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突触结合蛋白-1和突触结合蛋白-7依赖的融合机制将突触小泡靶向动力学上不同的内吞途径。

Synaptotagmin-1- and Synaptotagmin-7-Dependent Fusion Mechanisms Target Synaptic Vesicles to Kinetically Distinct Endocytic Pathways.

作者信息

Li Ying C, Chanaday Natali L, Xu Wei, Kavalali Ege T

机构信息

Department of Neuroscience, University of Texas Southwestern Medical Center, Dallas, TX 75390-9111, USA.

Department of Neuroscience, University of Texas Southwestern Medical Center, Dallas, TX 75390-9111, USA.

出版信息

Neuron. 2017 Feb 8;93(3):616-631.e3. doi: 10.1016/j.neuron.2016.12.010. Epub 2017 Jan 19.

Abstract

Synaptic vesicle recycling is essential for maintaining normal synaptic function. The coupling of exocytosis and endocytosis is assumed to be Ca dependent, but the exact role of Ca and its key effector synaptotagmin-1 (syt1) in regulation of endocytosis is poorly understood. Here, we probed the role of syt1 in single- as well as multi-vesicle endocytic events using high-resolution optical recordings. Our experiments showed that the slowed endocytosis phenotype previously reported after syt1 loss of function can also be triggered by other manipulations that promote asynchronous release such as Sr substitution and complexin loss of function. The link between asynchronous release and slowed endocytosis was due to selective targeting of fused synaptic vesicles toward slow retrieval by the asynchronous release Ca sensor synaptotagmin-7. In contrast, after single synaptic vesicle fusion, syt1 acted as an essential determinant of synaptic vesicle endocytosis time course by delaying the kinetics of vesicle retrieval in response to increasing Ca levels.

摘要

突触囊泡循环对于维持正常的突触功能至关重要。胞吐作用和内吞作用的偶联被认为是依赖于钙的,但钙及其关键效应分子突触结合蛋白-1(syt1)在调节内吞作用的确切作用仍知之甚少。在这里,我们使用高分辨率光学记录探究了syt1在单囊泡和多囊泡内吞事件中的作用。我们的实验表明,先前报道的syt1功能丧失后出现的内吞作用减慢表型,也可由其他促进异步释放的操作触发,如锶替代和结合蛋白功能丧失。异步释放与内吞作用减慢之间的联系是由于异步释放钙传感器突触结合蛋白-7将融合的突触囊泡选择性地导向缓慢回收。相反,在单个突触囊泡融合后,syt1通过响应钙水平升高延迟囊泡回收动力学,成为突触囊泡内吞作用时间进程的关键决定因素。

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