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内质网质量控制与细胞凋亡。

Endoplasmic reticulum quality control and apoptosis.

作者信息

Groenendyk Jody, Michalak Marek

机构信息

Department of Biochemistry, University of Alberta, Edmonton, Alberta, Canada.

出版信息

Acta Biochim Pol. 2005;52(2):381-95. Epub 2005 May 31.

PMID:15933766
Abstract

The ER is one of the most important folding compartments within the cell, as well as an intracellular Ca(2+) storage organelle and it contains a number of Ca(2+) regulated molecular chaperones responsible for the proper folding of glycosylated as well as non-glycosylated proteins. The luminal environment of the ER contains Ca(2+) which is involved in regulating chaperones such as calnexin and calreticulin, as well as apoptotic proteins caspase-12 and Bap31, which may play an important role in determining cellular sensitivity to ER stress and apoptosis. The ER quality control system consists of several molecular chaperones, including calnexin, that assist in properly folding proteins and transporting them through the ER as well as sensing misfolded proteins, attempting to refold them and if this is not possible, targeting them for degradation. Accumulation of misfolded protein in the ER leads to activation of genes responsible for the expression of ER chaperones. The UPR mechanism involves transcriptional activation of chaperones by the membrane-localized transcription factor ATF6, in conjunction with the ER membrane kinase IRE1, as well as translational repression of protein synthesis by another ER membrane kinase PERK. When accumulation of misfolded protein becomes toxic, apoptosis is triggered, potentially with IRE1 involved in signaling via caspase-12. Both the extrinsic and intrinsic apoptotic pathways appear to culminate in the activation of caspases and this results in the recruitment of mitochondria in an essential amplifying manner. Bap31 may direct pro-apoptotic crosstalk between the ER and the mitochondria via Ca(2+) in conjunction with caspase-12 and calnexin. Accordingly, ER stress and the resultant Ca(2+) release must be very carefully regulated because of their effects in virtually all areas of cell function.

摘要

内质网是细胞内最重要的折叠区室之一,也是一种细胞内钙离子储存细胞器,它含有许多钙离子调节分子伴侣,负责糖基化和非糖基化蛋白质的正确折叠。内质网的腔内环境含有钙离子,其参与调节伴侣蛋白如钙连蛋白和钙网蛋白,以及凋亡蛋白半胱天冬酶 - 12和Bap31,它们可能在决定细胞对内质网应激和凋亡的敏感性方面发挥重要作用。内质网质量控制系统由几种分子伴侣组成,包括钙连蛋白,其有助于蛋白质正确折叠并将它们运输通过内质网,同时感知错误折叠的蛋白质,尝试重新折叠它们,如果不可能,则将它们靶向降解。内质网中错误折叠蛋白质的积累导致负责内质网伴侣蛋白表达的基因激活。未折叠蛋白反应机制涉及膜定位转录因子ATF6与内质网膜激酶IRE1共同对伴侣蛋白的转录激活,以及另一种内质网膜激酶PERK对蛋白质合成的翻译抑制。当错误折叠蛋白质的积累变得有毒时,会触发凋亡,可能有IRE1通过半胱天冬酶 - 12参与信号传导。外在和内在凋亡途径似乎都以内切酶的激活而告终,这导致线粒体以一种重要的放大方式被募集。Bap31可能通过钙离子与半胱天冬酶 - 12和钙连蛋白一起介导内质网与线粒体之间的促凋亡串扰。因此,内质网应激及由此产生的钙离子释放必须得到非常仔细的调节,因为它们几乎对细胞功能的所有方面都有影响。

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