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首页> 外文期刊>Assay and drug development technologies >A fluorescence-based assay for monoacylglycerol lipase compatible with inhibitor screening.
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A fluorescence-based assay for monoacylglycerol lipase compatible with inhibitor screening.

机译:基于荧光的单酰基甘油脂肪酶检测方法,可与抑制剂筛选兼容。

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摘要

A novel fluorescence-based assay of monoacylglycerol lipase (MAGL) activity that is simple, sensitive, and amenable to the screening of small molecule inhibitors is described. Purified recombinant human MAGL protein and 7-hydroxycoumarinyl-arachidonate (7-HCA), a fluorogenic substrate for MAGL, were employed in the assay. MAGL protein catalyzes the hydrolysis of 7-HCA to generate arachidonic acid and the highly fluorescent 7-hydroxyl coumarin (7-HC). Release of 7-HC was measured using a fluorometer. MAGL protein catalyzed the hydrolysis of 7-HCA with an apparent K(m) of 9.8 microM and V(max) of 1.7 mmol/min/mg of protein. The assay is specific for MAGL as assay buffer alone or heat-denatured MAGL protein had no significant activity against 7-HCA. Furthermore, MAGL activity was inhibited in a dose-dependent manner by the specific inhibitor URB602 as well as N-arachidonyl maleimide with 50% inhibitory concentration values of 3.1 microM and 155 nM, respectively. The assay was further optimized under different conditions, including pH range and bovine serum albumin protein and dimethyl sulfoxide concentrations. The assay was found to be reproducible, having Z' values ranging from 0.7 to 0.9, and is therefore suitable for high-throughput screening.
机译:描述了一种新颖的基于荧光的单酰基甘油脂肪酶(MAGL)活性测定方法,该方法简单,灵敏并且适合小分子抑制剂的筛选。测定中使用了纯化的重组人MAGL蛋白和MAGL的荧光底物7-羟基香豆基-花生四烯酸酯(7-HCA)。 MAGL蛋白催化7-HCA水解,生成花生四烯酸和高荧光7-羟基香豆素(7-HC)。使用荧光计测量7-HC的释放。 MAGL蛋白质催化7-HCA的水解,表观K(m)为9.8 microM,V(max)为1.7 mmol / min / mg蛋白质。该测定法对MAGL具有特异性,因为单独的测定缓冲液或热变性的MAGL蛋白对7-HCA均无明显活性。此外,特异性抑制剂URB602以及50%抑制浓度分别为3.1 microM和155 nM的N-花生四烯酸马来酰亚胺以剂量依赖的方式抑制了MAGL的活性。在不同条件下进一步优化了测定,包括pH范围,牛血清白蛋白和二甲基亚砜浓度。发现该测定法是可重复的,其Z'值在0.7至0.9之间,因此适用于高通量筛选。

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