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哺乳动物神经递质释放位点上 Aczonin/Piccolo 及其相关蛋白的分子原位拓扑结构。

Molecular in situ topology of Aczonin/Piccolo and associated proteins at the mammalian neurotransmitter release site.

机构信息

Department of Neuroscience, Uppsala University, S-75124 Uppsala, Sweden.

出版信息

Proc Natl Acad Sci U S A. 2011 Aug 2;108(31):E392-401. doi: 10.1073/pnas.1101707108. Epub 2011 Jun 28.

DOI:10.1073/pnas.1101707108
PMID:21712437
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3150911/
Abstract

The protein machinery of neurotransmitter exocytosis requires efficient orchestration in space and time, for speed and precision of neurotransmission and also for synaptic ontogeny and plasticity. However, its spatial organization in situ is virtually unknown. Aczonin/Piccolo is a putative organizer protein of mammalian active zones. We determined by immunogold electron microscopy (EM) (i) the spatial arrangement (i.e., topology) of 11 segments of the Aczonin polypeptide in situ, and correlated it to (ii) the positioning of Aczonin-interacting domains of Bassoon, CAST/ELKS, Munc13, and RIM and (iii) the ultrastructurally defined presynaptic macromolecular aggregates known as dense projections and synaptic ribbons. At conventional synapses, Aczonin assumes a compact molecular topology within a layer 35 to 80 nm parallel to the plasma membrane (PM), with a "trunk" sitting on the dense projection top and a C-terminal "arm" extending down toward the PM and sideward to the dense projection periphery. At ribbon synapses, Aczonin occupies the whole ribbon area. Bassoon colocalizes with Aczonin at conventional synapses but not at ribbon synapses. At both conventional and ribbon synapses, CAST, Munc13, and RIM are segregated from Aczonin, closer to the PM, and Aczonin is positioned such that it may control the access of neurotransmitter vesicles to the fusion site.

摘要

神经递质胞吐的蛋白质机器需要在空间和时间上进行有效的协调,以实现神经传递的速度和精度,以及突触的发生和可塑性。然而,其在原位的空间组织实际上是未知的。Aczonin/Piccolo 是哺乳动物活性区的假定组织者蛋白。我们通过免疫金电子显微镜 (EM) 确定了(i)Aczonin 多肽的 11 个片段在原位的空间排列(即拓扑结构),并将其与(ii)Bassoon、CAST/ELKS、Munc13 和 RIM 的 Aczonin 相互作用域的定位以及(iii)超微结构定义的称为致密突起和突触带的前突触大分子聚集体相关联。在常规突触中,Aczonin 采用与质膜 (PM) 平行的 35 至 80nm 厚的层内紧凑的分子拓扑结构,“主干”位于致密突起的顶部,C 端“臂”向下延伸至 PM 并向致密突起的周边侧向延伸。在带状突触中,Aczonin 占据整个带状区域。Bassoon 在常规突触中与 Aczonin 共定位,但在带状突触中不共定位。在常规和带状突触中,CAST、Munc13 和 RIM 与 Aczonin 分离,更靠近 PM,并且 Aczonin 的定位可以控制神经递质囊泡到达融合位点的通道。

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