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Novel proteomic approach (PUNCH-P) reveals cell cycle-specific fluctuations in mRNA translation

机译:新型蛋白质组学方法(PUNCH-P)揭示了mRNA翻译中细胞周期特异性的波动

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摘要

Monitoring protein synthesis is essential to our understanding of gene expression regulation, as protein abundance is thought to be predominantly controlled at the level of translation. Mass-spectrometric and RNA sequencing methods have been recently developed for investigating mRNA translation at a global level, but these still involve technical limitations and are not widely applicable. In this study, we describe a novel system-wide proteomic approach for direct monitoring of translation, termed puromycin-associated nascent chain proteomics (PUNCH-P), which is based on incorporation of biotinylated puromycin into newly synthesized proteins under cell-free conditions followed by streptavidin affinity purification and liquid chromatography-tandem mass spectrometry analysis. Using PUNCH-P, we measured cell cycle-specific fluctuations in synthesis for >5000 proteins in mammalian cells, identified proteins not previously implicated in cell cycle processes, and generated the first translational profile of a whole mouse brain. This simple and economical technique is broadly applicable to any cell type and tissue, enabling the identification and quantification of rapid proteome responses under various biological conditions.
机译:监测蛋白质合成对于我们对基因表达调控的理解至关重要,因为据认为蛋白质丰度主要在翻译水平上控制。最近已经开发了质谱和RNA测序方法,用于在全球范围内研究mRNA的翻译,但是这些方法仍存在技术局限性,不能广泛应用。在这项研究中,我们描述了一种用于直接监测翻译的全系统蛋白质组学方法,称为嘌呤霉素相关新生链蛋白质组学(PUNCH-P),该方法基于在无细胞条件下将生物素化嘌呤霉素掺入新合成的蛋白质中,经链霉亲和素亲和纯化和液相色谱-串联质谱分析。使用PUNCH-P,我们测量了哺乳动物细胞中> 5000种蛋白质的合成中特定于细胞周期的波动,鉴定了以前不参与细胞周期过程的蛋白质,并生成了整个小鼠大脑的第一个翻译谱。这种简单而经济的技术广泛适用于任何细胞类型和组织,从而能够在各种生物学条件下鉴定和定量快速蛋白质组反应。

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