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Homogenous Phase Enrichment of Cysteine-Containing Peptides for Improved Proteome Coverage

机译:同源富集含半胱氨酸的肽用于改善蛋白质组覆盖率

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摘要

We describe a proteomic reactor-based homogeneous phase enrichment of cysteine-containing peptides in a filter aided sample preparation (FASP) format. In this approach thiol-reduced proteins are derivatized with thiol-activated polyethylene glycol (TAPEG) before protein cleavage. Consecutive digestion with endoproteinase LysC and trypsin allows isolation of two fractions of nonderivatized peptides. After reduction of disulfide bonds between cysteine-containing peptides and the polyethylene glycol moieties, a third fraction of peptides is collected. LC-MS/MS analyses revealed that on average this fraction consists of 95% cysteine-containing peptides. Since 85-93% of all peptides are unique to a single subfraction, the combination of TAPEG and FASP offers an efficient peptide separation strategy. Analysis of whole cell lysates of mouse brain, liver, red muscle fibers, and CaCo-2 cells using the TAPEG FASP approach allowed identification of 6,900, 5,800, 4,200 and 7,900 proteins, 10-30% more than were identified using two-step digestion without isolation of Cys-containing peptides. The fractionation also increased the protein sequence coverage by 10-30%.
机译:我们描述了基于蛋白质组学反应堆的半胱氨酸肽在过滤辅助样品制备(FASP)格式中的均相富集。在这种方法中,在切割蛋白质之前,先用硫醇活化的聚乙二醇(TAPEG)衍生化巯基还原的蛋白质。用内蛋白酶LysC和胰蛋白酶连续消化可分离出两部分非衍生肽。在含半胱氨酸的肽和聚乙二醇部分之间的二硫键还原后,收集第三部分肽。 LC-MS / MS分析表明,平均而言,该部分由95%的含半胱氨酸的肽组成。由于所有肽的85-93%是单个亚组分所特有的,因此TAPEG和FASP的组合可提供有效的肽分离策略。使用TAPEG FASP方法对小鼠大脑,肝脏,红色肌肉纤维和CaCo-2细胞的全细胞裂解液进行分析,可以鉴定出6,900、5,800、4,200和7,900种蛋白质,比采用两步消化法鉴定的蛋白质高出10-30%无需分离含Cys的肽。分馏还使蛋白质序列覆盖率增加了10-30%。

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  • 作者

    Wisniewski, J.; Prus, G.;

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  • 年度 2015
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  • 原文格式 PDF
  • 正文语种 eng
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