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钙连蛋白对MDCK细胞中主要分泌蛋白gp80折叠中间体的伴侣功能。氧化还原状态和ATP的调节作用。

Chaperone function of calnexin for the folding intermediate of gp80, the major secretory protein in MDCK cells. Regulation by redox state and ATP.

作者信息

Wada I, Ou W J, Liu M C, Scheele G

机构信息

Laboratory of Cell and Molecular Biology, Charles A. Dana Research Institute, Beth Israel Hospital, Boston, Massachusetts.

出版信息

J Biol Chem. 1994 Mar 11;269(10):7464-72.

PMID:7907329
Abstract

The endoplasmic reticulum (ER) not only links the translational machinery to the endomembrane system in eukaryotic cells but also provides a protective environment for the folding of exoplasmic proteins translocated across the ER membrane. Here we describe that the lumenal surface of the ER membranes transiently tethers the folding intermediate of secretory proteins via a 90-kDa ER membrane protein, calnexin. We demonstrate that p70, the precursor to gp80, the major secretory protein in Madin-Darby canine kidney (MDCK) cells, was bound transiently to calnexin in the immediate post-synthetic period (0-10 min) and showed a t1/2 for dissociation from calnexin of 2.5 min. The bound p70 was found to be incompletely folded as assessed by susceptibility to proteinase K digestion. Perturbation of the redox state by 5 mM dithiothreitol or 1 mM diamide markedly inhibited the dissociation of p70 from calnexin (t1/2 > 30 min). Cellular depletion of ATP led to premature dissociation of p70 from calnexin and the formation of p70 aggregates that did not bind calnexin. These findings demonstrate that nascent unfolded p70 is tethered to calnexin during normal protein maturation, including the formation and editing of disulfide bonds and that ATP is required for the productive interaction of gp80 and calnexin.

摘要

内质网(ER)不仅在真核细胞中将翻译机制与内膜系统相连,还为跨内质网膜转运的外质蛋白折叠提供了一个保护性环境。在此,我们描述内质网膜的腔表面通过一种90 kDa的内质网膜蛋白钙连蛋白,短暂地束缚分泌蛋白的折叠中间体。我们证明,在合成后即刻阶段(0 - 10分钟),Madin - Darby犬肾(MDCK)细胞中的主要分泌蛋白gp80的前体p70与钙连蛋白短暂结合,并且从钙连蛋白解离的半衰期为2.5分钟。通过蛋白酶K消化敏感性评估发现,结合的p70未完全折叠。5 mM二硫苏糖醇或1 mM二酰胺对氧化还原状态的扰动显著抑制了p70从钙连蛋白的解离(半衰期> 30分钟)。细胞内ATP的耗尽导致p70从钙连蛋白过早解离,并形成不与钙连蛋白结合的p70聚集体。这些发现表明,在正常蛋白质成熟过程中,包括二硫键的形成和编辑,新生的未折叠p70与钙连蛋白相连,并且ATP是gp80与钙连蛋白有效相互作用所必需的。

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