Development of a high throughput cell-based assay for soluble epoxide hydrolase using bacmam technology

机译:使用bacmam技术开发基于细胞的高通量可溶性环氧化物水解酶测定方法

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Epoxyeicosatrienoic acids (EETs) play important protective functions in cardiovascular and renal systems. Under physiological conditions, EETs are quickly converted by the soluble epoxide hydrolase (sEH) to diols which do not have the beneficiary roles. Inhibition of sEH with small molecules to increase the concentration of EETs therefore provides an attractive therapeutic strategy for cardiovascular diseases. We describe here the development of a high throughput cell-based assay to measure sEH activity and screen small molecular compounds as sEH inhibitors. This assay is based on the technology of fluorescence polarization (FP), utilizing a Cy3B labeled 14,15-DHET ligand and a rabbit anti-14,15-DHET antibody. With the optimized assay, we measured the cellular sEH activity of several cell lines expressing endogenous sEH as well as sEH BacMam transduced HEK-293 cells. The inhibitory effect of several known sEH inhibitors was evaluated in sEH BacMam transduced HEK-293 cells. Our data show that there is good agreement of pIC_(50) values obtained between the FP format and a commercially available ELISA kit. To our knowledge, this is the first report of a high throughput cell-based assay for screening sEH inhibitors.
机译:环氧二十碳三烯酸(EET)在心血管和肾脏系统中起重要的保护作用。在生理条件下,EET通过可溶性环氧化物水解酶(sEH)迅速转化为不具有受益作用的二醇。因此,用小分子抑制sEH以增加EET的浓度为心血管疾病提供了一种有吸引力的治疗策略。我们在这里描述了一种基于高通量细胞的测定方法的开发,以测定sEH活性并筛选作为sEH抑制剂的小分子化合物。此测定法基于荧光偏振(FP)技术,利用Cy3B标记的14,15-DHET配体和兔抗14,15-DHET抗体。通过优化的测定,我们测量了表达内源性sEH以及sEH BacMam转导的HEK-293细胞的几种细胞系的细胞sEH活性。在sEH BacMam转导的HEK-293细胞中评估了几种已知的sEH抑制剂的抑制作用。我们的数据表明,FP格式与市售ELISA试剂盒之间的pIC_(50)值具有很好的一致性。据我们所知,这是用于筛选sEH抑制剂的基于细胞的高通量检测的首次报道。

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