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SCX 荷质比选择性分离胰蛋白酶肽与二维反相高效液相色谱联用可实现更详细的蛋白质组图谱分析。

SCX charge state selective separation of tryptic peptides combined with 2D-RP-HPLC allows for detailed proteome mapping.

机构信息

Department of Proteomics, Center for Genetic Engineering and Biotechnology, Ave. 31 e/158 y 190, Cubanacán, Playa, P.O. Box 6162, 10600 Havana, Cuba.

出版信息

J Proteomics. 2013 Oct 8;91:164-71. doi: 10.1016/j.jprot.2013.06.033. Epub 2013 Jul 11.

DOI:10.1016/j.jprot.2013.06.033
PMID:23851314
Abstract

UNLABELLED

Multidimensional peptide fractionation is widely used in proteomics to reduce the complexity of peptide mixtures prior to mass spectrometric analysis. Here, we describe the sequential use of strong cation exchange and reversed phase liquid chromatography in both basic and acidic pH buffers for separating tryptic peptides from complex mixtures of proteins. Strong cation exchange exclusively separates peptide by their charge state into neutral, singly and multi-charged species. To further reduce complexity, each peptide group was separated by reversed phase liquid chromatography at basic pH and the resultant fractions were analyzed by LC-MS/MS. This workflow was applied to a soluble protein lysate from mouse embryonic fibroblast cells, and more than 5000 proteins from 29,843 peptides were identified. The high selectivity displayed during the SCX step (93% to 100%) and the overlaps between proteins identified from the SCX-separated peptide groups, are interesting assets of the procedure.

BIOLOGICAL SIGNIFICANCE

The present work shows how complex mixture of peptides can be selectively separated by SCX based essentially on the net charge of peptides. The proposed workflow results in three well-defined subset of peptides of specific amino acid composition, which are representative of the constituent proteins. The very high selectivity obtained (93% to 99%) on the peptide side, underscores for the first time the possibility of SCX chromatography to aid in validating identified peptides.

摘要

未标记

多维肽分级广泛用于蛋白质组学,以在质谱分析之前降低肽混合物的复杂性。在这里,我们描述了在碱性和酸性 pH 缓冲液中顺序使用强阳离子交换和反相液相色谱法从复杂的蛋白质混合物中分离胰蛋白酶肽。强阳离子交换仅根据其荷电状态将肽分离为中性、单电荷和多电荷物种。为了进一步降低复杂性,将每个肽组在碱性 pH 下通过反相液相色谱法分离,并通过 LC-MS/MS 分析所得馏分。该工作流程应用于来自小鼠胚胎成纤维细胞的可溶性蛋白质裂解物,从 29843 个肽中鉴定出超过 5000 种蛋白质。在 SCX 步骤中显示出的高选择性(93%至 100%)和从 SCX 分离的肽组中鉴定出的蛋白质之间的重叠,是该程序的有趣资产。

生物学意义

本工作展示了如何通过基本上基于肽的净电荷来选择性地分离复杂的肽混合物。所提出的工作流程产生了三个具有特定氨基酸组成的明确肽子集,它们代表了组成蛋白质。在肽侧获得的非常高的选择性(93%至 99%)首次强调了 SCX 色谱法有助于验证鉴定出的肽的可能性。

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