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基于等压质量标签的蛋白质定量实验中定量准确性的评估与改进

Evaluation and Improvement of Quantification Accuracy in Isobaric Mass Tag-Based Protein Quantification Experiments.

作者信息

Ahrné Erik, Glatter Timo, Viganò Cristina, Schubert Conrad von, Nigg Erich A, Schmidt Alexander

机构信息

Biozentrum, University of Basel , Klingelbergstrasse 50/70, 4056 Basel, Switzerland.

出版信息

J Proteome Res. 2016 Aug 5;15(8):2537-47. doi: 10.1021/acs.jproteome.6b00066. Epub 2016 Jul 7.

DOI:10.1021/acs.jproteome.6b00066
PMID:27345528
Abstract

The multiplexing capabilities of isobaric mass tag-based protein quantification, such as Tandem Mass Tags or Isobaric Tag for Relative and Absolute Quantitation have dramatically increased the scope of mass spectrometry-based proteomics studies. Not only does the technology allow for the simultaneous quantification of multiple samples in a single MS injection, but its seamless compatibility with extensive sample prefractionation methods allows for comprehensive studies of complex proteomes. However, reporter ion-based quantification has often been criticized for limited quantification accuracy due to interference from coeluting peptides and peptide fragments. In this study, we investigate the extent of this problem and propose an effective and easy-to-implement remedy that relies on spiking a 6-protein calibration mixture to the samples. We evaluated our ratio adjustment approach using two large scale TMT 10-plex data sets derived from a human cancer and noncancer cell line as well as E. coli cells grown at two different conditions. Furthermore, we analyzed a complex 2-proteome artificial sample mixture and investigated the precision of TMT and precursor ion intensity-based label free quantification. Studying the protein set identified by both methods, we found that differentially abundant proteins were assigned dramatically higher statistical significance when quantified using TMT. Data are available via ProteomeXchange with identifier PXD003346.

摘要

基于等压质量标签的蛋白质定量技术的多重分析能力,如串联质量标签或相对与绝对定量等压标签,极大地扩展了基于质谱的蛋白质组学研究范围。该技术不仅允许在一次质谱进样中同时对多个样品进行定量,而且其与广泛的样品预分级方法的无缝兼容性使得对复杂蛋白质组进行全面研究成为可能。然而,基于报告离子的定量方法常常因共洗脱肽和肽片段的干扰而导致定量准确性有限,受到批评。在本研究中,我们调查了这个问题的严重程度,并提出了一种有效且易于实施的补救方法,即向样品中加入一种6蛋白校准混合物。我们使用来自人类癌细胞系和非癌细胞系以及在两种不同条件下生长的大肠杆菌细胞的两个大规模TMT 10联数据集评估了我们的比率调整方法。此外,我们分析了一个复杂的双蛋白质组人工样品混合物,并研究了TMT和基于前体离子强度的无标记定量的精度。通过研究两种方法鉴定出的蛋白质组,我们发现使用TMT定量时,差异丰度蛋白质被赋予了显著更高的统计显著性。数据可通过ProteomeXchange获得,标识符为PXD003346。

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