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蛋白质二硫键异构酶相关蛋白ERp29的晶体结构与功能分析

Crystal structure and functional analysis of the protein disulfide isomerase-related protein ERp29.

作者信息

Barak Naomi N, Neumann Piotr, Sevvana Madhumati, Schutkowski Mike, Naumann Kai, Malesević Miroslav, Reichardt Heike, Fischer Gunter, Stubbs Milton T, Ferrari David M

机构信息

Max Planck Research Unit for Enzymology of Protein Folding, Halle (Saale), Germany.

出版信息

J Mol Biol. 2009 Feb 6;385(5):1630-42. doi: 10.1016/j.jmb.2008.11.052. Epub 2008 Dec 3.

DOI:10.1016/j.jmb.2008.11.052
PMID:19084538
Abstract

The protein disulfide isomerase-related protein ERp29 is a putative chaperone involved in processing and secretion of secretory proteins. Until now, however, both the structure and the exact nature of interacting substrates remained unclear. We provide for the first time a crystal structure of human ERp29, refined to 2.9 A, and show that the protein has considerable structural homology to its Drosophila homolog Wind. We show that ERp29 binds directly not only to thyroglobulin and thyroglobulin-derived peptides in vitro but also to the Wind client protein Pipe and Pipe-derived peptides, although it fails to process Pipe in vivo. A monomeric mutant of ERp29 and a D domain mutant in which the second peptide binding site is inactivated also bind protein substrates, indicating that the monomeric thioredoxin domain is sufficient for client protein binding. Indeed, the b domains of ERp29 or Wind, expressed alone, are sufficient for binding proteins and peptides. Interacting peptides have in common two or more aromatic residues, with stronger binding for sequences with overall basic character. Thus, the data allow a view of the two putative peptide binding sites of ERp29 and indicate that the apparent, different processing activity of the human and Drosophila proteins in vivo does not stem from differences in peptide binding properties.

摘要

蛋白质二硫键异构酶相关蛋白ERp29是一种推测的伴侣蛋白,参与分泌蛋白的加工和分泌。然而,迄今为止,其结构以及相互作用底物的确切性质仍不清楚。我们首次提供了人ERp29的晶体结构,分辨率达到2.9埃,并表明该蛋白与其果蝇同源物Wind具有相当大的结构同源性。我们表明,ERp29不仅在体外直接与甲状腺球蛋白和甲状腺球蛋白衍生的肽结合,而且还与Wind的客户蛋白Pipe和Pipe衍生的肽结合,尽管它在体内无法加工Pipe。ERp29的单体突变体和第二个肽结合位点失活的D结构域突变体也能结合蛋白质底物,这表明单体硫氧还蛋白结构域足以结合客户蛋白。实际上,单独表达的ERp29或Wind的b结构域足以结合蛋白质和肽。相互作用的肽共有两个或更多芳香族残基,对具有整体碱性特征的序列结合更强。因此,这些数据使我们能够了解ERp29的两个推测的肽结合位点,并表明人和果蝇蛋白在体内明显不同的加工活性并非源于肽结合特性的差异。

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