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基于硫醇导向的串联质量标签的等压标记定量自上而下蛋白质组学。

Quantitative Top-Down Proteomics by Isobaric Labeling with Thiol-Directed Tandem Mass Tags.

机构信息

Systematic Proteome Research & Bioanalytics, Institute for Experimental Medicine, Christian-Albrechts-Universität zu Kiel, Kiel 24105, Germany.

出版信息

J Proteome Res. 2021 Sep 3;20(9):4495-4506. doi: 10.1021/acs.jproteome.1c00460. Epub 2021 Aug 2.

DOI:10.1021/acs.jproteome.1c00460
PMID:34338531
Abstract

While identification-centric (qualitative) top-down proteomics (TDP) has seen rapid progress in the recent past, the quantification of intact proteoforms within complex proteomes is still challenging. The by far mostly applied approach is label-free quantification, which, however, provides limited multiplexing capacity, and its use in combination with multidimensional separation is encountered with a number of problems. Isobaric labeling, which is a standard quantification approach in bottom-up proteomics, circumvents these limitations. Here, we introduce the application of thiol-directed isobaric labeling for quantitative TDP. For this purpose, we analyzed the labeling efficiency and optimized tandem mass spectrometry parameters for optimal backbone fragmentation for identification and reporter ion formation for quantification. Two different separation schemes, gel-eluted liquid fraction entrapment electrophoresis × liquid chromatography-mass spectrometry (LC-MS) and high/low-pH LC-MS, were employed for the analyses of either () proteomes or combined /yeast samples (two-proteome interference model) to study potential ratio compression. While the thiol-directed labeling introduces a bias in the quantifiable proteoforms, being restricted to Cys-containing proteoforms, our approach showed excellent accuracy in quantification, which is similar to that achievable in bottom-up proteomics. For example, 876 proteoforms could be quantified with high accuracy in an lysate. The LC-MS data were deposited to the ProteomeXchange with the dataset identifier PXD026310.

摘要

虽然基于鉴定的(定性)自上而下的蛋白质组学(TDP)在过去的几年中取得了快速的进展,但对复杂蛋白质组中完整蛋白质形式的定量仍然具有挑战性。到目前为止,应用最广泛的方法是无标记定量,然而,它提供的多重化能力有限,并且在与多维分离结合使用时会遇到许多问题。同位素标记,这是一种在自下而上的蛋白质组学中常用的定量方法,规避了这些限制。在这里,我们介绍了硫醇导向的同量异位标记在定量 TDP 中的应用。为此,我们分析了标记效率,并优化了串联质谱参数,以获得最佳的骨架碎裂,用于鉴定和报告离子形成,用于定量。我们采用了两种不同的分离方案,凝胶洗脱的液相捕集电泳×液相色谱-质谱(LC-MS)和高/低 pH LC-MS,用于分析()蛋白质组或组合/酵母样品(双蛋白质组干扰模型),以研究潜在的比率压缩。虽然硫醇导向的标记会对可定量的蛋白质形式产生偏见,仅限于含有半胱氨酸的蛋白质形式,但我们的方法在定量方面表现出了优异的准确性,类似于在自下而上的蛋白质组学中实现的准确性。例如,在一个 裂解液中可以高精度地定量 876 个蛋白质形式。LC-MS 数据已被提交到 ProteomeXchange,数据集标识符为 PXD026310。

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