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使用无标记功能蛋白质组学对五种小鼠核心蛋白质组进行定量分析。

Quantitative profile of five murine core proteomes using label-free functional proteomics.

作者信息

Cutillas Pedro R, Vanhaesebroeck Bart

机构信息

Cell Signalling Group, Ludwig Institute for Cancer Research, London, UK.

出版信息

Mol Cell Proteomics. 2007 Sep;6(9):1560-73. doi: 10.1074/mcp.M700037-MCP200. Epub 2007 Jun 12.

DOI:10.1074/mcp.M700037-MCP200
PMID:17565973
Abstract

Analysis of primary animal and human tissues is key in biological and biomedical research. Comparative proteomics analysis of primary biological material would benefit from uncomplicated experimental work flows capable of evaluating an unlimited number of samples. In this report we describe the application of label-free proteomics to the quantitative analysis of five mouse core proteomes. We developed a computer program and normalization procedures that allow exploitation of the quantitative data inherent in LC-MS/MS experiments for relative and absolute quantification of proteins in complex mixtures. Important features of this approach include (i) its ability to compare an unlimited number of samples, (ii) its applicability to primary tissues and cultured cells, (iii) its straightforward work flow without chemical reaction steps, and (iv) its usefulness not only for relative quantification but also for estimation of absolute protein abundance. We applied this approach to quantitatively characterize the most abundant proteins in murine brain, heart, kidney, liver, and lung. We matched 8,800 MS/MS peptide spectra to 1,500 proteins and generated 44,000 independent data points to profile the approximately 1,000 most abundant proteins in mouse tissues. This dataset provides a quantitative profile of the fundamental proteome of a mouse, identifies the major similarities and differences between organ-specific proteomes, and serves as a paradigm of how label-free quantitative MS can be used to characterize the phenotype of mammalian primary tissues at the molecular level.

摘要

对原代动物和人体组织进行分析是生物学和生物医学研究的关键。对原代生物材料进行比较蛋白质组学分析,将受益于能够评估无限数量样本的简单实验流程。在本报告中,我们描述了无标记蛋白质组学在五种小鼠核心蛋白质组定量分析中的应用。我们开发了一个计算机程序和标准化程序,可利用液相色谱-串联质谱(LC-MS/MS)实验中固有的定量数据,对复杂混合物中的蛋白质进行相对和绝对定量。该方法的重要特点包括:(i)能够比较无限数量的样本;(ii)适用于原代组织和培养细胞;(iii)工作流程简单,无需化学反应步骤;(iv)不仅可用于相对定量,还可用于估计蛋白质的绝对丰度。我们应用该方法对小鼠脑、心脏、肾脏、肝脏和肺中最丰富的蛋白质进行定量表征。我们将8800个MS/MS肽谱与1500种蛋白质进行匹配,生成了44000个独立数据点,以描绘小鼠组织中约1000种最丰富的蛋白质。该数据集提供了小鼠基本蛋白质组的定量概况,确定了器官特异性蛋白质组之间的主要异同,并为无标记定量质谱如何用于在分子水平表征哺乳动物原代组织的表型提供了范例。

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