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合成及一系列高萤光基化谷胱甘肽转移酶底物的特性、一般策略。

Synthesis and characterization of a series of highly fluorogenic substrates for glutathione transferases, a general strategy.

机构信息

Institute of Environmental Medicine, Division of Biochemical Toxicology, Karolinska Institutet, Stockholm, Sweden.

出版信息

J Am Chem Soc. 2011 Sep 7;133(35):14109-19. doi: 10.1021/ja205500y. Epub 2011 Aug 15.

DOI:10.1021/ja205500y
PMID:21786801
Abstract

Glutathione transferases (GSTs) are used in biotechnology applications as fusion partners for facile purification and are also overexpressed in certain tumors. Consequently, there is a need for sensitive detection of the enzymes. Here we describe a general strategy for the synthesis and characterization of novel fluorogenic substrates for GSTs. The substrates were synthesized by introducing an electrophilic sulfonamide linkage to fluorescent molecules containing an amino group [e.g., 2,4-dinitrobenzenesulfonamide (DNs) derivatives of coumarin, cresyl violet, and rhodamine]. The derivatives were essentially nonfluorescent, and upon GST catalyzed cleavage of the dinitrobenzenesulfonamide, free fluorophore is released (and 1-glutathionyl-2,4-dinitrobenzene + SO(2)). All the coumarin-, cresyl violet- and rhodamine-based fluorogenic probes turned out to be good substrates for most GSTs, especially for GSTA(1-1), in terms of strong fluorescence increases (71-1200-fold), high k(cat)/K(m) values (10(4)-10(7) M(-1) s(-1)) and significant rate enhancements (10(6)-10(9)-fold). The substrates were successfully applied to quantitate very low levels of GST activity in cell extracts and DNs-cresyl violet was also successfully applied to the imaging of microsomal MGST(1) activity in living cells. The cresyl violet stained cells retained their fluorescence after fixation, which is a very useful property. In summary, we describe a general and versatile strategy to generate fluorogenic GST substrates, some of them providing the most sensitive assays so far described for GSTs.

摘要

谷胱甘肽转移酶(GSTs)在生物技术应用中被用作融合伴侣,以便于进行简单的纯化,并且在某些肿瘤中过度表达。因此,需要对这些酶进行灵敏的检测。在这里,我们描述了一种用于 GSTs 的新型荧光底物的合成和表征的通用策略。通过向含有氨基的荧光分子中引入亲电磺酰胺键[例如,香豆素、甲酚紫和罗丹明的 2,4-二硝基苯磺酰胺(DNs)衍生物]来合成这些底物。这些衍生物基本上没有荧光,在 GST 催化裂解二硝基苯磺酰胺后,游离荧光团被释放(同时形成 1-谷胱甘肽-2,4-二硝基苯+SO(2))。所有香豆素、甲酚紫和罗丹明基荧光探针对于大多数 GSTs,尤其是 GSTA(1-1),都是很好的底物,其荧光强度增加(71-1200 倍)、k(cat)/K(m)值(10(4)-10(7) M(-1) s(-1))和速率增强(10(6)-10(9)-倍)都很高。这些底物成功地应用于定量细胞提取物中的非常低水平的 GST 活性,并且 DNs-甲酚紫也成功地应用于活细胞中微粒体 MGST(1)活性的成像。固定后,甲酚紫染色的细胞保留其荧光,这是一个非常有用的特性。总之,我们描述了一种通用且灵活的生成荧光 GST 底物的策略,其中一些底物提供了迄今为止对 GSTs 最灵敏的检测。

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