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差异蛋白质组学筛选以证明非洲爪蟾胚胎无细胞提取物中在有丝分裂退出时泛素化的蛋白质。

Differential proteomic screen to evidence proteins ubiquitinated upon mitotic exit in cell-free extract of Xenopus laevis embryos.

作者信息

Bazile Franck, Gagné Jean-Philippe, Mercier Geneviève, Lo Ken Sin, Pascal Aude, Vasilescu Julian, Figeys Daniel, Poirier Guy G, Kubiak Jacek Z, Chesnel Franck

机构信息

CNRS UMR 6061, Institute of Genetics & Development, University of Rennes 1, Mitosis & Meiosis Group, IFR 140 GFAS, 35 043 Rennes Cedex, France.

出版信息

J Proteome Res. 2008 Nov;7(11):4701-14. doi: 10.1021/pr800250x. Epub 2008 Sep 30.

DOI:10.1021/pr800250x
PMID:18823142
Abstract

Post-translational modification of proteins via ubiquitination plays a crucial role in numerous vital functions of the cell. Polyubiquitination is one of the key regulatory processes involved in regulation of mitotic progression. Here we describe a differential proteomic screen dedicated to identification of novel proteins ubiquitinated upon mitotic exit in cell-free extract of Xenopus laevis embryo. Mutated recombinant His6-tagged ubiquitin (Ubi (K48R)) was added to mitotic extract from which we purified conjugated proteins, as well as associated proteins in nondenaturing conditions by cobalt affinity chromatography. Proteins eluted from Ubi (K48R) supplemented and control extracts were compared by LC-MS/MS analysis after monodimensional SDS-PAGE. A total of 144 proteins potentially ubiquitinated or associated with them were identified. Forty-one percent of these proteins were shown to be involved in ubiquitination and/or proteasomal degradation pathway confirming the specificity of the screen. Twelve proteins, among them ubiquitin itself, were shown to carry a "GG" or "LRGG" remnant tag indicating their direct ubiquitination. Interestingly, sequence analysis of ubiquitinated substrates carrying these tags indicated that in Xenopus cell-free embryo extract supplemented with Ubi (K48R) the majority of polyubiquitination occurred through lysine-11 specific ubiquitin chain polymerization. The potential interest in this atypical form of ubiquitination as well as usefulness of our method in analyzing atypical polyubiquitin species is discussed.

摘要

蛋白质的泛素化修饰在细胞的众多重要功能中起着关键作用。多聚泛素化是参与有丝分裂进程调控的关键调节过程之一。在此,我们描述了一种差异蛋白质组学筛选方法,旨在鉴定非洲爪蟾胚胎无细胞提取物有丝分裂退出时泛素化的新蛋白质。将突变的重组His6标签泛素(Ubi (K48R))添加到有丝分裂提取物中,我们通过钴亲和色谱在非变性条件下纯化缀合蛋白以及相关蛋白。在一维SDS-PAGE后,通过LC-MS/MS分析比较从添加Ubi (K48R)的提取物和对照提取物中洗脱的蛋白质。总共鉴定出144种可能泛素化或与其相关的蛋白质。这些蛋白质中有41%被证明参与泛素化和/或蛋白酶体降解途径,证实了筛选的特异性。其中包括泛素本身在内的12种蛋白质被证明带有“GG”或“LRGG”残余标签,表明它们直接被泛素化。有趣的是,对携带这些标签的泛素化底物的序列分析表明,在添加Ubi (K48R)的非洲爪蟾无细胞胚胎提取物中,大多数多聚泛素化是通过赖氨酸-11特异性泛素链聚合发生的。本文讨论了这种非典型泛素化形式的潜在意义以及我们的方法在分析非典型多聚泛素种类方面的实用性。

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