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尿调节蛋白聚合分析为调节ZP结构域介导的蛋白质组装机制提供了新见解。

Analysis of uromodulin polymerization provides new insights into the mechanisms regulating ZP domain-mediated protein assembly.

作者信息

Schaeffer Céline, Santambrogio Sara, Perucca Simone, Casari Giorgio, Rampoldi Luca

机构信息

Dulbecco Telethon Institute, Molecular Genetics of Renal Disorders, San Raffaele Scientific Institute, 20132 Milan, Italy.

出版信息

Mol Biol Cell. 2009 Jan;20(2):589-99. doi: 10.1091/mbc.e08-08-0876. Epub 2008 Nov 12.

Abstract

Uromodulin is the most abundant protein secreted in urine, in which it is found as a high-molecular-weight polymer. Polymerization occurs via its zona pellucida (ZP) domain, a conserved module shared by many extracellular eukaryotic proteins that are able to assemble into matrices. In this work, we identified two motifs in uromodulin, mapping in the linker region of the ZP domain and in between protein cleavage and glycosylphosphatidylinositol (GPI)-anchoring sites, which regulate its polymerization. Indeed, mutations in either module led to premature intracellular polymerization of a soluble uromodulin isoform, demonstrating the inhibitory role of these motifs for ZP domain-mediated protein assembly. Proteolytic cleavage separating the external motif from the mature monomer is necessary to release the inhibitory function and allow protein polymerization. Moreover, we report absent or abnormal assembly into filaments of GPI-anchored uromodulin mutated in either the internal or the external motif. This effect is due to altered processing on the plasma membrane, demonstrating that the presence of the two modules has not only an inhibitory function but also can positively regulate protein polymerization. Our data expand previous knowledge on the control of ZP domain function and suggest a common mechanism regulating polymerization of ZP domain proteins.

摘要

尿调节蛋白是尿液中分泌的最丰富的蛋白质,它以高分子量聚合物的形式存在。聚合作用通过其透明带(ZP)结构域发生,ZP结构域是许多能够组装成基质的细胞外真核蛋白质所共有的保守模块。在这项研究中,我们在尿调节蛋白中鉴定出两个基序,分别位于ZP结构域的连接区以及蛋白质裂解和糖基磷脂酰肌醇(GPI)锚定位点之间,它们调节尿调节蛋白的聚合。事实上,任一模块中的突变都会导致可溶性尿调节蛋白异构体在细胞内过早聚合,这表明这些基序对ZP结构域介导的蛋白质组装具有抑制作用。将外部基序与成熟单体分离的蛋白水解裂解对于释放抑制功能并允许蛋白质聚合是必要的。此外,我们报道了在内部或外部基序中发生突变的GPI锚定尿调节蛋白无法正常组装成细丝或组装异常。这种效应是由于质膜上的加工改变所致,表明这两个模块的存在不仅具有抑制功能,还可以正向调节蛋白质聚合。我们的数据扩展了先前关于ZP结构域功能控制的知识,并提出了一种调节ZP结构域蛋白聚合的共同机制。

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