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使用与 18O 标记偶联的非透膜化学探针定量分析细胞膜表面蛋白。

Quantitative analysis of cell surface membrane proteins using membrane-impermeable chemical probe coupled with 18O labeling.

机构信息

Biological Sciences Division and Environmental Molecular Sciences Laboratory, Pacific Northwest National Laboratory, Richland, Washington 99352, USA.

出版信息

J Proteome Res. 2010 May 7;9(5):2160-9. doi: 10.1021/pr9009113.

Abstract

We report a mass spectrometry-based strategy for quantitative analysis of cell surface membrane proteome changes. The strategy includes enrichment of surface membrane proteins using a membrane-impermeable chemical probe followed by stable isotope (18)O labeling and LC-MS analysis. We applied this strategy for enriching membrane proteins expressed by Shewanella oneidensis MR-1, a Gram-negative bacterium with known metal-reduction capability via extracellular electron transfer between outer membrane proteins and extracellular electron receptors. LC/MS/MS analysis resulted in the identification of about 400 proteins with 79% of them being predicted to be membrane localized. Quantitative aspects of the membrane enrichment were shown by peptide level (16)O and (18)O labeling of proteins from wild-type and mutant cells (generated from deletion of a type II secretion protein, GspD) prior to LC-MS analysis. Using a chemical probe labeled pure protein as an internal standard for normalization, the quantitative data revealed reduced abundances in Delta gspD mutant cells of many outer membrane proteins including the outer membrane c-type cytochromes OmcA and MtrC, in agreement with a previous report that these proteins are substrates of the type II secretion system.

摘要

我们报道了一种基于质谱的策略,用于定量分析细胞膜蛋白质组的变化。该策略包括使用不可渗透细胞膜的化学探针来富集细胞膜蛋白,然后进行稳定同位素(18)O 标记和 LC-MS 分析。我们应用该策略来富集 Shewanella oneidensis MR-1 表达的膜蛋白,这是一种革兰氏阴性菌,通过外膜蛋白和细胞外电子受体之间的胞外电子传递具有已知的金属还原能力。LC/MS/MS 分析鉴定了约 400 种蛋白质,其中 79%的蛋白质被预测定位于膜上。通过对野生型和突变细胞(从 II 型分泌蛋白 GspD 的缺失中产生)的肽水平(16)O 和(18)O 标记进行膜富集的定量方面,然后进行 LC-MS 分析。使用标记纯蛋白的化学探针作为归一化的内部标准,定量数据显示,Delta gspD 突变细胞中许多外膜蛋白的丰度降低,包括外膜 c 型细胞色素 OmcA 和 MtrC,这与先前的报道一致,即这些蛋白质是 II 型分泌系统的底物。

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