钙离子/钙调蛋白将v-SNARE突触小泡蛋白的膜近端脂质结合结构域从顺式双层转移至反式双层。
Ca2+/calmodulin transfers the membrane-proximal lipid-binding domain of the v-SNARE synaptobrevin from cis to trans bilayers.
作者信息
de Haro Luc, Ferracci Géraldine, Opi Sandrine, Iborra Cécile, Quetglas Stéphanie, Miquelis Raymond, Lévêque Christian, Seagar Michael
机构信息
Institut National de la Santé et de la Recherche Médicale/Université de la Méditerranée, Unité Mixte de Recherche 464, Faculté de Médecine Secteur Nord, Boulevard Pierre Dramard, 13916 Marseille, France.
出版信息
Proc Natl Acad Sci U S A. 2004 Feb 10;101(6):1578-83. doi: 10.1073/pnas.0303274101. Epub 2004 Feb 2.
Soluble N-ethylmaleimide-sensitive fusion protein attachment protein receptor (SNARE) protein interactions at the synaptic vesicle/plasma membrane interface play an essential role in neurotransmitter release. The membrane-proximal region (amino acids 77-90) of the v-SNARE vesicle-associated membrane protein 2 (VAMP 2, synaptobrevin) binds acidic phospholipids or Ca(2+)/calmodulin in a mutually exclusive manner, processes that are required for Ca(2+)-dependent exocytosis. To address the mechanisms involved, we asked whether this region of VAMP can interact with cis (outer vesicle leaflet) and/or trans (inner plasma membrane leaflet) lipids. To evaluate cis lipid binding, recombinant VAMP was reconstituted into liposomes and accessibility to site-directed antibodies was probed by surface plasmon resonance. Data indicated that the membrane-proximal domain of VAMP dips into the cis lipid bilayer, sequestering epitopes between the tetanus toxin cleavage site and the membrane anchor. These epitopes were unmasked by VAMP double mutation W89A, W90A, which abolishes lipid interactions. To evaluate trans lipid binding, VAMP was reconstituted in cis liposomes, which were then immobilized on beads. The ability of VAMP to capture protein-free (3)H-labeled trans liposomes was then measured. When cis lipid interactions were eliminated by omitting negatively charged lipids, trans lipid binding to VAMP was revealed. In contrast, when cis and trans liposomes both contained acidic headgroups (i.e., approximating physiological conditions), cis lipid interactions totally occluded trans lipid binding. In these conditions Ca(2+)/calmodulin displaced cis inhibition, transferring the lipid-binding domain of VAMP from the cis to the trans bilayer. Our results suggest that calmodulin acts as a unidirectional Ca(2+)-activated shuttle that docks the juxtamembrane portion of the v-SNARE in the target membrane to prepare fusion.
可溶性N - 乙基马来酰亚胺敏感融合蛋白附着蛋白受体(SNARE)蛋白在突触小泡/质膜界面的相互作用在神经递质释放中起关键作用。v - SNARE囊泡相关膜蛋白2(VAMP 2,突触小泡蛋白)的膜近端区域(氨基酸77 - 90)以互斥方式结合酸性磷脂或Ca²⁺/钙调蛋白,这些过程是Ca²⁺依赖性胞吐作用所必需的。为了探究其中涉及的机制,我们研究了VAMP的这个区域是否能与顺式(外小泡叶)和/或反式(内质膜叶)脂质相互作用。为了评估顺式脂质结合,将重组VAMP重构到脂质体中,并通过表面等离子体共振探测定点抗体的可及性。数据表明,VAMP的膜近端结构域深入顺式脂质双层,将表位隔离在破伤风毒素切割位点和膜锚之间。这些表位被VAMP双突变W89A、W90A暴露,该突变消除了脂质相互作用。为了评估反式脂质结合,将VAMP重构到顺式脂质体中,然后固定在珠子上。接着测量VAMP捕获无蛋白³H标记反式脂质体的能力。当通过省略带负电荷的脂质消除顺式脂质相互作用时,揭示了VAMP与反式脂质的结合。相反,当顺式和反式脂质体都含有酸性头部基团时(即接近生理条件),顺式脂质相互作用完全阻断了反式脂质结合。在这些条件下,Ca²⁺/钙调蛋白取代了顺式抑制作用,将VAMP的脂质结合结构域从顺式双层转移到反式双层。我们的结果表明,钙调蛋白作为一种单向Ca²⁺激活的穿梭体,将v - SNARE的近膜部分对接在靶膜中以准备融合。
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