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尿路上皮斑块的组装:四跨膜蛋白在膜蛋白运输中的功能

Assembly of urothelial plaques: tetraspanin function in membrane protein trafficking.

作者信息

Hu Chih-Chi Andrew, Liang Feng-Xia, Zhou Ge, Tu Liyu, Tang Chih-Hang Anthony, Zhou Jessica, Kreibich Gert, Sun Tung-Tien

机构信息

Epithelial Biology Unit, The Ronald O. Perelman Department of Dermatology, New York University School of Medicine, New York, NY 10016, USA.

出版信息

Mol Biol Cell. 2005 Sep;16(9):3937-50. doi: 10.1091/mbc.e05-02-0136. Epub 2005 Jun 15.

Abstract

The apical surface of mammalian urothelium is covered by 16-nm protein particles packed hexagonally to form 2D crystals of asymmetric unit membranes (AUM) that contribute to the remarkable permeability barrier function of the urinary bladder. We have shown previously that bovine AUMs contain four major integral membrane proteins, i.e., uroplakins Ia, Ib, II, and IIIa, and that UPIa and Ib (both tetraspanins) form heterodimers with UPII and IIIa, respectively. Using a panel of antibodies recognizing different conformational states of uroplakins, we demonstrate that the UPIa-dependent, furin-mediated cleavage of the prosequence of UPII leads to global conformational changes in mature UPII and that UPIb also induces conformational changes in its partner UPIIIa. We further demonstrate that tetraspanins CD9, CD81, and CD82 can stabilize their partner protein CD4. These results indicate that tetraspanin uroplakins, and some other tetraspanin proteins, can induce conformational changes leading to the ER-exit, stabilization, and cell surface expression of their associated, single-transmembrane-domained partner proteins and thus can function as "maturation-facilitators." We propose a model of AUM assembly in which conformational changes in integral membrane proteins induced by uroplakin interactions, differentiation-dependent glycosylation, and the removal of the prosequence of UPII play roles in regulating the assembly of uroplakins to form AUM.

摘要

哺乳动物尿路上皮的顶端表面覆盖着16纳米的蛋白质颗粒,这些颗粒呈六边形排列,形成不对称单位膜(AUM)的二维晶体,有助于膀胱具有卓越的渗透屏障功能。我们之前已经表明,牛AUM包含四种主要的整合膜蛋白,即uroplakins Ia、Ib、II和IIIa,并且UPIa和Ib(两者均为四跨膜蛋白)分别与UPII和IIIa形成异源二聚体。使用一组识别uroplakins不同构象状态的抗体,我们证明UPIa依赖性、弗林蛋白酶介导的UPII前序列切割导致成熟UPII发生全局构象变化,并且UPIb也会诱导其伴侣UPIIIa发生构象变化。我们进一步证明,四跨膜蛋白CD9、CD81和CD82可以稳定其伴侣蛋白CD4。这些结果表明,四跨膜蛋白uroplakins以及其他一些四跨膜蛋白可以诱导构象变化,导致其相关的单跨膜结构域伴侣蛋白从内质网输出、稳定并在细胞表面表达, 因此可以作为“成熟促进因子”发挥作用。我们提出了一个AUM组装模型,其中uroplakin相互作用、分化依赖性糖基化以及UPII前序列的去除所诱导的整合膜蛋白构象变化在调节uroplakins组装形成AUM中发挥作用。

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