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固定化金属亲和色谱再探讨:磷酸蛋白质组学中实现高选择性的pH/酸控制

Immobilized metal affinity chromatography revisited: pH/acid control toward high selectivity in phosphoproteomics.

作者信息

Tsai Chia-Feng, Wang Yi-Ting, Chen Yet-Ran, Lai Chen-Yu, Lin Pei-Yi, Pan Kuan-Ting, Chen Jeou-Yuan, Khoo Kay-Hooi, Chen Yu-Ju

机构信息

Department of Chemistry, National Taiwan Normal University, Taipei, Taiwan.

出版信息

J Proteome Res. 2008 Sep;7(9):4058-69. doi: 10.1021/pr800364d. Epub 2008 Aug 16.

DOI:10.1021/pr800364d
PMID:18707149
Abstract

Despite recent advances in instrumentation and analytical strategies for identification and quantitation of protein phosphorylation, a highly specific enrichment protocol is still a challenge in large-scale studies. Here, we report a simple pH/acid control method that addresses the poor specificity seriously criticized in IMAC. Detailed evaluation of the capture and release mechanism in IMAC revealed that pH, buffer and salt yield a complex interplay in enrichment of phosphopeptides, yet they play individual roles in recovery and specificity. A revised one-step IMAC method with low sample loss and high specificity can be rationally designed by controlling salt, pH and the structure and concentration of organic acid. Without methyl esterification, the one-step IMAC enrichment with single LC-MS/MS identified 386 phosphoproteins in 550 mug of non-small-cell lung cancer cell lysate with 96% specificity. Additional fractionation by SDS-PAGE from 4 mg of cell lysate revealed the comprehensive proteome map, identifying 2747 phosphorylation sites from 2360 nondegenerate phosphopeptides and 1219 phosphoproteins with a false discovery rate of 0.63%. To our knowledge, this pH/acid-controlled IMAC procedure provides higher specificity than any other one-step IMAC purification procedure. Furthermore, the simple and reproducible IMAC protocol can be adapted to other solid supports, fully automated or manual, for large-scale identification of the vastly under-explored phosphoproteome.

摘要

尽管在蛋白质磷酸化鉴定和定量的仪器及分析策略方面取得了最新进展,但在大规模研究中,高度特异性的富集方案仍是一项挑战。在此,我们报告一种简单的pH/酸控制方法,该方法解决了在固定金属离子亲和色谱(IMAC)中受到严厉批评的特异性差的问题。对IMAC中捕获和释放机制的详细评估表明,pH、缓冲液和盐在磷酸肽富集过程中产生复杂的相互作用,但它们在回收率和特异性方面发挥着各自的作用。通过控制盐、pH以及有机酸的结构和浓度,可以合理设计出一种具有低样品损失和高特异性的改进型一步IMAC方法。无需甲酯化,采用单重液相色谱-串联质谱(LC-MS/MS)的一步IMAC富集法在550微克非小细胞肺癌细胞裂解物中鉴定出386种磷酸化蛋白,特异性达96%。从4毫克细胞裂解物中通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)进行额外分级分离,揭示了完整的蛋白质组图谱,从2360条非简并磷酸肽中鉴定出2747个磷酸化位点以及1219种磷酸化蛋白,错误发现率为0.63%。据我们所知,这种pH/酸控制的IMAC方法比任何其他一步IMAC纯化方法具有更高的特异性。此外,这种简单且可重复的IMAC方案可适用于其他固体支持物,无论是全自动还是手动操作,用于大规模鉴定研究较少的磷酸蛋白质组。

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