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从人结肠肿瘤细胞系 LIM1215 释放的 A33 免疫亲和纯化的外泌体的蛋白质组学分析揭示了组织特异性蛋白质特征。

Proteomics analysis of A33 immunoaffinity-purified exosomes released from the human colon tumor cell line LIM1215 reveals a tissue-specific protein signature.

机构信息

Joint ProteomicS Laboratory, Ludwig Institute for Cancer Research and the Walter and Eliza Hall Institute of Medical Research, Parkville, Victoria 3050, Australia.

出版信息

Mol Cell Proteomics. 2010 Feb;9(2):197-208. doi: 10.1074/mcp.M900152-MCP200. Epub 2009 Oct 16.

Abstract

Exosomes are 40-100-nm-diameter nanovesicles of endocytic origin that are released from diverse cell types. To better understand the biological role of exosomes and to avoid confounding data arising from proteinaceous contaminants, it is important to work with highly purified material. Here, we describe an immunoaffinity capture method using the colon epithelial cell-specific A33 antibody to purify colorectal cancer cell (LIM1215)-derived exosomes. LC-MS/MS revealed 394 unique exosomal proteins of which 112 proteins (28%) contained signal peptides and a significant enrichment of proteins containing coiled coil, RAS, and MIRO domains. A comparative protein profiling analysis of LIM1215-, murine mast cell-, and human urine-derived exosomes revealed a subset of proteins common to all exosomes such as endosomal sorting complex required for transport (ESCRT) proteins, tetraspanins, signaling, trafficking, and cytoskeletal proteins. A conspicuous finding of this comparative analysis was the presence of host cell-specific (LIM1215 exosome) proteins such as A33, cadherin-17, carcinoembryonic antigen, epithelial cell surface antigen (EpCAM), proliferating cell nuclear antigen, epidermal growth factor receptor, mucin 13, misshapen-like kinase 1, keratin 18, mitogen-activated protein kinase 4, claudins (1, 3, and 7), centrosomal protein 55 kDa, and ephrin-B1 and -B2. Furthermore, we report the presence of the enzyme phospholipid scramblase implicated in transbilayer lipid distribution membrane remodeling. The LIM1215-specific exosomal proteins identified in this study may provide insights into colon cancer biology and potential diagnostic biomarkers.

摘要

外泌体是直径为 40-100nm 的内体起源的纳米囊泡,由多种细胞类型释放。为了更好地了解外泌体的生物学作用,并避免因蛋白质污染物而产生混淆的数据,使用高度纯化的材料非常重要。在这里,我们描述了一种使用结肠上皮细胞特异性 A33 抗体的免疫亲和捕获方法,以纯化结直肠癌细胞(LIM1215)衍生的外泌体。LC-MS/MS 揭示了 394 种独特的外泌体蛋白,其中 112 种蛋白(28%)含有信号肽,并且富含卷曲螺旋、RAS 和 MIRO 结构域的蛋白。LIM1215、鼠肥大细胞和人尿衍生的外泌体的比较蛋白质谱分析显示,所有外泌体都有一组共同的蛋白质,如内体分选复合物所需的运输蛋白(ESCRT)蛋白、四跨膜蛋白、信号转导、运输和细胞骨架蛋白。这项比较分析的一个显著发现是存在宿主细胞特异性(LIM1215 外泌体)蛋白,如 A33、钙粘蛋白 17、癌胚抗原、上皮细胞表面抗原(EpCAM)、增殖细胞核抗原、表皮生长因子受体、粘蛋白 13、畸形样激酶 1、角蛋白 18、丝裂原激活蛋白激酶 4、紧密连接蛋白(1、3 和 7)、中心体蛋白 55kDa、ephrin-B1 和 -B2。此外,我们还报告了参与跨膜脂质分布膜重塑的磷脂 scramblase 酶的存在。本研究中鉴定的 LIM1215 特异性外泌体蛋白可能为结肠癌生物学和潜在的诊断生物标志物提供新的见解。

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