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趋化因子跨人血管内皮细胞的转运。

Chemokine transport across human vascular endothelial cells.

作者信息

Mordelet Elodie, Davies Heather A, Hillyer Philippa, Romero Ignacio A, Male David

机构信息

Department of Biological Sciences, The Open University, Milton Keynes, UK.

出版信息

Endothelium. 2007 Jan-Feb;14(1):7-15. doi: 10.1080/10623320601177312.

DOI:10.1080/10623320601177312
PMID:17364892
Abstract

Leukocyte migration across vascular endothelium is mediated by chemokines that are either synthesized by the endothelium or transferred across the endothelium from the tissue. The mechanism of transfer of two chemokines, CXCL10 (interferon gamma-inducible protein [IP]-10) and CCL2 (macrophage chemotactic protein [MCP]-1), was compared across dermal and lung microvessel endothelium and saphenous vein endothelium. The rate of transfer depended on both the type of endothelium and the chemokine. The permeability coefficient (Pe) for CCL2 movement across saphenous vein was twice the value for dermal endothelium and four times that for lung endothelium. In contrast, the Pe value for CXCL10 was lower for saphenous vein endothelium than the other endothelia. The differences in transfer rate between endothelia was not related to variation in paracellular permeability using a paracellular tracer, inulin, and immunoelectron microscopy showed that CXCL10 was transferred from the basal membrane in a vesicular compartment, before distribution to the apical membrane. Although all three endothelia expressed high levels of the receptor for CXCL10 (CXCR3), the transfer was not readily saturable and did not appear to be receptor dependent. After 30 min, the chemokine started to be reinternalized from the apical membrane in clathrin-coated vesicles. The data suggest a model for chemokine transcytosis, with a separate pathway for clearance of the apical surface.

摘要

白细胞穿过血管内皮的迁移是由趋化因子介导的,这些趋化因子要么由内皮细胞合成,要么从组织穿过内皮细胞转移而来。比较了两种趋化因子CXCL10(干扰素γ诱导蛋白[IP]-10)和CCL2(巨噬细胞趋化蛋白[MCP]-1)在真皮和肺微血管内皮以及大隐静脉内皮中的转移机制。转移速率取决于内皮细胞的类型和趋化因子。CCL2穿过大隐静脉的通透系数(Pe)是真皮内皮的两倍,是肺内皮的四倍。相比之下,大隐静脉内皮中CXCL10的Pe值低于其他内皮。内皮细胞之间转移速率的差异与使用细胞旁示踪剂菊粉时细胞旁通透性的变化无关,免疫电子显微镜显示CXCL10在分布到顶膜之前,从基底膜在一个囊泡区室中转移。尽管所有三种内皮细胞都高表达CXCL10的受体(CXCR3),但转移不容易饱和,似乎也不依赖受体。30分钟后,趋化因子开始从顶膜通过网格蛋白包被的囊泡重新内化。这些数据提示了一种趋化因子转胞吞作用的模型,以及一种清除顶表面的独立途径。

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