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纤连蛋白片段调节人视网膜毛细血管细胞的增殖和迁移。

Fibronectin fragments modulate human retinal capillary cell proliferation and migration.

作者信息

Grant M B, Caballero S, Bush D M, Spoerri P E

机构信息

Department of Medicine, University of Florida, Gainesville 32610-0226, USA.

出版信息

Diabetes. 1998 Aug;47(8):1335-40. doi: 10.2337/diab.47.8.1335.

DOI:10.2337/diab.47.8.1335
PMID:9703336
Abstract

Capillary morphogenesis involves cell-cell and cell-matrix interactions. Proteases elaborated by capillary cells modify the extracellular matrix (ECM) to facilitate capillary tube formation. Previously, we detected the presence of fibronectin fragments (Fn-f) associated with the proform of matrix metalloprotease-2 (MMP-2) in conditioned medium of human retinal endothelial cells (HRECs). Association of this fragment to latent MMP-2 prevented autocatalytic activation of MMP-2, suggesting a modulatory role of Fn-f in MMP-2 activation. In this report, we examined the potential role of Fn-f on two processes involved in angiogenesis, proliferation and migration of vascular cells. The effects of Fn-f on proliferation were determined by DNA synthesis and cell counts. Their effects on migration were assessed using modified Boyden chambers. Seven Fn-f were tested on vascular cell migration and/or proliferation. Three Fn-f induced migration. Fn-f of 30-kDa and 120-kDa size positively affected proliferation of microvascular cells but not macrovascular cells. A 45-kDa gelatin binding fragment of Fn inhibited HREC proliferation but stimulated pericyte and smooth muscle cell proliferation. The potency of these fragments exceeded that of the known angiogenic growth factor, basic fibroblast growth factor (bFGF), on HREC migration. ECM components such as fibronectin may influence capillary morphogenesis by the generation of fragments that can modulate proliferation, migration, and protease activation. In the setting of diabetes, excess Fn is generated and is available for degradation. Thus, the production of Fn-f may be specifically relevant to the angiogenesis observed in proliferative diabetic retinopathy.

摘要

毛细血管形态发生涉及细胞间和细胞与基质的相互作用。毛细血管细胞分泌的蛋白酶可修饰细胞外基质(ECM)以促进毛细血管管腔的形成。此前,我们在人视网膜内皮细胞(HREC)的条件培养基中检测到与基质金属蛋白酶-2(MMP-2)前体形式相关的纤连蛋白片段(Fn-f)。该片段与潜伏性MMP-2的结合可阻止MMP-2的自催化激活,提示Fn-f在MMP-2激活中具有调节作用。在本报告中,我们研究了Fn-f在血管生成的两个过程,即血管细胞增殖和迁移中所起的潜在作用。通过DNA合成和细胞计数来确定Fn-f对增殖的影响。使用改良的博伊登小室评估其对迁移的影响。对7种Fn-f进行了血管细胞迁移和/或增殖测试。3种Fn-f可诱导迁移。30 kDa和120 kDa大小的Fn-f对微血管细胞的增殖有正向影响,但对大血管细胞无影响。Fn的一种45 kDa明胶结合片段可抑制HREC增殖,但可刺激周细胞和平滑肌细胞增殖。这些片段对HREC迁移的作用强度超过了已知的血管生成生长因子碱性成纤维细胞生长因子(bFGF)。纤连蛋白等ECM成分可能通过产生可调节增殖、迁移和蛋白酶激活的片段来影响毛细血管形态发生。在糖尿病状态下,会产生过量的Fn并可供降解。因此,Fn-f的产生可能与增殖性糖尿病视网膜病变中观察到的血管生成特别相关。

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