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Fluorophoric assay for the high-throughput determination of amidase activity

机译:荧光法高通量测定酰胺酶活性

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An assay has been developed for the high-throughput identification of amidase activity. Amines released from the enzyme-catalyzed hydrolysis of corresponding amides were detected by the formation of a fluorescent dye by coupling with 4-nitro-7-chloro-benzo-2-oxa-1,3-diazole (NBD-C1). Using this format, 22 lipases and esterases were tested for their ability to hydrolyze aromatic substituted N-acylamines in a microtiter plate format. Identified active enzymes were further characterized toward a broad range of compounds to determine the influence of substrate structure on activity. For recombinantly produced esterases, it could be shown that the assay works with high reproducibility and sensitivity, even in the presence of amino acids and proteins present in culture media and cell debris. [References: 31]
机译:已经开发出用于高通量鉴定酰胺酶活性的测定法。通过与4-硝基-7-氯-苯并-2-苯并-2-恶唑-1,3-二唑(NBD-C1)偶联形成荧光染料,检测了相应酰胺的酶催化水解过程中释放的胺。使用这种格式,测试了22种脂肪酶和酯酶以微孔板的形式水解芳族取代的N-酰基胺的能力。鉴定出的活性酶针对多种化合物进行了进一步表征,以确定底物结构对活性的影响。对于重组产生的酯酶,即使在培养基和细胞碎片中存在氨基酸和蛋白质的情况下,也可以证明该测定具有很高的重现性和敏感性。 [参考:31]

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