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A coiled coil trigger site is essential for rapid binding of synaptobrevin to the SNARE acceptor complex.

机译:盘绕的线圈触发位点对于突触短肽与SNARE受体复合物的快速结合是必不可少的。

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摘要

Exocytosis from synaptic vesicles is driven by stepwise formation of a tight alpha-helical complex between the fusing membranes. The complex is composed of the three SNAREs: synaptobrevin 2, SNAP-25, and syntaxin 1a. An important step in complex formation is fast binding of vesicular synaptobrevin to the preformed syntaxin 1.SNAP-25 dimer. Exactly how this step relates to neurotransmitter release is not well understood. Here, we combined different approaches to gain insights into this reaction. Using computational methods, we identified a stretch in synaptobrevin 2 that may function as a coiled coil "trigger site." This site is also present in many synaptobrevin homologs functioning in other trafficking steps. Point mutations in this stretch inhibited binding to the syntaxin 1.SNAP-25 dimer and slowed fusion of liposomes. Moreover, the point mutations severely inhibited secretion from chromaffin cells. Altogether, this demonstrates that the trigger site in synaptobrevin is crucial for productive SNARE zippering.
机译:突触小泡的胞吐作用是通过在融合膜之间逐步形成紧密的α-螺旋复合物来驱动的。该复合体由三个SNARE组成:突触短蛋白2,SNAP-25和语法1a。复合物形成中的重要步骤是将囊泡突触壁蛋白与1.SNAP-25二聚体中预先形成的语法快速结合。确切地讲,该步骤与神经递质释放的关系如何。在这里,我们结合了不同的方法来深入了解这一反应。使用计算方法,我们确定了突触融合蛋白2中的一段延伸,该延伸可能起卷曲的线圈“触发位点”的作用。该位点也存在于在其他贩运步骤中起作用的许多突触素的同源物中。在此拉伸中的点突变抑制了与语法1.SNAP-25二聚体的结合并减慢了脂质体的融合。而且,这些点突变严重抑制了嗜铬细胞的分泌。总而言之,这表明突触臂蛋白中的触发位点对于生产高效的SNARE拉链至关重要。

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