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依赖于突触融合蛋白-1、Munc18-1 和 Munc13-1 的少数神经元 SNARE 介导的脂质体融合。

Synaptotagmin-1-, Munc18-1-, and Munc13-1-dependent liposome fusion with a few neuronal SNAREs.

机构信息

Department of Biophysics, University of Texas Southwestern Medical Center, Dallas, TX 75390.

Department of Biochemistry, University of Texas Southwestern Medical Center, Dallas, TX 75390.

出版信息

Proc Natl Acad Sci U S A. 2021 Jan 26;118(4). doi: 10.1073/pnas.2019314118.

Abstract

Neurotransmitter release is governed by eight central proteins among other factors: the neuronal SNAREs syntaxin-1, synaptobrevin, and SNAP-25, which form a tight SNARE complex that brings the synaptic vesicle and plasma membranes together; NSF and SNAPs, which disassemble SNARE complexes; Munc18-1 and Munc13-1, which organize SNARE complex assembly; and the Ca sensor synaptotagmin-1. Reconstitution experiments revealed that Munc18-1, Munc13-1, NSF, and α-SNAP can mediate Ca-dependent liposome fusion between synaptobrevin liposomes and syntaxin-1-SNAP-25 liposomes, but high fusion efficiency due to uncontrolled SNARE complex assembly did not allow investigation of the role of synaptotagmin-1 on fusion. Here, we show that decreasing the synaptobrevin-to-lipid ratio in the corresponding liposomes to very low levels leads to inefficient fusion and that synaptotagmin-1 strongly stimulates fusion under these conditions. Such stimulation depends on Ca binding to the two C domains of synaptotagmin-1. We also show that anchoring SNAP-25 on the syntaxin-1 liposomes dramatically enhances fusion. Moreover, we uncover a synergy between synaptotagmin-1 and membrane anchoring of SNAP-25, which allows efficient Ca-dependent fusion between liposomes bearing very low synaptobrevin densities and liposomes containing very low syntaxin-1 densities. Thus, liposome fusion in our assays is achieved with a few SNARE complexes in a manner that requires Munc18-1 and Munc13-1 and that depends on Ca binding to synaptotagmin-1, all of which are fundamental features of neurotransmitter release in neurons.

摘要

神经递质的释放受八种核心蛋白控制,此外还有其他因素:神经元 SNARE 蛋白突触融合蛋白 1、融合衔接蛋白和 SNAP-25,它们形成紧密的 SNARE 复合体,使突触囊泡和质膜靠近; NSF 和 SNAPs,它们使 SNARE 复合体解体;Munc18-1 和 Munc13-1,它们组织 SNARE 复合体的组装;以及钙传感器突触融合蛋白 1。重建实验表明,Munc18-1、Munc13-1、NSF 和 α-SNAP 可以介导融合衔接蛋白囊泡和突触融合蛋白 1-SNAP-25 囊泡之间的 Ca 依赖性脂质体融合,但由于 SNARE 复合体组装不受控制,融合效率很高,无法研究突触融合蛋白 1 对融合的作用。在这里,我们表明,将相应脂质体中的融合衔接蛋白与脂质的比例降低到非常低的水平会导致融合效率降低,而突触融合蛋白 1 在这些条件下强烈刺激融合。这种刺激依赖于 Ca 结合到突触融合蛋白 1 的两个 C 结构域。我们还表明,将 SNAP-25 锚定在突触融合蛋白 1 脂质体上可显著增强融合。此外,我们发现突触融合蛋白 1 和 SNAP-25 的膜锚定之间存在协同作用,这使得具有非常低的融合衔接蛋白密度的脂质体和含有非常低的突触融合蛋白 1 密度的脂质体之间能够有效地进行 Ca 依赖性融合。因此,我们的实验中脂质体融合是通过几种 SNARE 复合体实现的,这种方式需要 Munc18-1 和 Munc13-1,并且依赖于 Ca 与突触融合蛋白 1 的结合,所有这些都是神经元中神经递质释放的基本特征。

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