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基于质谱法对人类蛋白质组中赖氨酸和精氨酸甲基化的鉴定与表征

Mass spectrometry-based identification and characterisation of lysine and arginine methylation in the human proteome.

作者信息

Bremang Michael, Cuomo Alessandro, Agresta Anna Maria, Stugiewicz Magdalena, Spadotto Valeria, Bonaldi Tiziana

机构信息

Department of Experimental Oncology, European Institute of Oncology, Via Adamello 16, 20139 Milan, Italy.

出版信息

Mol Biosyst. 2013 Sep;9(9):2231-47. doi: 10.1039/c3mb00009e.

DOI:10.1039/c3mb00009e
PMID:23748837
Abstract

Protein methylation is a post-translational modification (PTM) by which a variable number of methyl groups are transferred to lysine and arginine residues within proteins. Despite increased interest in this modification due to its reversible nature and its emerging role in a diverse set of biological pathways beyond chromatin, global identification of protein methylation has remained an unachieved goal. To characterise sites of lysine and arginine methylation beyond histones, we employed an approach that combines heavy methyl stable isotope labelling by amino acids in cell culture (hmSILAC) with high-resolution mass spectrometry-based proteomics. Through a broad evaluation of immuno-affinity enrichment and the application of two classical protein separation techniques prior to mass spectrometry, to nucleosolic and cytosolic fractions separately, we identified a total of 501 different methylation types, on 397 distinct lysine and arginine sites, present on 139 unique proteins. Our results considerably extend the number of known in vivo methylation sites and indicate their significant presence on several protein complexes involved at all stages of gene expression, from chromatin remodelling and transcription to splicing and translation. In addition, we describe the potential of the hmSILAC approach for accurate relative quantification of methylation levels between distinct functional states.

摘要

蛋白质甲基化是一种翻译后修饰(PTM),通过该修饰,可变数量的甲基被转移到蛋白质内的赖氨酸和精氨酸残基上。尽管由于其可逆性以及在染色质以外的多种生物途径中新兴的作用,人们对这种修饰的兴趣有所增加,但蛋白质甲基化的全面鉴定仍然是一个未实现的目标。为了表征组蛋白以外的赖氨酸和精氨酸甲基化位点,我们采用了一种方法,即将细胞培养中氨基酸的重甲基稳定同位素标记(hmSILAC)与基于高分辨率质谱的蛋白质组学相结合。通过对免疫亲和富集的广泛评估以及在质谱分析之前分别对核质和胞质部分应用两种经典蛋白质分离技术,我们在139种独特蛋白质上的397个不同的赖氨酸和精氨酸位点鉴定出总共501种不同的甲基化类型。我们的结果大大扩展了已知的体内甲基化位点数量,并表明它们在参与基因表达各个阶段的几种蛋白质复合物中大量存在,从染色质重塑、转录到剪接和翻译。此外,我们描述了hmSILAC方法在准确相对定量不同功能状态之间甲基化水平方面的潜力。

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