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A novel region in the CaV2.1 α1 subunit C-terminus regulates fast synaptic vesicle fusion and vesicle docking at the mammalian presynaptic active zone

机译:CaV2.1α1亚基C末端的一个新区域调节了突触前囊泡的快速融合和在哺乳动物突触前活性区的囊泡对接

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摘要

In central nervous system (CNS) synapses, action potential-evoked neurotransmitter release is principally mediated by CaV2.1 calcium channels (CaV2.1) and is highly dependent on the physical distance between CaV2.1 and synaptic vesicles (coupling). Although various active zone proteins are proposed to control coupling and abundance of CaV2.1 through direct interactions with the CaV2.1 α1 subunit C-terminus at the active zone, the role of these interaction partners is controversial. To define the intrinsic motifs that regulate coupling, we expressed mutant CaV2.1 α1 subunits on a CaV2.1 null background at the calyx of Held presynaptic terminal. Our results identified a region that directly controlled fast synaptic vesicle release and vesicle docking at the active zone independent of CaV2.1 abundance. In addition, proposed individual direct interactions with active zone proteins are insufficient for CaV2.1 abundance and coupling. Therefore, our work advances our molecular understanding of CaV2.1 regulation of neurotransmitter release in mammalian CNS synapses.>DOI:
机译:在中枢神经系统(CNS)突触中,动作电位诱发的神经递质释放主要由CaV2.1钙通道(CaV2.1)介导,并且高度依赖于CaV2.1与突触小泡之间的物理距离(耦合)。尽管提出了各种活性区蛋白来通过与活性区中CaV2.1α1亚基C末端的直接相互作用来控制CaV2.1的偶联和丰度,但这些相互作用伙伴的作用还是有争议的。为了定义调节偶联的内在基元,我们在Held突触前末端的花萼上的CaV2.1无效背景上表达了突变的CaV2.1α1亚基。我们的结果确定了一个区域,该区域直接控制突触小泡的快速释放和小泡停靠在独立于CaV2.1丰度的活性区。此外,建议的与活性区蛋白的直接相互作用不足以实现CaV2.1的丰度和偶联。因此,我们的工作提高了我们对哺乳动物CNS突触中CaV2.1调节神经递质释放的分子理解。> DOI:

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