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伴侣蛋白钙网蛋白从内质网腔向细胞质的逆向转运。

Retrotranslocation of the chaperone calreticulin from the endoplasmic reticulum lumen to the cytosol.

作者信息

Afshar Nima, Black Ben E, Paschal Bryce M

机构信息

Center for Cell Signaling, University of Virginia, Charlottesville, 22908, USA.

出版信息

Mol Cell Biol. 2005 Oct;25(20):8844-53. doi: 10.1128/MCB.25.20.8844-8853.2005.

Abstract

Polypeptide folding and quality control in the endoplasmic reticulum (ER) are mediated by protein chaperones, including calreticulin (CRT). ER localization of CRT is specified by two types of targeting signals, an N-terminal hydrophobic signal sequence that directs insertion into the ER and a C-terminal KDEL sequence that is responsible for retention in the ER. CRT has been implicated in a number of cytoplasmic and nuclear processes, suggesting that there may be a pathway for generating cytosolic CRT. Here we show that CRT is fully inserted into the ER, undergoes processing by signal peptidase, and subsequently undergoes retrotranslocation to the cytoplasm. A transcription-based reporter assay revealed an important role for the C-terminal Ca(2+) binding domain in CRT retrotranslocation. Neither ubiquitylation nor proteasome activity was necessary for retrotranslocation, which indicates that the pathway is different from that used by unfolded proteins targeted for destruction. Forced expression of cytosolic CRT is sufficient to rescue a cell adhesion defect observed in mouse embryo fibroblasts from crt(-/-) mice. The ability of CRT to retrotranslocate from the ER lumen to the cytosol explains how CRT can change compartments and modulate cell adhesion, transcription, and translation.

摘要

内质网(ER)中的多肽折叠和质量控制由包括钙网蛋白(CRT)在内的蛋白质伴侣介导。CRT的内质网定位由两种类型的靶向信号决定,一种是引导其插入内质网的N端疏水信号序列,另一种是负责将其保留在内质网中的C端KDEL序列。CRT已被证明参与了许多细胞质和细胞核过程,这表明可能存在一条产生胞质CRT的途径。在这里,我们表明CRT完全插入内质网,经过信号肽酶处理,随后逆向转运到细胞质中。基于转录的报告基因分析揭示了CRT逆向转运过程中C端Ca(2+)结合结构域的重要作用。逆向转运既不需要泛素化也不需要蛋白酶体活性,这表明该途径与用于靶向降解的未折叠蛋白所使用的途径不同。强制表达胞质CRT足以挽救crt(-/-)小鼠的小鼠胚胎成纤维细胞中观察到的细胞粘附缺陷。CRT从内质网腔逆向转运到细胞质中的能力解释了CRT如何能够改变区室并调节细胞粘附、转录和翻译。

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