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Synaptotagmin C2A Loop 2 Mediates Ca2+-dependent SNARE Interactions Essential for Ca2+-triggered Vesicle Exocytosis

机译:Synaptotagmin C2A回路2介导Ca2 +依赖性囊泡相互作用对Ca2 +触发的囊泡胞吐作用至关重要。

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Synaptotagmins contain tandem C2 domains and function as Ca2+ sensors for vesicle exocytosis but the mechanism for coupling Ca2+ rises to membrane fusion remains undefined. Synaptotagmins bind SNAREs, essential components of the membrane fusion machinery, but the role of these interactions in Ca2+-triggered vesicle exocytosis has not been directly assessed. We identified sites on synaptotagmin?1 that mediate Ca2+-dependent SNAP25 binding by zero-length cross-linking. Mutation of these sites in C2A and C2B eliminated Ca2+-dependent synaptotagmin?1 binding to SNAREs without affecting Ca2+-dependent membrane binding. The mutants failed to confer Ca2+ regulation on SNARE-dependent liposome fusion and failed to restore Ca2+-triggered vesicle exocytosis in synaptotagmin-deficient PC12 cells. The results provide direct evidence that Ca2+-dependent SNARE binding by synaptotagmin is essential for Ca2+-triggered vesicle exocytosis and that Ca2+-dependent membrane binding by itself is insufficient to trigger fusion. A structure-based model of the SNARE-binding surface of C2A provided a new view of how Ca2+-dependent SNARE and membrane binding occur simultaneously.
机译:突触标签蛋白含有串联的C2结构域,并作为Ca 2 + 传感器用于囊泡胞吐作用,但偶联Ca 2 + 上升至膜融合的机制仍不清楚。突触结合素结合SNAREs,SNAREs是膜融合机制的重要组成部分,但尚未直接评估这些相互作用在Ca 2 + 触发的囊泡胞吐作用中的作用。我们在突触标记素?1上确定了通过零长度交联介导Ca 2 + 依赖性SNAP25结合的位点。这些位点在C2A和C2B中的突变消除了Ca 2 + 依赖的突触标记素?1与SNARE的结合,而不影响Ca 2 + 依赖性的膜结合。该突变体未能赋予SNARE依赖性脂质体融合Ca 2 + 调控,并未能恢复突触标记素缺陷型PC12细胞中Ca 2 + 触发的囊泡胞吐作用。这些结果提供了直接的证据,表明突触标记素与Ca 2 + 依赖的SNARE结合对于Ca 2 + 触发的囊泡胞吐作用和Ca 2 + 依赖的SNARE和膜结合如何同时发生提供了新的视角。

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