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一种协调的蛋白质组学方法,用于鉴定与大肠杆菌核糖体蛋白 S12 相互作用的蛋白质。

A coordinated proteomic approach for identifying proteins that interact with the E. coli ribosomal protein S12.

机构信息

Laboratory of Neurotoxicology, National Institute of Mental Health , Bethesda, Maryland 20892, United States.

出版信息

J Proteome Res. 2013 Mar 1;12(3):1289-99. doi: 10.1021/pr3009435. Epub 2013 Feb 1.

Abstract

The bacterial ribosomal protein S12 contains a universally conserved D88 residue on a loop region thought to be critically involved in translation due to its proximal location to the A site of the 30S subunit. While D88 mutants are lethal this residue has been found to be post-translationally modified to β-methylthioaspartic acid, a post-translational modification (PTM) identified in S12 orthologs from several phylogenetically distinct bacteria. In a previous report focused on characterizing this PTM, our results provided evidence that this conserved loop region might be involved in forming multiple proteins-protein interactions ( Strader , M. B. ; Costantino , N. ; Elkins , C. A. ; Chen , C. Y. ; Patel , I. ; Makusky , A. J. ; Choy , J. S. ; Court , D. L. ; Markey , S. P. ; Kowalak , J. A. A proteomic and transcriptomic approach reveals new insight into betamethylthiolation of Escherichia coli ribosomal protein S12. Mol. Cell. Proteomics 2011 , 10 , M110 005199 ). To follow-up on this study, the D88 containing loop was probed to identify candidate binders employing a two-step complementary affinity purification strategy. The first involved an endogenously expressed S12 protein containing a C-terminal tag for capturing S12 binding partners. The second strategy utilized a synthetic biotinylated peptide representing the D88 conserved loop region for capturing S12 loop interaction partners. Captured proteins from both approaches were detected by utilizing SDS-PAGE and one-dimensional liquid chromatography-tandem mass spectrometry. The results presented in this report revealed proteins that form direct interactions with the 30S subunit and elucidated which are likely to interact with S12. In addition, we provide evidence that two proteins involved in regulating ribosome and/or mRNA transcript levels under stress conditions, RNase R and Hfq, form direct interactions with the S12 conserved loop, suggesting that it is likely part of a protein binding interface.

摘要

核糖体蛋白 S12 的细菌包含一个普遍保守的 D88 残基在一个环区,由于其接近 30S 亚基的 A 位点,被认为在翻译中至关重要。虽然 D88 突变体是致命的,但这个残基已经被发现被翻译后修饰为β-甲基硫代天冬氨酸,这是一种在几种系统发育上不同的细菌的 S12 同源物中发现的翻译后修饰 (PTM)。在之前的一份专注于描述这种 PTM 的报告中,我们的结果提供了证据表明,这个保守的环区可能参与形成多个蛋白质-蛋白质相互作用 (Strader, M. B. ; Costantino, N. ; Elkins, C. A. ; Chen, C. Y. ; Patel, I. ; Makusky, A. J. ; Choy, J. S. ; Court, D. L. ; Markey, S. P. ; Kowalak, J. A. A proteomic and transcriptomic approach reveals new insight into betamethylthiolation of Escherichia coli ribosomal protein S12. Mol. Cell. Proteomics 2011, 10, M110 005199)。为了跟进这项研究,用两步互补亲和纯化策略探测含有 D88 的环以鉴定候选结合物。第一步涉及一种含有 C 端标签的内源性表达的 S12 蛋白,用于捕获 S12 结合伙伴。第二种策略利用一种代表 D88 保守环区的合成生物素化肽来捕获 S12 环相互作用伙伴。从两种方法捕获的蛋白质都通过 SDS-PAGE 和一维液相串联质谱检测到。本报告中提出的结果揭示了与 30S 亚基直接相互作用的蛋白质,并阐明了哪些可能与 S12 相互作用。此外,我们提供的证据表明,两种参与调节核糖体和/或应激条件下 mRNA 转录水平的蛋白质,RNase R 和 Hfq,与 S12 保守环直接相互作用,这表明它可能是一个蛋白质结合界面的一部分。

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