Publication | Open Access
Fusion pore formation and expansion induced by Ca <sup>2+</sup> and synaptotagmin 1
103
Citations
25
References
2013
Year
Protein SecretionMolecular BiologyCytoskeletonNeurotransmissionCellular NeurobiologySynaptic SignalingCellular PhysiologyContent MixingMembrane TransportSecretory PathwayBiophysicsFusion Pore FormationMolecular NeuroscienceBiochemistryCell TraffickingMembrane BiologyProtein TransportCell BiologyPore ExpansionSynaptic PlasticitySignal TransductionNatural SciencesIntracellular TraffickingMedicine
Fusion pore formation and expansion, crucial steps for neurotransmitter release and vesicle recycling in soluble N-ethylmaleimide-sensitive factor attachment protein receptor (SNARE)-dependent vesicle fusion, have not been well studied in vitro due to the lack of a reliable content-mixing fusion assay. Using methods detecting the intervesicular mixing of small and large cargoes at a single-vesicle level, we found that the neuronal SNARE complexes have the capacity to drive membrane hemifusion. However, efficient fusion pore formation and expansion require synaptotagmin 1 and Ca(2+). Real-time measurements show that pore expansion detected by content mixing of large DNA cargoes occurs much slower than initial pore formation that transmits small cargoes. Slow pore expansion perhaps provides a time window for vesicles to escape the full collapse fusion pathway via alternative mechanisms such as kiss-and-run. The results also show that complexin 1 stimulates pore expansion significantly, which could put bias between two pathways of vesicle recycling.
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