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用于监测泛素链重塑的双功能多聚泛素底物的化学酶法合成。

Chemoenzymatic synthesis of bifunctional polyubiquitin substrates for monitoring ubiquitin chain remodeling.

作者信息

Trang Vivian H, Rodgers Margaret L, Boyle Kevin J, Hoskins Aaron A, Strieter Eric R

机构信息

Department of Chemistry, University of Wisconsin-Madison, 1101 University Ave. Madison, WI 53706 (USA).

出版信息

Chembiochem. 2014 Jul 21;15(11):1563-8. doi: 10.1002/cbic.201402059. Epub 2014 Jun 24.

Abstract

Covalent attachment of ubiquitin to target proteins is one of the most pervasive post-translational modifications in eukaryotes. Target proteins are often modified with polymeric ubiquitin chains of defined lengths and linkages that may further undergo dynamic changes in composition in response to cellular signals. Biochemical characterization of the enzymes responsible for building and destroying ubiquitin chains is often thwarted by the lack of methods for preparation of the appropriate substrates containing probes for biochemical or biophysical studies. We have discovered that a yeast ubiquitin C-terminal hydrolase (Yuh1) also catalyzes transamidation reactions that can be exploited to prepare site-specifically modified polyubiquitin chains produced by thiol-ene chemistry. We have used this chemoenzymatic approach to prepare dual-functionalized ubiquitin chains containing fluorophore and biotin modifications. These dual-functionalized ubiquitin chains enabled the first real-time assay of ubiquitin chain disassembly by a human deubiquitinase (DUB) enzyme by single molecule fluorescence microscopy. In summary, this work provides a powerful new tool for elucidating the mechanisms of DUBs and other ubiquitin processing enzymes.

摘要

泛素与靶蛋白的共价连接是真核生物中最普遍的翻译后修饰之一。靶蛋白通常会被具有特定长度和连接方式的多聚泛素链修饰,这些泛素链可能会根据细胞信号进一步发生组成上的动态变化。负责构建和破坏泛素链的酶的生化特性研究常常因缺乏制备含有用于生化或生物物理研究探针的合适底物的方法而受阻。我们发现酵母泛素C末端水解酶(Yuh1)也催化转酰胺反应,该反应可用于制备通过硫醇-烯化学产生的位点特异性修饰的多聚泛素链。我们已使用这种化学酶法制备了含有荧光团和生物素修饰的双功能化泛素链。这些双功能化泛素链通过单分子荧光显微镜首次实现了对人去泛素化酶(DUB)催化的泛素链拆解的实时检测。总之,这项工作为阐明DUB和其他泛素加工酶的作用机制提供了一个强大的新工具。

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