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Quantitative proteomics: a review of different methodologies

机译:定量蛋白质组学:不同方法的综述

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The present review attempts to cover the vast array of methods which have appeared in the last few years for performing quantitative proteome analysis. These methods are divided into two classes: those applicable to conventional two-dimensional map analysis. These methods are divided into two classes: those applicable to conventional two-dimensional map analysis, coupling orthogonally a charge-based step (isoelectric focusing) to a size-based separation [sodium dodecylsulfate (SDS)-electrophoresis] and those applicable to two-dimensional chromatographic protocols. The first method, although being by and large the most popular approach, can offer differential display of paired samples with relatively few methods, the oldest one being based on statistical analysis performed on sets of gels via powerful software packages, such as the MELANIE, PDQuest, Z3 and Z4000, Phoretix and Progenesis. Recent developments comprise analysis performed on a single gel containing mixed samples differentially labeled, either with fluorophors (Cy3 and Cy5) or with d_0 /d_3 acrylamide. Conversely, chromatographic approaches, which mostly rely on analysis not of intact proteins but of their tryptic digests, offer a panoply of differential labeling protocols, most of which rely on stable isotope tagging. Essentially, all possible reactions have been described, such as those involving Lys, Asp, Glu, Cys residues, as well as a number of methods exploiting differential derivatization of amine and carboxyl groups generated during proteolysis. All such methods are described and evaluated.
机译:本综述试图涵盖近几年来进行定量蛋白质组分析的大量方法。这些方法分为两类:适用于常规二维地图分析的方法。这些方法分为两类:适用于常规二维图分析的方法,将基于电荷的步骤(等电聚焦)与基于尺寸的分离[十二烷基硫酸钠(SDS)-电泳]正交耦合的方法和适用于两步法的方法。尺寸色谱协议。第一种方法虽然总的来说是最流行的方法,但可以用相对较少的方法提供配对样品的差异显示,最古老的方法是基于通过功能强大的软件包(例如MELANIE,PDQuest)对凝胶组进行的统计分析,Z3和Z4000,Phoretix和Progenesis。最近的发展包括在单个凝胶上进行的分析,该凝胶包含用荧光团(Cy3和Cy5)或d_0 / d_3丙烯酰胺差异标记的混合样品。相反,色谱方法主要依赖于完整蛋白质的分析而不是胰蛋白酶消化物的分析,因此提供了一系列差异化标记方案,其中大多数依赖于稳定的同位素标记。基本上,已描述了所有可能的反应,例如涉及Lys,Asp,Glu,Cys残基的反应,以及利用蛋白质水解过程中产生的胺和羧基的差异衍生化的许多方法。描述并评估了所有此类方法。

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