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稳定同位素编码脂肪酸转甲基化和质谱法对凝胶分离蛋白质的 S-脂肪酸酰化的比较分析。

Comparative analysis of S-fatty acylation of gel-separated proteins by stable isotope-coded fatty acid transmethylation and mass spectrometry.

机构信息

Key Laboratory of Pesticides and Chemical Biology, Ministry of Education, College of Chemistry, Central China Normal University, Wuhan, Hubei, China.

出版信息

Nat Protoc. 2011 Aug 18;6(9):1377-90. doi: 10.1038/nprot.2011.358.

Abstract

Covalent attachment of palmitic acid or other fatty acids to the thiol groups of cysteine residues of proteins through reversible thioester bonds has an important role in the regulation of diverse biological processes. We describe here the development of a mass spectrometry protocol based on stable isotope-coded fatty acid transmethylation (iFAT) for qualitative and comparative analysis of protein S-fatty acylation under different experimental conditions. In this approach, cellular proteins extracted from different cell states are separated by SDS-PAGE and then the gel is stained with either Coomassie blue or Nile red for improved sensitivity. Protein bands are excised and then an in-gel stable iFAT procedure is performed. The fatty acid methyl esters resulting from derivatization with d0- and d3-methanol are identified by mass spectrometry. By measuring the intensities of labeled and unlabeled fragment ion pairs of fatty acid methyl esters, the levels of S-fatty acylation in different cells or tissues can be compared. This approach has been applied to monitor the changes of S-fatty acylation of zebrafish liver proteome in response to environmental dichlorodiphenyltrichloroethane exposure. Compared with the approach using metabolic incorporation of radioactive fatty acid analogs, it is not only simple and effective but also eliminates the hazards of handling radioactive isotopes.

摘要

通过可逆硫酯键,将棕榈酸或其他脂肪酸共价连接到蛋白质半胱氨酸残基的巯基上,在调节多种生物过程中具有重要作用。我们在这里描述了一种基于稳定同位素编码脂肪酸转甲基化(iFAT)的质谱分析方案的开发,用于在不同实验条件下定性和比较分析蛋白质 S-脂肪酸酰化。在这种方法中,从不同细胞状态提取的细胞蛋白通过 SDS-PAGE 分离,然后用考马斯亮蓝或尼罗红染色以提高灵敏度。然后切除蛋白质条带,并进行凝胶内稳定 iFAT 处理。用 d0-和 d3-甲醇衍生化得到的脂肪酸甲酯通过质谱鉴定。通过测量脂肪酸甲酯标记和未标记片段离子对的强度,可以比较不同细胞或组织中的 S-脂肪酸酰化水平。该方法已应用于监测环境二氯二苯三氯乙烷暴露对斑马鱼肝脏蛋白质组 S-脂肪酸酰化的变化。与使用放射性脂肪酸类似物代谢掺入的方法相比,该方法不仅简单有效,而且消除了处理放射性同位素的危险。

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