IRE1α is an endogenous substrate of endoplasmic-reticulum-associated degradation

被引:0
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作者
Shengyi Sun
Guojun Shi
Haibo Sha
Yewei Ji
Xuemei Han
Xin Shu
Hongming Ma
Takamasa Inoue
Beixue Gao
Hana Kim
Pengcheng Bu
Robert D. Guber
Xiling Shen
Ann-Hwee Lee
Takao Iwawaki
Adrienne W. Paton
James C. Paton
Deyu Fang
Billy Tsai
John R. Yates III
Haoquan Wu
Sander Kersten
Qiaoming Long
Gerald E. Duhamel
Kenneth W. Simpson
Ling Qi
机构
[1] Graduate Program in Biochemistry,Division of Nutritional Sciences
[2] Molecular and Cell Biology,Department of Chemical Physiology
[3] Cornell University,Department of Biomedical Sciences
[4] Cornell University,Department of Cell and Developmental Biology
[5] The Scripps Research Institute,Department of Pathology
[6] Paul L. Foster School of Medicine,Department of Electrical and Computer Engineering
[7] Texas Tech University Health Sciences Center,Department of Biomedical Engineering
[8] University of Michigan Medical School,Department of Biomedical Engineering
[9] Northwestern University,Department of Pathology and Laboratory Medicine
[10] Cornell University,Department of Biomedical Sciences
[11] Cornell University,Department of Clinical Science
[12] Duke University,undefined
[13] Durham,undefined
[14] Weill Cornell Medical College,undefined
[15] Education and Research Support Center,undefined
[16] Gunma University Graduate School of Medicine,undefined
[17] 3-39-22 Showa-machi,undefined
[18] Research Centre for Infectious Diseases,undefined
[19] School of Molecular and Biomedical Science,undefined
[20] University of Adelaide,undefined
[21] Nutrition Metabolism and Genomics group,undefined
[22] Wageningen University,undefined
[23] Laboratory Animal Research Center,undefined
[24] Medical College of Soochow University,undefined
[25] College of Veterinary Medicine,undefined
[26] Cornell University,undefined
[27] College of Veterinary Medicine,undefined
[28] Cornell University,undefined
来源
Nature Cell Biology | 2015年 / 17卷
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摘要
Endoplasmic reticulum (ER)-associated degradation (ERAD) represents a principle quality control mechanism to clear misfolded proteins in the ER; however, its physiological significance and the nature of endogenous ERAD substrates remain largely unexplored. Here we discover that IRE1α, the sensor of the unfolded protein response (UPR), is a bona fide substrate of the Sel1L–Hrd1 ERAD complex. ERAD-mediated IRE1α degradation occurs under basal conditions in a BiP-dependent manner, requires both the intramembrane hydrophilic residues of IRE1α and the lectin protein OS9, and is attenuated by ER stress. ERAD deficiency causes IRE1α protein stabilization, accumulation and mild activation both in vitro and in vivo. Although enterocyte-specific Sel1L-knockout mice (Sel1LΔIEC) are viable and seem normal, they are highly susceptible to experimental colitis and inflammation-associated dysbiosis, in an IRE1α-dependent but CHOP-independent manner. Hence, Sel1L–Hrd1 ERAD serves a distinct, essential function in restraint of IRE1α signalling in vivo by managing its protein turnover.
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页码:1546 / 1555
页数:9
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