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A high-throughput, low-volume enzyme assay on solid support

机译:固体支持物上的高通量,小体积酶分析

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A high-throughput enzyme assay is described that uses 1 muL or less of enzyme solution for each test. Enzyme solutions are deposited by robotic handling in a throughput of over 1000 tests/h on the surface of silica gel plates that have been preimpregnated with fluorogenic substrates. The reaction is quantitated by fluorescence. The method is compatible with water-insoluble substrates (lipases), water-soluble substrates (glycosidases), whole-protein substrates (proteases), and enzyme inhibition measurements. Hydrolytically labile umbelliferyl esters can be used to assay lipases in this format without background hydrolysis. High throughput and reproducibility were tested by fingerprint analysis of lipases and esterases against 37 different fluorogenic ester substrates. A set of eight fluorogenic unbelliferyl esters was selected for optimal activity screening of lipases and esterases on silica gel plates.
机译:描述了一种高通量酶测定法,该测定法每次测试使用1μL或更少的酶溶液。酶溶液通过机器人处理以超过1000次/小时的处理量沉积在已预浸渍有荧光底物的硅胶板上。通过荧光定量反应。该方法与水不溶性底物(脂肪酶),水溶性底物(糖苷酶),全蛋白底物(蛋白酶)和酶抑制测量兼容。水解不稳定的伞形酯可用于以这种形式测定脂肪酶,而无需进行背景水解。通过针对37种不同的荧光酯底物的脂肪酶和酯酶的指纹分析,测试了高通量和重现性。选择了一组八种荧光去甲壬基酯,以最佳活性筛选硅胶板上的脂肪酶和酯酶。

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