Literature DB >> 33664131

Synaptophysin Regulates Fusion Pores and Exocytosis Mode in Chromaffin Cells.

Che-Wei Chang1,2, Yu-Tien Hsiao3, Meyer B Jackson3,2.   

Abstract

Synaptophysin (syp) is a major integral membrane protein of secretory vesicles. Previous work has demonstrated functions for syp in synaptic vesicle cycling, endocytosis, and synaptic plasticity, but the role of syp in the process of membrane fusion during Ca2+-triggered exocytosis remains poorly understood. Furthermore, although syp resides on both large dense-core and small synaptic vesicles, its role in dense-core vesicle function has received less attention compared to synaptic vesicle function. To explore the role of syp in membrane fusion and dense-core vesicle function, we used amperometry to measure catecholamine release from single vesicles in male and female mouse chromaffin cells with altered levels of syp and the related tetraspanner protein synaptogyrin (syg). Knocking out syp slightly reduced the frequency of vesicle fusion events below wild-type levels, but knocking out both syp and syg reduced the frequency two-fold. Knocking out both proteins stabilized initial fusion pores, promoted fusion pore closure (kiss-and-run), and reduced late-stage fusion pore expansion. Introduction of a syp construct lacking its C-terminal dynamin-binding domain in syp knock-outs increased the duration and fraction of kiss-and-run events, increased total catecholamine release per event, and reduced late-stage fusion pore expansion. These results demonstrated that syp and syg regulate dense-core vesicle function at multiple stages to initiate fusion, control the choice of mode between full fusion and kiss-and-run, and influence the dynamics of both initial and late-stage fusion pores. The transmembrane domain influences small initial fusion pores, and the C-terminal domain influences large late-stage fusion pores, possibly through an interaction with dynamin.SIGNIFICANCE STATEMENT:The secretory vesicle protein synaptophysin is known to function in synaptic vesicle cycling, but its roles in dense-core vesicle functions, and in controlling membrane fusion during Ca2+-triggered exocytosis remain unclear. The present study used amperometry recording of catecholamine release from endocrine cells to assess the impact of synaptophysin and related proteins on membrane fusion. A detailed analysis of amperometric spikes arising from the exocytosis of single vesicles showed that these proteins influence fusion pores at multiple stages and control the choice between kiss-and-run and full fusion. Experiments with a synaptophysin construct lacking its C-terminus indicated that the transmembrane domain influences the initial fusion pore, while the C-terminal domain influences later stages after fusion pore expansion.
Copyright © 2021 the authors.

Entities:  

Year:  2021        PMID: 33664131      PMCID: PMC8055083          DOI: 10.1523/JNEUROSCI.2833-20.2021

Source DB:  PubMed          Journal:  J Neurosci        ISSN: 0270-6474            Impact factor:   6.167


  72 in total

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10.  Structural transitions in the synaptic SNARE complex during Ca2+-triggered exocytosis.

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  3 in total

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