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利用高分辨率自上而下质谱法分析小鼠脑中的组蛋白翻译后修饰

Profiling of Histone Post-Translational Modifications in Mouse Brain with High-Resolution Top-Down Mass Spectrometry.

作者信息

Zhou Mowei, Paša-Tolić Ljiljana, Stenoien David L

机构信息

Pacific Northwest National Laboratory, Earth and Biological Sciences Directorate , P.O. Box 999, Richland, Washington 99352, United States.

出版信息

J Proteome Res. 2017 Feb 3;16(2):599-608. doi: 10.1021/acs.jproteome.6b00694. Epub 2016 Dec 21.

Abstract

As histones play central roles in most chromosomal functions including regulation of DNA replication, DNA damage repair, and gene transcription, both their basic biology and their roles in disease development have been the subject of intense study. Because multiple post-translational modifications (PTMs) along the entire protein sequence are potential regulators of histones, a top-down approach, where intact proteins are analyzed, is ultimately required for complete characterization of proteoforms. However, significant challenges remain for top-down histone analysis primarily because of deficiencies in separation/resolving power and effective identification algorithms. Here we used state-of-the-art mass spectrometry and a bioinformatics workflow for targeted data analysis and visualization. The workflow uses ProMex for intact mass deconvolution, MSPathFinder as a search engine, and LcMsSpectator as a data visualization tool. When complemented with the open-modification tool TopPIC, this workflow enabled identification of novel histone PTMs including tyrosine bromination on histone H4 and H2A, H3 glutathionylation, and mapping of conventional PTMs along the entire protein for many histone subunits.

摘要

由于组蛋白在包括DNA复制调控、DNA损伤修复和基因转录在内的大多数染色体功能中发挥着核心作用,其基础生物学特性及其在疾病发展中的作用一直是深入研究的主题。由于整个蛋白质序列上的多种翻译后修饰(PTM)是组蛋白的潜在调节因子,因此最终需要一种自上而下的方法,即分析完整蛋白质,来全面表征蛋白质变体。然而,自上而下的组蛋白分析仍然面临重大挑战,主要是因为分离/分辨能力和有效识别算法存在不足。在这里,我们使用了最先进的质谱技术和生物信息学工作流程进行靶向数据分析和可视化。该工作流程使用ProMex进行完整质量去卷积,使用MSPathFinder作为搜索引擎,使用LcMsSpectator作为数据可视化工具。当与开放修饰工具TopPIC结合使用时,该工作流程能够识别新的组蛋白PTM,包括组蛋白H4和H2A上的酪氨酸溴化、H3谷胱甘肽化,以及许多组蛋白亚基沿整个蛋白质的常规PTM图谱绘制。

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