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N型钙通道与突触核心复合体的钙依赖性相互作用。

Calcium-dependent interaction of N-type calcium channels with the synaptic core complex.

作者信息

Sheng Z H, Rettig J, Cook T, Catterall W A

机构信息

Department of Pharmacology, University of Washington, Seattle 98195-7280, USA.

出版信息

Nature. 1996 Feb 1;379(6564):451-4. doi: 10.1038/379451a0.

Abstract

Neurotransmitter release is initiated by influx of Ca2+ through voltage-gated Ca2+ channels, within 200 microseconds of the action potential arriving at the synaptic terminal, as the Ca2+ concentration increases from 100 nM to > 200 microM. Exocytosis requires high Ca2+ concentration, with a threshold of 20-50 microM and half-maximal activation at 190 microM. The synaptic membrane proteins syntaxin, 25K synaptosome-associated protein (SNAP25), and vesicle-associated membrane protein (VAMP)/synaptobrevin, are thought to form a synaptic core complex which mediates vesicle docking and membrane fusion. Synaptotagmin may be the low-affinity Ca(2+)-sensor, but other Ca(2+)-sensors are involved as residual neurotransmission persists in synaptotagmin-null mutants. Syntaxin binds to N-type Ca2+ channels at a site in the intracellular loop connecting domains II and III. Here we describe Ca(2+)-dependent interaction of this site with syntaxin and SNAP25 which has a biphasic dependence on Ca2+, with maximal binding at 20 microM free Ca2+, near the threshold for transmitter release. Ca(2+)-dependent interaction of Ca2+ channels with the synaptic core complex may be important for Ca(2+)-dependent docking and fusion of synaptic vesicles.

摘要

神经递质的释放是由动作电位到达突触末端后200微秒内,通过电压门控Ca2+通道流入Ca2+引发的,此时Ca2+浓度从100 nM增加到>200 μM。胞吐作用需要高Ca2+浓度,阈值为20 - 50 μM,半最大激活浓度为190 μM。突触膜蛋白 syntaxin、25K突触体相关蛋白(SNAP25)和囊泡相关膜蛋白(VAMP)/突触小泡蛋白,被认为形成了一个突触核心复合体,介导囊泡对接和膜融合。突触结合蛋白可能是低亲和力Ca(2+)传感器,但其他Ca(2+)传感器也参与其中,因为在突触结合蛋白缺失的突变体中仍存在残余的神经传递。Syntaxin在连接结构域II和III的细胞内环中的一个位点与N型Ca2+通道结合。在此我们描述了该位点与 syntaxin和SNAP25的Ca(2+)依赖性相互作用,其对Ca2+具有双相依赖性,在游离Ca2+浓度为20 μM时结合力最大,接近递质释放的阈值。Ca2+通道与突触核心复合体的Ca(2+)依赖性相互作用可能对突触小泡的Ca(2+)依赖性对接和融合很重要。

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