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Fast Global Phosphoproteome Profiling of Jurkat T Cells by HIFU-TiO2-SCX-LC-MS/MS

机译:HIFU-TiO2-SCX-LC-MS / MS的快速全局磷酸磷蛋白酶谱分析

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摘要

We propose a new workflow for fast phosphoproteome profiling. The workflow is based on the use of accelerated in-solution trypsin digestion under an ultrasonic field provided by high-intensity focused ultrasound (HIFU) combined with an inverse strategy based on TiO2 selective phosphopeptide enrichment, fractionation by strong cation exchange chromatography (SCX) and analysis by liquid chromatography tandem mass spectrometry (LC-MS/MS) using a high-resolution mass spectrometer. The performance of the method was established for the global phosphoproteome analysis of unstimulated human Jurkat leukemia T cells (E6.1). Using this accelerated workflow, 15367 phosphorylation sites from 13029 different phosphopeptides belonging to 3163 different phosphoproteins were efficiently identified with high-throughput and reproducibility in less than 15 h. The functional analysis revealed significant phosphorylation-based networks that are implicated in immune function and tumor development pathways. The present strategy, HIFU-TiO2-SCX-LC-MS/MS, is the fastest analytical method reported to date for generating large-scale phosphoproteomics data sets (<15 h).
机译:我们提出了一种新的工作流程,用于快速磷脂蛋白组成本。工作流程基于在高强度聚焦超声(HIFU)提供的超声波场下使用加速的溶液胰蛋白酶消化,其基于基于TiO2选择性磷酸富集的逆策略,通过强阳离子交换色谱(SCX)和使用高分辨率质谱仪液相色谱串联质谱(LC-MS / MS)分析。建立了该方法的性能,用于全球磷脂蛋白酶分析的非刺激性人为Jurkat白血病T细胞(E6.1)。使用该加速的工作流程,15367个磷酸化位点,来自属于3163种不同磷蛋白的不同磷酸肽的不同磷酸肽,在少于15小时的情况下有效地鉴定出高通量和再现性。功能分析显示出涉及免疫功能和肿瘤发育途径的显着基于磷酸化的网络。目前的策略HIFU-TiO2-SCX-LC-MS / MS是迄今为止迄今为止的最快分析方法,用于产生大规模磷蛋白组数据集(<15小时)。

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