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通过选择反应监测质谱法表征多聚泛素链的连接性

Characterizing the connectivity of poly-ubiquitin chains by selected reaction monitoring mass spectrometry.

作者信息

Mirzaei Hamid, Rogers Richard S, Grimes Barbara, Eng Jimmy, Aderem Alan, Aebersold Ruedi

机构信息

Institute for Systems Biology, Seattle, WA 98103, USA.

出版信息

Mol Biosyst. 2010 Oct;6(10):2004-14. doi: 10.1039/c005242f. Epub 2010 Aug 6.

Abstract

Protein ubiquitination is an essential post-translational modification (PTM) involved in the regulation of a variety of cellular functions, including transcription and protein degradation. Proteins can be both mono- or poly-ubiquitinated. Poly-ubiquitin chains vary in the manner by which the ubiquitin proteins are linked and their total length. Different poly-ubiquitin structures are thought to specify different fates for the target protein but the correlation between poly-ubiquitin structures and their specific cellular function(s) is not well understood. We have developed a set of specific and quantitative targeted mass spectrometry assays to determine the frequency of different types of inter-ubiquitin linkages in poly-ubiquitin chains relative to the total ubiquitin concentration. We chemically synthesized heavy isotope labeled reference peptides that represent the products generated by tryptic digestion of the known forms of inter-ubiquitin links for the yeast Saccharomyces cerevisiae and human, in addition to all peptides from tryptic digestion of a single ubiquitin molecule for these two species. We used these peptides to develop optimized Selected Reaction Monitoring (SRM) assays for their unambiguous detection in biological samples. We used these assays to profile the frequency of the different types of inter-ubiquitin linkages in a mixture of in vitro assembled human poly-ubiquitin chains and 15 isolated poly-ubiquitinated proteins from S. cerevisiae. We then applied the method to detect toxin induced changes in the poly-ubiquitination profile in complex and enriched protein samples.

摘要

蛋白质泛素化是一种重要的翻译后修饰(PTM),参与多种细胞功能的调控,包括转录和蛋白质降解。蛋白质可以被单泛素化或多泛素化。多聚泛素链在泛素蛋白的连接方式及其总长度方面存在差异。不同的多聚泛素结构被认为决定了靶蛋白的不同命运,但多聚泛素结构与其特定细胞功能之间的相关性尚未得到很好的理解。我们开发了一套特异性和定量的靶向质谱分析方法,以确定相对于总泛素浓度,多聚泛素链中不同类型泛素间连接的频率。我们化学合成了重同位素标记的参考肽,这些肽代表了酿酒酵母和人类已知形式的泛素间连接经胰蛋白酶消化产生的产物,以及这两个物种单个泛素分子经胰蛋白酶消化产生的所有肽段。我们使用这些肽开发了优化的选择反应监测(SRM)分析方法,以便在生物样品中进行明确检测。我们使用这些分析方法对体外组装的人类多聚泛素链混合物以及来自酿酒酵母的15种分离的多聚泛素化蛋白质中不同类型泛素间连接的频率进行了分析。然后,我们应用该方法检测复杂且富集的蛋白质样品中毒素诱导的多聚泛素化谱变化。

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