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通过选择反应监测(SRM)质谱法定量检测蛋白质剪接变体。

Quantitative Detection of Protein Splice Variants by Selected Reaction Monitoring (SRM) Mass Spectrometry.

机构信息

Biozentrum of the University of Basel, Basel, Switzerland.

出版信息

Methods Mol Biol. 2022;2537:231-246. doi: 10.1007/978-1-0716-2521-7_14.

Abstract

Molecular diversification of the cellular proteome through alternative splicing has emerged as an important biological principle. However, the lack of tools to specifically detect and quantify proteoforms (Smith et al., Nat Methods 10:186-187, 2013) is a major impediment to functional studies. Recently, biological mass spectrometry (MS) has undergone impressive advances (Mann, Nat Rev Mol Cell Biol 17:678, 2016), including the generation of a highly diverse set of biological applications (Aebersold and Mann, Nature 537:347-355, 2016), and has demonstrated to be an essential tool to address many biological questions (Savitski et al., Science 346:1255784, 2014; Rinner et al., Nat Methods 5:315-318, 2008). In particular, targeted LC-MS, with its high selectivity and specificity, is ideally suited for the precise and sensitive quantification of specific proteins and their proteoforms (Picotti and Aebersold, Nat Methods 9:555-566, 2012). We describe in detail the application of this workflow applied to dissect the molecular diversity of the synaptic adhesion proteins and their splicing-derived proteoforms (Schreiner et al., Elife 4:e07794, 2015).

摘要

通过选择性剪接使细胞蛋白质组的分子多样化已经成为一个重要的生物学原理。然而,缺乏专门用于检测和定量蛋白质异构体的工具(Smith 等人,Nat Methods 10:186-187, 2013)是功能研究的主要障碍。最近,生物质谱(MS)取得了令人瞩目的进展(Mann,Nat Rev Mol Cell Biol 17:678, 2016),包括产生了高度多样化的生物应用(Aebersold 和 Mann,Nature 537:347-355, 2016),并已被证明是解决许多生物学问题的重要工具(Savitski 等人,Science 346:1255784, 2014;Rinner 等人,Nat Methods 5:315-318, 2008)。特别是,靶向 LC-MS 以其高选择性和特异性,非常适合特定蛋白质及其蛋白质异构体的精确和敏感定量(Picotti 和 Aebersold,Nat Methods 9:555-566, 2012)。我们详细描述了这种工作流程在剖析突触黏附蛋白及其剪接衍生蛋白质异构体的分子多样性中的应用(Schreiner 等人,Elife 4:e07794, 2015)。

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