Otoferlin acts as a Ca2+ sensor for vesicle fusion and vesicle pool replenishment at auditory hair cell ribbon synapses

Nicolas Michalski(Inserm), Juan D. Goutman(Consejo Nacional de Investigaciones Científicas y Técnicas), Sarah M. Auclair(Yale University), Jacques Boutet de Monvel(Inserm), Margot Tertrais(Université de Bordeaux), Alice Emptoz(Inserm), Alexandre Parrin(Inserm), Sylvie Nouaille(Inserm), Marc Guillon(Délégation Paris 5), Martin Sachse(Institut Pasteur), Danica Ćirić(Inserm), Amel Bahloul(Centre National de la Recherche Scientifique), Jean‐Pierre Hardelin(Inserm), R. Bryan Sutton(Texas Tech University), Paul Avan(Inserm), Shyam S. Krishnakumar(Yale University), James E. Rothman(Yale University), Didier Dulon(Université de Bordeaux), Saaïd Safieddine(Centre National de la Recherche Scientifique), Christine Petit(Institut de la Vision)
eLife
November 7, 2017
Cited by 146Open Access
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Abstract

Hearing relies on rapid, temporally precise, and sustained neurotransmitter release at the ribbon synapses of sensory cells, the inner hair cells (IHCs). This process requires otoferlin, a six C2-domain, Ca2+-binding transmembrane protein of synaptic vesicles. To decipher the role of otoferlin in the synaptic vesicle cycle, we produced knock-in mice (Otof Ala515,Ala517/Ala515,Ala517) with lower Ca2+-binding affinity of the C2C domain. The IHC ribbon synapse structure, synaptic Ca2+ currents, and otoferlin distribution were unaffected in these mutant mice, but auditory brainstem response wave-I amplitude was reduced. Lower Ca2+ sensitivity and delay of the fast and sustained components of synaptic exocytosis were revealed by membrane capacitance measurement upon modulations of intracellular Ca2+ concentration, by varying Ca2+ influx through voltage-gated Ca2+-channels or Ca2+ uncaging. Otoferlin thus functions as a Ca2+ sensor, setting the rates of primed vesicle fusion with the presynaptic plasma membrane and synaptic vesicle pool replenishment in the IHC active zone.


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