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星形细胞纤维连接蛋白在视网膜血管生成中的整合素依赖和非依赖功能。

Integrin-dependent and -independent functions of astrocytic fibronectin in retinal angiogenesis.

机构信息

Vascular Biology Laboratory, London Research Institute - Cancer Research UK, London WC2A 3PX, UK.

出版信息

Development. 2011 Oct;138(20):4451-63. doi: 10.1242/dev.071381. Epub 2011 Aug 31.

DOI:10.1242/dev.071381
PMID:21880786
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3177315/
Abstract

Fibronectin (FN) is a major component of the extracellular matrix and functions in cell adhesion, cell spreading and cell migration. In the retina, FN is transiently expressed and assembled on astrocytes (ACs), which guide sprouting tip cells and deposit a provisional matrix for sprouting angiogenesis. The precise function of FN in retinal angiogenesis is largely unknown. Using genetic tools, we show that astrocytes are the major source of cellular FN during angiogenesis in the mouse retina. Deletion of astrocytic FN reduces radial endothelial migration during vascular plexus formation in a gene dose-dependent manner. This effect correlates with reduced VEGF receptor 2 and PI3K/AKT signalling, and can be mimicked by selectively inhibiting VEGF-A binding to FN through intraocular injection of blocking peptides. By contrast, AC-specific replacement of the integrin-binding RGD sequence with FN-RGE or endothelial deletion of itga5 shows little effect on migration and PI3K/AKT signalling, but impairs filopodial alignment along AC processes, suggesting that FN-integrin α5β1 interaction is involved in filopodial adhesion to the astrocytic matrix. AC FN shares its VEGF-binding function and cell-surface distribution with heparan-sulfate (HS), and genetic deletion of both FN and HS together greatly enhances the migration defect, indicating a synergistic function of FN and HS in VEGF binding. We propose that in vivo the VEGF-binding properties of FN and HS promote directional tip cell migration, whereas FN integrin-binding functions to support filopodia adhesion to the astrocytic migration template.

摘要

纤连蛋白 (FN) 是细胞外基质的主要成分,在细胞黏附、细胞铺展和细胞迁移中发挥作用。在视网膜中,FN 短暂表达并装配在星形胶质细胞 (ACs) 上,AC 引导发芽尖端细胞并为发芽血管生成沉积临时基质。FN 在视网膜血管生成中的精确功能在很大程度上尚不清楚。使用遗传工具,我们表明在小鼠视网膜血管生成过程中,星形胶质细胞是细胞 FN 的主要来源。星形胶质细胞 FN 的缺失以基因剂量依赖性方式减少血管丛形成过程中的血管内皮细胞径向迁移。这种效应与 VEGF 受体 2 和 PI3K/AKT 信号的减少相关,并且可以通过眼内注射阻断肽选择性抑制 FN 与 VEGF-A 的结合来模拟。相比之下,通过在 AC 特异性上用 FN-RGE 替换整合素结合 RGD 序列或内皮缺失 itga5,对迁移和 PI3K/AKT 信号的影响很小,但会损害沿 AC 突起排列的丝状伪足,表明 FN-整合素 α5β1 相互作用参与丝状伪足与星形胶质细胞基质的黏附。AC FN 与肝素硫酸盐 (HS) 共享其 VEGF 结合功能和细胞表面分布,FN 和 HS 的遗传缺失共同极大地增强了迁移缺陷,表明 FN 和 HS 在 VEGF 结合中具有协同功能。我们提出,在体内,FN 和 HS 的 VEGF 结合特性促进了定向尖端细胞的迁移,而 FN 整合素结合功能则支持丝状伪足黏附到星形胶质细胞迁移模板。

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