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使用同位素编码 GTP 探针靶向定量分析癌细胞中的 GTP 结合蛋白。

Targeted Quantitative Profiling of GTP-Binding Proteins in Cancer Cells Using Isotope-Coded GTP Probes.

机构信息

Department of Chemistry , University of California, Riverside , Riverside , California 92521 , United States.

Environmental Toxicology Graduate Program , University of California, Riverside , Riverside , California 92521 , United States.

出版信息

Anal Chem. 2018 Dec 18;90(24):14339-14346. doi: 10.1021/acs.analchem.8b03727. Epub 2018 Nov 28.

Abstract

GTP-binding proteins play important roles in many essential biological processes, including cell signaling, trafficking, and protein synthesis. To assess quantitatively these proteins at the whole proteome level, we developed a high-throughput targeted proteomic method based on the use of isotope-coded GTP probes and multiple-reaction monitoring (MRM) analysis. Targeted proteins were labeled with desthiobiotin-GTP probes, digested with trypsin, and the ensuing desthiobiotin-conjugated peptides were enriched with streptavidin beads for LC-MS/MS analysis. We also established a Skyline MRM library based on shotgun proteomic data acquired for 12 different human cell lines. The library contained 605 tryptic peptides derived from 217 GTP-binding proteins, representing approximately 60% of the annotated human GTP-binding proteome. By using this library, in conjunction with isotope-coded GTP probes and scheduled LC-MRM analysis, we investigated the differential expression of GTP-binding proteins in a pair of primary/metastatic colon cancer cell lines (SW480 and SW620). We were able to quantify 97 GTP-binding proteins, and we further validated the differential expression of several GTP-binding proteins by Western blot analysis. Together, we developed a facile targeted quantitative proteomic method for the high-throughput analysis of GTP-binding proteins and applied the method for probing the altered expression of these proteins involved in colon cancer metastasis.

摘要

GTP 结合蛋白在许多重要的生物过程中发挥着重要作用,包括细胞信号转导、运输和蛋白质合成。为了在整个蛋白质组水平上定量评估这些蛋白质,我们开发了一种基于使用同位素编码 GTP 探针和多重反应监测 (MRM) 分析的高通量靶向蛋白质组学方法。靶向蛋白质用去硫生物素-GTP 探针标记,用胰蛋白酶消化,随后用链霉亲和素珠富集去硫生物素缀合的肽,用于 LC-MS/MS 分析。我们还基于 12 种不同的人细胞系获得的 shotgun 蛋白质组学数据建立了一个 Skyline MRM 文库。该文库包含 605 个来自 217 个 GTP 结合蛋白的胰蛋白酶肽段,代表约 60%的注释人类 GTP 结合蛋白质组。通过使用该文库,结合同位素编码 GTP 探针和预定的 LC-MRM 分析,我们研究了一对原发性/转移性结肠癌细胞系(SW480 和 SW620)中 GTP 结合蛋白的差异表达。我们能够定量 97 个 GTP 结合蛋白,并且通过 Western blot 分析进一步验证了几个 GTP 结合蛋白的差异表达。总之,我们开发了一种简单的靶向定量蛋白质组学方法,用于高通量分析 GTP 结合蛋白,并应用该方法探测参与结肠癌转移的这些蛋白的改变表达。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b8b2/6434709/bac1c3dde920/nihms-1018815-f0002.jpg

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