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TRPP2/PKD1复合物组装的结构和分子基础。

Structural and molecular basis of the assembly of the TRPP2/PKD1 complex.

作者信息

Yu Yong, Ulbrich Maximilian H, Li Ming-Hui, Buraei Zafir, Chen Xing-Zhen, Ong Albert C M, Tong Liang, Isacoff Ehud Y, Yang Jian

机构信息

Department of Biological Sciences, Columbia University, New York, NY 10027, USA.

出版信息

Proc Natl Acad Sci U S A. 2009 Jul 14;106(28):11558-63. doi: 10.1073/pnas.0903684106. Epub 2009 Jun 25.

Abstract

Mutations in PKD1 and TRPP2 account for nearly all cases of autosomal dominant polycystic kidney disease (ADPKD). These 2 proteins form a receptor/ion channel complex on the cell surface. Using a combination of biochemistry, crystallography, and a single-molecule method to determine the subunit composition of proteins in the plasma membrane of live cells, we find that this complex contains 3 TRPP2 and 1 PKD1. A newly identified coiled-coil domain in the C terminus of TRPP2 is critical for the formation of this complex. This coiled-coil domain forms a homotrimer, in both solution and crystal structure, and binds to a single coiled-coil domain in the C terminus of PKD1. Mutations that disrupt the TRPP2 coiled-coil domain trimer abolish the assembly of both the full-length TRPP2 trimer and the TRPP2/PKD1 complex and diminish the surface expression of both proteins. These results have significant implications for the assembly, regulation, and function of the TRPP2/PKD1 complex and the pathogenic mechanism of some ADPKD-producing mutations.

摘要

多囊蛋白1(PKD1)和多囊蛋白-2(TRPP2)的突变几乎导致了所有常染色体显性多囊肾病(ADPKD)病例。这两种蛋白质在细胞表面形成一种受体/离子通道复合物。我们运用生物化学、晶体学和单分子方法相结合的手段,来确定活细胞质膜中蛋白质的亚基组成,结果发现该复合物包含3个TRPP2和1个PKD1。TRPP2 C末端新鉴定出的卷曲螺旋结构域对于该复合物的形成至关重要。此卷曲螺旋结构域在溶液和晶体结构中均形成同源三聚体,并与PKD1 C末端的单个卷曲螺旋结构域结合。破坏TRPP2卷曲螺旋结构域三聚体的突变会消除全长TRPP2三聚体和TRPP2/PKD1复合物的组装,并减少这两种蛋白质的表面表达。这些结果对TRPP2/PKD1复合物的组装、调节和功能以及某些导致ADPKD的突变的致病机制具有重要意义。

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