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Comparative Studies of Thiol-Sensitive Fluorogenic Probes for HAT Assays

机译:抗帽子测定硫醇敏感荧光探针的比较研究

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摘要

Histone acetyltransferases (HATs) catalyze the acetylation of specific lysine residues in histone and nonhistone proteins. Recent studies showed that acetylation is widely distributed among cellular proteins, suggestive of diverse functions of HATs in cellular pathways. Nevertheless, currently available assays for HAT activity study are still quite limited. Here we evaluated a series of thiol-sensitive fluorogenic compounds for the detection of the enzymatic activities of different HAT proteins. Upon conjugation to the thiol group of HSCoA, these molecules gain enhanced quantum yields and strong fluorescence, permitting facile quantitation of HAT activities. We investigated and compared the assay performances of these fluorogenic compounds for their capability as HAT activity reporters, including kinetics of reaction with HSCoA, influence on HAT activity, and fluorescence amplification factors. Our data suggest that CPM and CME are excellent HAT probes owing to their fast reaction kinetics and dramatic fluorescence enhancement during the HAT reaction. Further, the microtiter plate measurements show that this fluorescent approach is robust and well suited for adaption to high throughput screening of small molecule inhibitors of HATs, highlighting the value of this assay strategy in new drug discovery.
机译:组蛋白乙酰基转移酶(HATs)催化组蛋白和非组蛋白蛋白中特定赖氨酸残基的乙酰化。最近的研究表明,乙酰化作用广泛分布于细胞蛋白之间,提示HAT在细胞途径中具有多种功能。尽管如此,目前用于HAT活性研究的检测方法仍然十分有限。在这里,我们评估了一系列对硫醇敏感的荧光化合物,用于检测不同HAT蛋白的酶促活性。与HSCoA的巯基结合后,这些分子获得增强的量子产率和强荧光,从而可以轻松地定量测定HAT活性。我们调查并比较了这些荧光化合物作为HAT活性报告基因的能力,包括与HSCoA的反应动力学,对HAT活性的影响以及荧光放大因子的测定性能。我们的数据表明,由于CPM和CME在HAT反应过程中具有快速的反应动力学和显着的荧光增强作用,因此它们是出色的HAT探针。此外,微量滴定板测量结果表明,这种荧光方法坚固耐用,非常适合用于HATs小分子抑制剂的高通量筛选,从而突出了该测定策略在新药开发中的价值。

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