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Munc18-2 和 syntaxin 3 控制肥大细胞脱颗粒的两个不同的关键步骤。

Munc18-2 and syntaxin 3 control distinct essential steps in mast cell degranulation.

机构信息

Inserm UMRS-699, 75018 Paris, France.

Université Paris Diderot, Sorbonne Paris Cite, Laboratoire d'excellence INFLAMEX, 75018 Paris, France.

出版信息

J Immunol. 2014 Jan 1;192(1):41-51. doi: 10.4049/jimmunol.1301277. Epub 2013 Dec 9.

DOI:10.4049/jimmunol.1301277
PMID:24323579
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3905451/
Abstract

Mast cell degranulation requires N-ethylmaleimide-sensitive factor attachment protein receptors (SNARE) and mammalian uncoordinated18 (Munc18) fusion accessory proteins for membrane fusion. However, it is still unknown how their interaction supports fusion. In this study, we found that small interfering RNA-mediated silencing of the isoform Munc18-2 in mast cells inhibits cytoplasmic secretory granule (SG) release but not CCL2 chemokine secretion. Silencing of its SNARE-binding partner syntaxin 3 (STX3) also markedly inhibited degranulation, whereas combined knockdown produced an additive inhibitory effect. Strikingly, while Munc18-2 silencing impaired SG translocation, silencing of STX3 inhibited fusion, demonstrating unique roles of each protein. Immunogold studies showed that both Munc18-2 and STX3 are located on the granule surface, but also within the granule matrix and in small nocodazole-sensitive clusters of the cytoskeletal meshwork surrounding SG. After stimulation, clusters containing both effectors were detected at fusion sites. In resting cells, Munc18-2, but not STX3, interacted with tubulin. This interaction was sensitive to nocodazole treatment and decreased after stimulation. Our results indicate that Munc18-2 dynamically couples the membrane fusion machinery to the microtubule cytoskeleton and demonstrate that Munc18-2 and STX3 perform distinct, but complementary, functions to support, respectively, SG translocation and membrane fusion in mast cells.

摘要

肥大细胞脱颗粒需要 N-乙基马来酰亚胺敏感因子附着蛋白受体(SNARE)和哺乳动物无协调蛋白 18(Munc18)融合辅助蛋白进行膜融合。然而,它们的相互作用如何支持融合仍然未知。在这项研究中,我们发现,小干扰 RNA 介导的肥大细胞中 Munc18-2 异构体的沉默抑制了细胞质分泌颗粒(SG)的释放,但不抑制 CCL2 趋化因子的分泌。其 SNARE 结合伙伴突触融合蛋白 3(STX3)的沉默也显著抑制脱颗粒,而联合敲低则产生附加的抑制作用。引人注目的是,虽然 Munc18-2 的沉默会损害 SG 的易位,但 STX3 的沉默会抑制融合,这表明每种蛋白都具有独特的作用。免疫金研究表明,Munc18-2 和 STX3 都位于颗粒表面,但也位于颗粒基质中和围绕 SG 的细胞骨架网格中的小长春花碱敏感簇中。刺激后,在融合部位检测到含有这两种效应物的簇。在静止细胞中,Munc18-2 而不是 STX3 与微管蛋白相互作用。这种相互作用对长春花碱处理敏感,刺激后减少。我们的结果表明,Munc18-2 动态地将膜融合机制与微管细胞骨架偶联,并表明 Munc18-2 和 STX3 分别执行不同但互补的功能,以分别支持肥大细胞中 SG 的易位和膜融合。

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