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拟南芥蛋白二硫键异构酶-2 参与蛋白折叠,并定位于分泌途径和细胞核,在细胞核中与母体效应胚胎阻滞因子相互作用。

Protein disulfide isomerase-2 of Arabidopsis mediates protein folding and localizes to both the secretory pathway and nucleus, where it interacts with maternal effect embryo arrest factor.

机构信息

Department of Molecular Biosciences and Bioengineering, University of Hawaii, Hawaii, USA.

出版信息

Mol Cells. 2011 Nov;32(5):459-75. doi: 10.1007/s10059-011-0150-3. Epub 2011 Sep 5.

Abstract

Protein disulfide isomerase (PDI) is a thiodisulfide oxidoreductase that catalyzes the formation, reduction and rearrangement of disulfide bonds in proteins of eukaryotes. The classical PDI has a signal peptide, two CXXC-containing thioredoxin catalytic sites (a,a'), two noncatalytic thioredoxin fold domains (b,b'), an acidic domain (c) and a C-terminal endoplasmic reticulum (ER) retention signal. Although PDI resides in the ER where it mediates the folding of nascent polypeptides of the secretory pathway, we recently showed that PDI5 of Arabidopsis thaliana chaperones and inhibits cysteine proteases during trafficking to vacuoles prior to programmed cell death of the endothelium in developing seeds. Here we describe Arabidopsis PDI2, which shares a primary structure similar to that of classical PDI. Recombinant PDI2 is imported into ER-derived microsomes and complements the E. coli protein-folding mutant, dsbA. PDI2 interacted with proteins in both the ER and nucleus, including ER-resident protein folding chaperone, BiP1, and nuclear embryo transcription factor, MEE8. The PDI2-MEE8 interaction was confirmed to occur in vitro and in vivo. Transient expression of PDI2-GFP fusions in mesophyll protoplasts resulted in labeling of the ER, nucleus and vacuole. PDI2 is expressed in multiple tissues, with relatively high expression in seeds and root tips. Immunoelectron microscopy with GFP- and PDI2-specific antisera on transgenic seeds (PDI2-GFP) and wild type roots demonstrated that PDI2 was found in the secretory pathway (ER, Golgi, vacuole, cell wall) and the nuclei. Our results indicate that PDI2 mediates protein folding in the ER and has new functional roles in the nucleus.

摘要

蛋白质二硫键异构酶(PDI)是一种硫二硫键氧化还原酶,可催化真核生物蛋白质中二硫键的形成、还原和重排。经典的 PDI 具有信号肽、两个含 CXXC 的硫氧还蛋白催化位点(a,a')、两个非催化性硫氧还蛋白折叠结构域(b,b')、一个酸性结构域(c)和一个内质网(ER)保留信号。虽然 PDI 位于 ER 中,在那里它介导分泌途径中新生多肽的折叠,但我们最近表明,拟南芥 PDI5 伴侣并抑制半胱氨酸蛋白酶在编程性内皮细胞死亡之前向液泡的运输中死亡发育中的种子。在这里,我们描述了拟南芥 PDI2,它与经典 PDI 的一级结构相似。重组 PDI2 被导入 ER 衍生的微粒体中,并补充了大肠杆菌蛋白折叠突变体 dsbA。PDI2 与 ER 和核中的蛋白质相互作用,包括 ER 驻留的蛋白折叠伴侣 BiP1 和核胚胎转录因子 MEE8。PDI2-MEE8 相互作用被证实发生在体外和体内。PDI2-GFP 融合蛋白在叶肉原生质体中的瞬时表达导致 ER、核和液泡的标记。PDI2 在多种组织中表达,在种子和根尖中表达较高。用 GFP 和 PDI2 特异性抗血清对转基因种子(PDI2-GFP)和野生型根进行免疫电子显微镜研究表明,PDI2 存在于分泌途径(ER、高尔基体、液泡、细胞壁)和核中。我们的结果表明,PDI2 介导 ER 中的蛋白折叠,并在核中具有新的功能作用。

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