AI Article Synopsis

  • Munc18-1 and syntaxin-1A are essential for the process of neuroexocytosis in neurons, and their organization in specific areas on the cell membrane is crucial for vesicle fusion.
  • A mutant form of Munc18-1 that lacks certain residues leads to increased docking time of secretory vesicles, indicating the importance of its structure in facilitating vesicle fusion.
  • Changes in the movement of Munc18-1 and syntaxin-1A in response to stimulation suggest that a specific region of Munc18-1 regulates the engagement of syntaxin-1A in forming SNARE complexes, which are necessary for the release of neurotransmitters.

Article Abstract

Munc18-1 and syntaxin-1A control SNARE-dependent neuroexocytosis and are organized in nanodomains on the plasma membrane of neurons and neurosecretory cells. Deciphering the intra- and intermolecular steps via which they prepare secretory vesicles (SVs) for fusion is key to understanding neuronal and hormonal communication. Here, we demonstrate that expression of a priming-deficient mutant lacking 17 residues of the domain 3a hinge-loop (Munc18-1(Δ317-333)) in PC12 cells engineered to knockdown Munc18-1/2 markedly prolonged SV docking. Single-molecule analysis revealed nonhomogeneous diffusion of Munc18-1 and syntaxin-1A in and out of partially overlapping nanodomains. Whereas Munc18-1(WT) mobility increased in response to stimulation, syntaxin-1A became less mobile. These Munc18-1 and syntaxin-1A diffusional switches were blocked by the expression of Munc18-1(Δ317-333), suggesting that a conformational change in the Munc18-1 hinge-loop controls syntaxin-1A and subsequent SNARE complex assembly. Accordingly, syntaxin-1A confinement was prevented by expression of botulinum neurotoxin type E. The Munc18-1 domain 3a hinge-loop therefore controls syntaxin-1A engagement into SNARE complex formation during priming.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5037406PMC
http://dx.doi.org/10.1083/jcb.201508118DOI Listing

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