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Studies on peptide acetylation for stable-isotope labeling after 1-D PAGE separation in quantitative proteomics

机译:一维PAGE分离后定量蛋白质组学中用于稳定同位素标记的肽乙酰化研究

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摘要

Acetylation is a single labeling process to label peptides in control and experimental samples universally, and is independent of amino acid composition or post-translational modification. Here, we propose a new strategy especially useful to quantify either hydrophobic or extremely acidic and basic proteins involved in acetylation of tryptic peptides after sodium dodecyl sulfate polyarcylamide gel electrophoresis (SDS-PAGE) separation. We studied some essential parameters of acetylation labeling reactions in either in-solution tryptic peptides or in-gel digested extracts systematically. We have found that the acetylation efficiency varies markedly on account of different reactive systems, and demonstrated that stable isotope labeling can be steadily obtained with in-gel digested peptides under optimized conditions. We use this protocol to quantify some proteins of two kinds of hepatocellular carcinoma cell line, non-metastatic hepatocellular carcinoma cells, Hep3B, and metastatic hepatocellular carcinoma cells, MHCC97-H. The experimental results provide positive evidence for the potential application of an acetylation labeling strategy in quantitative proteomics, and an efficient way for global proteome quantification.
机译:乙酰化是单个标记过程,可以普遍地标记对照和实验样品中的肽,并且不依赖于氨基酸组成或翻译后修饰。在这里,我们提出了一种新的策略,特别适用于量化十二烷基硫酸钠聚芳酰胺凝胶电泳(SDS-PAGE)分离后的胰蛋白酶肽的乙酰化反应所涉及的疏水性或极酸性和碱性蛋白。我们系统地研究了溶液中胰蛋白酶肽或凝胶消化的提取物中乙酰化标记反应的一些基本参数。我们已经发现,由于不同的反应体系,乙酰化效率显着不同,并证明在优化的条件下,凝胶内消化的肽可以稳定地获得稳定的同位素标记。我们使用此协议来量化两种肝细胞癌细胞系,非转移性肝细胞癌细胞Hep3B和转移性肝细胞癌细胞MHCC97-H的某些蛋白质。实验结果为乙酰化标记策略在定量蛋白质组学中的潜在应用和整体蛋白质组定量的有效方法提供了积极的证据。

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