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利用自下而上和自上而下的质谱分析方法研究果蝇连接组蛋白 H1 的翻译后修饰模式。

Combined bottom-up and top-down mass spectrometry analyses of the pattern of post-translational modifications of Drosophila melanogaster linker histone H1.

机构信息

Institute of Molecular Biology of Barcelona, CSIC, 08028 Barcelona, Spain.

出版信息

J Proteomics. 2012 Jul 16;75(13):4124-38. doi: 10.1016/j.jprot.2012.05.034. Epub 2012 May 27.

DOI:10.1016/j.jprot.2012.05.034
PMID:22647927
Abstract

Linker histone H1 is a major chromatin component that binds internucleosomal DNA and mediates the folding of nucleosomes into a higher-order structure, namely the 30-nm chromatin fiber. Multiple post-translational modifications (PTMs) of core histones H2A, H2B, H3 and H4 have been identified and their important contribution to the regulation of chromatin structure and function is firmly established. In contrast, little is known about histone H1 modifications and their function. Here we address this question in Drosophila melanogaster, which, in contrast to most eukaryotic species, contains a single histone H1 variant, dH1. For this purpose, we combined bottom-up and top-down mass-spectrometry strategies. Our results indicated that dH1 is extensively modified by phosphorylation, methylation, acetylation and ubiquitination, with most PTMs falling in the N-terminal domain. Interestingly, several dH1 N-terminal modifications have also been reported in specific human and/or mouse H1 variants, suggesting that they have conserved functions. In this regard, we also provide evidence for the contribution of one of such conserved PTMs, dimethylation of K27, to heterochromatin organization during mitosis. Furthermore, our results also identified multiple dH1 isoforms carrying several phosphorylations and/or methylations, illustrating the high structural heterogeneity of dH1. In particular, we identified several non-CDK sites at the N-terminal domain that appear to be hierarchically phosphorylated. This study provides the most comprehensive PTM characterization of any histone H1 variant to date.

摘要

连接组蛋白 H1 是一种主要的染色质成分,它与核小体间 DNA 结合,并介导核小体折叠成更高阶的结构,即 30nm 染色质纤维。核心组蛋白 H2A、H2B、H3 和 H4 的多种翻译后修饰(PTMs)已被鉴定,其对染色质结构和功能的调节的重要贡献已得到确立。相比之下,人们对组蛋白 H1 修饰及其功能知之甚少。在这里,我们在黑腹果蝇中解决了这个问题,与大多数真核生物不同,果蝇只含有一种组蛋白 H1 变体,即 dH1。为此,我们结合了自上而下和自下而上的质谱策略。我们的结果表明,dH1 广泛被磷酸化、甲基化、乙酰化和泛素化修饰,大多数 PTM 位于 N 端结构域。有趣的是,几种 dH1 N 端修饰也在特定的人源和/或鼠源 H1 变体中被报道,这表明它们具有保守的功能。在这方面,我们还提供了证据表明,其中一种保守的 PTM,即 K27 的二甲基化,对有丝分裂过程中的异染色质组织有贡献。此外,我们的结果还鉴定了多个携带多种磷酸化和/或甲基化的 dH1 同工型,说明了 dH1 具有高度的结构异质性。特别是,我们在 N 端结构域鉴定了多个似乎是分层磷酸化的非 CDK 位点。这项研究提供了迄今为止任何组蛋白 H1 变体最全面的 PTM 特征描述。

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