Method for recovery and immunoaffinity enrichment of membrane proteins illustrated with metastatic ovarian cancer tissues.

International journal of proteomics Pub Date : 2012-01-01 Epub Date: 2012-07-12 DOI:10.1155/2012/838630
Luke V Schneider, Varsha Likhte, William H Wright, Frances Chu, Emma Cambron, Anne Baldwin-Burnett, Jessica Krakow, Gary B Smejkal
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引用次数: 2

Abstract

Integral membrane proteins play key biological roles in cell signaling, transport, and pathogen invasion. However, quantitative clinical assays for this critical class of proteins remain elusive and are generally limited to serum-soluble extracellular fragments. Furthermore, classic proteomic approaches to membrane protein analysis typically involve proteolytic digestion of the soluble pieces, resulting in separation of intra- and extracellular segments and significant informational loss. In this paper, we describe the development of a new method for the quantitative extraction of intact integral membrane proteins (including GPCRs) from solid metastatic ovarian tumors using pressure cycling technology in combination with a new (ProteoSolve-TD) buffer system. This new extraction buffer is compatible with immunoaffinity methods (e.g., ELISA and immunoaffinity chromatography), as well as conventional proteomic techniques (e.g., 2D gels, western blots). We demonstrate near quantitative recovery of membrane proteins EDG2, EDG4, FASLG, KDR, and LAMP-3 by western blots. We have also adapted commercial ELISAs for serum-soluble membrane protein fragments (e.g., sVEGFR2) to measure the tissue titers of their transmembrane progenitors. Finally, we demonstrate the compatibility of the new buffers with immunoaffinity enrichment/mass spectrometric characterization of tissue proteins.

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转移性卵巢癌组织膜蛋白的恢复和免疫亲和富集方法。
整体膜蛋白在细胞信号传导、运输和病原体入侵中起着关键的生物学作用。然而,这类关键蛋白质的定量临床分析仍然难以捉摸,通常仅限于血清可溶性细胞外片段。此外,膜蛋白分析的经典蛋白质组学方法通常涉及可溶性片段的蛋白质水解消化,导致细胞内和细胞外片段的分离和显著的信息丢失。在本文中,我们描述了一种利用压力循环技术结合新的(proteosolution - td)缓冲系统,从转移性卵巢肿瘤中定量提取完整完整膜蛋白(包括gpcr)的新方法的发展。这种新的提取缓冲液与免疫亲和方法(例如,ELISA和免疫亲和层析)以及传统的蛋白质组学技术(例如,2D凝胶,western blots)兼容。我们证明了膜蛋白EDG2、EDG4、FASLG、KDR和LAMP-3的近定量恢复。我们还采用了血清可溶性膜蛋白片段(例如,sVEGFR2)的商业化elisa来测量其跨膜祖细胞的组织滴度。最后,我们证明了新缓冲液与组织蛋白免疫亲和富集/质谱表征的相容性。
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