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囊泡钙调节着前高尔基体中间产物的衣被保留、融合性和大小。

Vesicular calcium regulates coat retention, fusogenicity, and size of pre-Golgi intermediates.

机构信息

Division of Biological Sciences and Center for Structural and Functional Neuroscience, The University of Montana, Missoula, MT 59812-4824, USA.

出版信息

Mol Biol Cell. 2010 Mar 15;21(6):1033-46. doi: 10.1091/mbc.e09-10-0914. Epub 2010 Jan 20.

DOI:10.1091/mbc.e09-10-0914
PMID:20089833
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2836956/
Abstract

The significance and extent of Ca(2+) regulation of the biosynthetic secretory pathway have been difficult to establish, and our knowledge of regulatory relationships integrating Ca(2+) with vesicle coats and function is rudimentary. Here, we investigated potential roles and mechanisms of luminal Ca(2+) in the early secretory pathway. Specific depletion of luminal Ca(2+) in living normal rat kidney cells using cyclopiazonic acid (CPA) resulted in the extreme expansion of vesicular tubular cluster (VTC) elements. Consistent with this, a suppressive role for vesicle-associated Ca(2+) in COPII vesicle homotypic fusion was demonstrated in vitro using Ca(2+) chelators. The EF-hand-containing protein apoptosis-linked gene 2 (ALG-2), previously implicated in the stabilization of sec31 at endoplasmic reticulum exit sites, inhibited COPII vesicle fusion in a Ca(2+)-requiring manner, suggesting that ALG-2 may be a sensor for the effects of vesicular Ca(2+) on homotypic fusion. Immunoisolation established that Ca(2+) chelation inhibits and ALG-2 specifically favors residual retention of the COPII outer shell protein sec31 on pre-Golgi fusion intermediates. We conclude that vesicle-associated Ca(2+), acting through ALG-2, favors the retention of residual coat molecules that seem to suppress membrane fusion. We propose that in cells, these Ca(2+)-dependent mechanisms temporally regulate COPII vesicle interactions, VTC biogenesis, cargo sorting, and VTC maturation.

摘要

细胞内钙离子对生物合成分泌途径的调控意义和程度一直难以确定,我们对整合钙离子与囊泡外壳和功能的调控关系的了解还处于初级阶段。在这里,我们研究了腔内腔钙离子在早期分泌途径中的潜在作用和机制。使用环匹阿尼酸(CPA)特异性耗尽活正常大鼠肾细胞中的腔内腔钙离子,导致囊泡管状簇(VTC)元件的极度扩张。与此一致,使用钙离子螯合剂在体外证明了囊泡相关钙离子在 COPII 囊泡同源融合中的抑制作用。含有 EF 手的蛋白凋亡相关基因 2(ALG-2)先前被认为在稳定内质网出口部位的 sec31 方面起作用,以钙离子依赖的方式抑制 COPII 囊泡融合,这表明 ALG-2 可能是囊泡钙离子对同源融合影响的传感器。免疫分离确立了钙离子螯合抑制和 ALG-2 特别有利于 COPII 外壳蛋白 sec31 在高尔基前融合中间体上的残留保留。我们得出结论,囊泡相关的钙离子通过 ALG-2 促进保留似乎抑制膜融合的残留外套分子。我们提出,在细胞中,这些依赖钙离子的机制暂时调节 COPII 囊泡相互作用、VTC 的生物发生、货物分拣和 VTC 的成熟。

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