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一种无去污剂和溴化氰的完整膜蛋白质组学方法:应用于嗜盐菌紫膜和人类表皮膜蛋白质组

A detergent- and cyanogen bromide-free method for integral membrane proteomics: application to Halobacterium purple membranes and the human epidermal membrane proteome.

作者信息

Blonder Josip, Conrads Thomas P, Yu Li-Rong, Terunuma Atsushi, Janini George M, Issaq Haleem J, Vogel Jonathan C, Veenstra Timothy D

机构信息

SAIC-Frederick Inc., Laboratory of Proteomics and Analytical Technologies Mass Spectrometry Center, National Cancer Institute at Frederick, Frederick, MD 21702-1201, USA.

出版信息

Proteomics. 2004 Jan;4(1):31-45. doi: 10.1002/pmic.200300543.

DOI:10.1002/pmic.200300543
PMID:14730670
Abstract

A simple and rapid method for characterizing hydrophobic integral membrane proteins and its utility for membrane proteomics using microcapillary liquid chromatography coupled on-line with tandem mass spectrometry (microLC-MS/MS) is described. The present technique does not rely on the use of detergents, strong organic acids or cyanogen bromide-mediated proteolysis. A buffered solution of 60% methanol was used to extract, solubilize, and tryptically digest proteins within a preparation of Halobacterium (H.) halobium purple membranes. Analysis of the digested purple membrane proteins by microLC-MS/MS resulted in the identification of all the predicted tryptic peptides of bacteriorhodopsin, including those that are known to be post-translationally modified. In addition, 40 proteins from the purple membrane preparation were also identified, of which 80% are predicted to contain between 1 and 16 transmembrane domains. To evaluate the general applicability of the method, the same extraction, solubilization, and digestion conditions were applied to a plasma membrane fraction prepared from human epidermal sheets. A total of 117 proteins was identified in a single microLC-MS/MS analysis, of which 55% are known to be integral or associated with the plasma membrane. Due to its simplicity, efficiency, and absence of MS interfering compounds, this technique can be used for the characterization of other integral membrane proteins and may be concomitantly applied for the analysis of membrane protein complexes or large-scale proteomic studies of different membrane samples.

摘要

本文描述了一种简单快速的方法,用于表征疏水整合膜蛋白及其在使用微毛细管液相色谱与串联质谱联用(microLC-MS/MS)的膜蛋白质组学中的应用。本技术不依赖于使用去污剂、强有机酸或溴化氰介导的蛋白水解。用60%甲醇的缓冲溶液提取、溶解并胰蛋白酶消化嗜盐菌(H.)紫膜制备物中的蛋白质。通过microLC-MS/MS对消化后的紫膜蛋白进行分析,鉴定出了细菌视紫红质所有预测的胰蛋白酶肽段,包括那些已知经过翻译后修饰的肽段。此外,还鉴定出了来自紫膜制备物的40种蛋白质,其中80%预计含有1至16个跨膜结构域。为了评估该方法的普遍适用性,将相同的提取、溶解和消化条件应用于人表皮片制备的质膜部分。在一次microLC-MS/MS分析中总共鉴定出117种蛋白质,其中55%已知是整合蛋白或与质膜相关的蛋白。由于其简单性、高效性以及不存在质谱干扰化合物,该技术可用于表征其他整合膜蛋白,并可同时应用于膜蛋白复合物的分析或不同膜样品的大规模蛋白质组学研究。

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