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Mass spectrometric-based approaches in quantitative proteomics.

机译:定量蛋白质组学中基于质谱的方法。

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摘要

Classically, experiments aimed at studying changes in protein expression have always followed a small set of proteins. This focused approach was necessary since tools to efficiently analyze large numbers of proteins were simply not available. Large-scale quantitative proteomics promises to produce reams of data that previously would have taken decades to measure with classical methods. Mass spectrometry is already a well-established protein identification tool and recent methodological developments indicate that it can also be successfully applied to extract quantitative data of protein abundance. From the first reports 4 years ago, numerous schemes to take advantage of stable isotope nuclei incorporation in proteins and peptides have been developed. Here we review the benefits and pitfalls of some of the most commonly used protocols, focusing on a procedure now being used extensively in our laboratory, stable isotope labeling with amino acids in cell culture (SILAC). The basic theory, application, anddata analysis of a SILAC experiment are discussed. The emerging nature of these techniques and the rapid pace of technological development make forecasting the directions of the field difficult but we speculate that SILAC will soon be a key tool of quantitative proteomics.
机译:传统上,旨在研究蛋白质表达变化的实验始终遵循一小组蛋白质。这种集中的方法是必要的,因为根本没有有效地分析大量蛋白质的工具。大规模定量蛋白质组学有望产生大量以前用传统方法测量需要数十年的数据。质谱已经是一种成熟的蛋白质鉴定工具,最近的方法学发展表明它也可以成功地用于提取蛋白质丰度的定量数据。从4年前的第一份报告中,已经开发出了许多利用蛋白质和肽中稳定同位素核掺入的方案。在这里,我们回顾一些最常用的方案的好处和陷阱,重点介绍目前在我们的实验室中广泛使用的程序,即在细胞培养物中用氨基酸稳定同位素标记(SILAC)。讨论了SILAC实验的基本理论,应用和数据分析。这些技术的新兴性质以及技术发展的迅速步伐使得很难预测该领域的发展方向,但我们推测SILAC将很快成为定量蛋白质组学的重要工具。

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