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丝氨酸糖蛋白是极化的人内皮细胞中的主要蛋白聚糖,并与趋化因子 GROalpha/CXCL1 的分泌有关。

Serglycin is a major proteoglycan in polarized human endothelial cells and is implicated in the secretion of the chemokine GROalpha/CXCL1.

机构信息

Department of Nutrition, University of Oslo, Box 1046, Blindern, 0316 Oslo, Norway.

出版信息

J Biol Chem. 2011 Jan 28;286(4):2636-47. doi: 10.1074/jbc.M110.151944. Epub 2010 Nov 12.

Abstract

Proteoglycan (PG) expression was studied in primary human umbilical vein endothelial cells (HUVEC). RT-PCR analyses showed that the expression of the PG serglycin core protein was much higher than that of the extracellular matrix PG decorin and the cell surface PG syndecan-1. PG biosynthesis was further studied by biosynthetic [(35)S]sulfate labeling of polarized HUVEC. Interestingly, a major part of (35)S-PGs was secreted to the apical medium. A large portion of these PGs was trypsin-resistant, a typical feature of serglycin. The trypsin-resistant PGs were mainly of the chondroitin/dermatan sulfate type but also contained a minor heparan sulfate component. Secreted serglycin was identified by immunoprecipitation as a PG with a core protein of ∼30 kDa. Serglycin was furthermore shown to be present in perinuclear regions and in two distinct types of vesicles throughout the cytoplasm using immunocytochemistry. To search for possible serglycin partner molecules, HUVEC were stained for the chemokine growth-related oncogene α (GROα/CXCL1). Co-localization with serglycin could be demonstrated, although not in all vesicles. Serglycin did not show overt co-localization with tissue-type plasminogen activator-positive vesicles. When PG biosynthesis was abrogated using benzyl-β-D-xyloside, serglycin secretion was decreased, and the number of vesicles with co-localized serglycin and GROα was reduced. The level of GROα in the apical medium was also reduced after xyloside treatment. Together, these findings indicate that serglycin is a major PG in human endothelial cells, mainly secreted to the apical medium and implicated in chemokine secretion.

摘要

蛋白聚糖(PG)在原代人脐静脉内皮细胞(HUVEC)中的表达进行了研究。RT-PCR 分析表明,PG 核心蛋白糖胺聚糖的表达远高于细胞外基质 PG 饰胶蛋白聚糖和细胞表面 PG 黏附素-1。通过对极化 HUVEC 的生物合成 [(35)S]硫酸根标记进一步研究了 PG 生物合成。有趣的是,大部分 (35)S-PG 被分泌到顶端培养基中。这些 PG 的很大一部分对胰蛋白酶具有抗性,这是糖胺聚糖的典型特征。胰蛋白酶抗性 PG 主要为软骨素/角质素硫酸盐型,但也含有少量肝素硫酸盐成分。通过免疫沉淀鉴定,分泌的糖胺聚糖是一种核心蛋白约为 30 kDa 的 PG。免疫细胞化学进一步显示,糖胺聚糖存在于核周区域和细胞质中的两种不同类型的囊泡中。为了寻找可能的糖胺聚糖伴侣分子,用趋化因子生长相关癌基因α(GROα/CXCL1)对 HUVEC 进行染色。虽然不是所有囊泡都能证明与糖胺聚糖共定位,但可以证明与糖胺聚糖共定位。糖胺聚糖与组织型纤溶酶原激活物阳性囊泡没有明显的共定位。当使用苯甲基-β-D-木糖苷阻断 PG 生物合成时,糖胺聚糖的分泌减少,与共定位糖胺聚糖和 GROα 的囊泡数量减少。木糖苷处理后,顶端培养基中 GROα 的水平也降低。这些发现表明糖胺聚糖是人类内皮细胞中的主要 PG,主要分泌到顶端培养基中,并与趋化因子分泌有关。

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