Optimized and Robust Workflow for Quantifying the Canonical Histone Ubiquitination Marks H2AK119ub and H2BK120ub by LC–MS/MS

IF 3.8 2区 生物学 Q1 BIOCHEMICAL RESEARCH METHODS Journal of Proteome Research Pub Date : 2024-11-18 DOI:10.1021/acs.jproteome.4c0051910.1021/acs.jproteome.4c00519
Mariana Lopes, Peder J. Lund* and Benjamin A. Garcia*, 
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Abstract

The eukaryotic genome is packaged around histone proteins, which are subject to a myriad of post-translational modifications. By controlling DNA accessibility and the recruitment of protein complexes that mediate chromatin-related processes, these modifications constitute a key mechanism of epigenetic regulation. Since mass spectrometry can easily distinguish between these different modifications, it has become an essential technique in deciphering the histone code. Although robust LC–MS/MS methods are available to analyze modifications on the histone N-terminal tails, routine methods for characterizing ubiquitin marks on histone C-terminal regions, especially H2AK119ub, are less robust. Here, we report the development of a simple workflow for the detection and improved quantification of the canonical histone ubiquitination marks H2AK119ub and H2BK120ub. The method entails a fully tryptic digestion of acid-extracted histones, followed by derivatization with heavy or light propionic anhydride. A pooled sample is then spiked into oppositely labeled single samples as a reference channel for relative quantification, and data is acquired using PRM-based nano-LC–MS/MS. We validated our approach with synthetic peptides as well as treatments known to modulate the levels of H2AK119ub and H2BK120ub. This new method complements existing histone workflows, largely focused on the lysine-rich N-terminal regions, by extending modification analysis to other sequence contexts.

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真核生物基因组是由组蛋白包装而成的,而组蛋白会受到无数翻译后修饰的影响。通过控制 DNA 的可及性和介导染色质相关过程的蛋白质复合物的招募,这些修饰构成了表观遗传调控的关键机制。由于质谱法可以轻松区分这些不同的修饰,因此它已成为破译组蛋白密码的重要技术。虽然已有可靠的 LC-MS/MS 方法来分析组蛋白 N 端尾部的修饰,但表征组蛋白 C 端(尤其是 H2AK119ub)泛素标记的常规方法却不那么可靠。在这里,我们报告了一种用于检测和改进定量组蛋白泛素化标记 H2AK119ub 和 H2BK120ub 的简单工作流程。该方法需要对酸提取的组蛋白进行完全胰蛋白酶消化,然后用重或轻丙酸酐进行衍生。然后将集合样品添加到对立标记的单个样品中,作为相对定量的参考通道,并使用基于 PRM 的纳米液相色谱-质谱(nano-LC-MS/MS)获取数据。我们用合成肽以及已知会调节 H2AK119ub 和 H2BK120ub 水平的处理方法验证了我们的方法。这种新方法通过将修饰分析扩展到其他序列上下文,对现有的组蛋白工作流程(主要集中在富含赖氨酸的 N 端区域)进行了补充。
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来源期刊
Journal of Proteome Research
Journal of Proteome Research 生物-生化研究方法
CiteScore
9.00
自引率
4.50%
发文量
251
审稿时长
3 months
期刊介绍: Journal of Proteome Research publishes content encompassing all aspects of global protein analysis and function, including the dynamic aspects of genomics, spatio-temporal proteomics, metabonomics and metabolomics, clinical and agricultural proteomics, as well as advances in methodology including bioinformatics. The theme and emphasis is on a multidisciplinary approach to the life sciences through the synergy between the different types of "omics".
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