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使用由QconCAT基因编码的串联特征肽进行蛋白质组学的多重绝对定量分析。

Multiplexed absolute quantification for proteomics using concatenated signature peptides encoded by QconCAT genes.

作者信息

Pratt Julie M, Simpson Deborah M, Doherty Mary K, Rivers Jenny, Gaskell Simon J, Beynon Robert J

机构信息

Department of Veterinary Preclinical Sciences, University of Liverpool, Crown Street, Liverpool, L69 7ZJ, UK.

出版信息

Nat Protoc. 2006;1(2):1029-43. doi: 10.1038/nprot.2006.129.

Abstract

An important area of proteomics involves the need for quantification, whether relative or absolute. Many methods now exist for relative quantification, but to support biomarker proteomics and systems biology, absolute quantification rather than relative quantification is required. Absolute quantification usually involves the concomitant mass spectrometric determination of signature proteotypic peptides and stable isotope-labeled analogs. However, the availability of standard labeled signature peptides in accurately known amounts is a limitation to the widespread adoption of this approach. We describe the design and synthesis of artificial QconCAT proteins that are concatamers of tryptic peptides for several proteins. This protocol details the methods for the design, expression, labeling, purification, characterization and use of the QconCATs in the absolute quantification of complex protein mixtures. The total time required to complete this protocol (from the receipt of the QconCAT expression plasmid to the absolute quantification of the set of proteins encoded by the QconCAT protein in an analyte sample) is approximately 29 d.

摘要

蛋白质组学的一个重要领域涉及定量需求,无论是相对定量还是绝对定量。目前存在许多用于相对定量的方法,但为了支持生物标志物蛋白质组学和系统生物学,需要的是绝对定量而非相对定量。绝对定量通常涉及对标志性蛋白质型肽段和稳定同位素标记类似物进行同步质谱测定。然而,精确已知量的标准标记标志性肽段的可得性限制了这种方法的广泛应用。我们描述了人工QconCAT蛋白的设计与合成,这些蛋白是几种蛋白质的胰蛋白酶肽段的串联体。本方案详细介绍了QconCAT在复杂蛋白质混合物绝对定量中的设计、表达、标记、纯化、表征及使用方法。完成本方案所需的总时间(从收到QconCAT表达质粒到对分析物样品中QconCAT蛋白编码的一组蛋白质进行绝对定量)约为29天。

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