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β8整合素与Rho GDP解离抑制剂-1结合并激活Rac1以抑制系膜细胞肌成纤维细胞分化。

Beta8 integrin binds Rho GDP dissociation inhibitor-1 and activates Rac1 to inhibit mesangial cell myofibroblast differentiation.

作者信息

Lakhe-Reddy Sujata, Khan Shenaz, Konieczkowski Martha, Jarad George, Wu Karen L, Reichardt Louis F, Takai Yoshimi, Bruggeman Leslie A, Wang Bingcheng, Sedor John R, Schelling Jeffrey R

机构信息

Department of Medicine, Case Western Reserve University School of Medicine, Rammelkamp Center for Education and Research, MetroHealth Medical Center, Cleveland, Ohio 44109, USA.

出版信息

J Biol Chem. 2006 Jul 14;281(28):19688-99. doi: 10.1074/jbc.M601110200. Epub 2006 May 11.

Abstract

Alpha(v)beta8 integrin expression is restricted primarily to kidney, brain, and placenta. Targeted alpha(v) or beta8 deletion is embryonic lethal due to defective placenta and brain angiogenesis, precluding investigation of kidney alpha(v)beta8 function. We find that kidney beta8 is localized to glomerular mesangial cells, and expression is decreased in mouse models of glomerulosclerosis, suggesting that beta8 regulates normal mesangial cell differentiation. To interrogate beta8 signaling pathways, yeast two-hybrid and co-precipitation studies demonstrated beta8 interaction with Rho guanine nucleotide dissociation inhibitor-1 (GDI). Selective beta8 stimulation enhanced beta8-GDI interaction as well as Rac1 (but not RhoA) activation and lamellipodia formation. Mesangial cells from itgb8-/- mice backcrossed to a genetic background that permitted survival, or gdi-/- mice, which develop glomerulosclerosis, demonstrated RhoA (but not Rac1) activity and alpha-smooth muscle actin assembly, which characterizes mesangial cell myofibroblast transformation in renal disease. To determine whether Rac1 directly modulates RhoA-associated myofibroblast differentiation, mesangial cells were transduced with inhibitory Rac peptide fused to human immunodeficiency virus-Tat, resulting in enhanced alpha-smooth muscle actin organization. We conclude that the beta8 cytosolic tail in mesangial cells organizes a signaling complex that culminates in Rac1 activation to mediate wild-type differentiation, whereas decreased beta8 activation shifts mesangial cells toward a RhoA-dependent myofibroblast phenotype.

摘要

α(v)β8整合素的表达主要局限于肾脏、大脑和胎盘。由于胎盘和脑血管生成缺陷,靶向性缺失α(v)或β8会导致胚胎致死,这使得对肾脏α(v)β8功能的研究无法进行。我们发现肾脏中的β8定位于肾小球系膜细胞,并且在肾小球硬化的小鼠模型中其表达降低,这表明β8调节正常的系膜细胞分化。为了探究β8信号通路,酵母双杂交和共沉淀研究表明β8与Rho鸟嘌呤核苷酸解离抑制剂-1(GDI)相互作用。选择性刺激β8可增强β8-GDI相互作用以及Rac1(而非RhoA)的激活和片状伪足的形成。回交到允许存活的遗传背景的itgb8-/-小鼠的系膜细胞,或患有肾小球硬化的gdi-/-小鼠的系膜细胞,表现出RhoA(而非Rac1)活性和α-平滑肌肌动蛋白组装,这是肾脏疾病中系膜细胞肌成纤维细胞转化的特征。为了确定Rac1是否直接调节与RhoA相关的肌成纤维细胞分化,用与人免疫缺陷病毒-Tat融合的抑制性Rac肽转导系膜细胞,导致α-平滑肌肌动蛋白组织增强。我们得出结论,系膜细胞中的β8胞质尾部组织形成一个信号复合物,最终导致Rac1激活以介导野生型分化,而β8激活的降低会使系膜细胞向依赖RhoA的肌成纤维细胞表型转变。

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