4.7 Article

Synaptotagmin2 (Syt2) Drives Fast Release Redundantly with Syt1 at the Output Synapses of Parvalbumin-Expressing Inhibitory Neurons

Journal

JOURNAL OF NEUROSCIENCE
Volume 37, Issue 17, Pages 4604-4617

Publisher

SOC NEUROSCIENCE
DOI: 10.1523/JNEUROSCI.3736-16.2017

Keywords

calcium sensor; inhibitory synapse; neurotransmitter release; optogenetics; parvalbumin interneuron; synaptotagmin

Categories

Funding

  1. Swiss National Science Foundation [310030B_156934/1]
  2. National Competence Center for Research
  3. German Research Foundation (DFG) [SCHN 451/5-2]
  4. Swiss National Science Foundation (SNF) [310030B_156934] Funding Source: Swiss National Science Foundation (SNF)

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Parvalbumin-expressing inhibitory neurons in the mammalian CNS are specialized for fast transmitter release at their output synapses. However, the Ca2+ sensor(s) used by identified inhibitory synapses, including the output synapses of parvalbumin-expressing inhibitory neurons, have only recently started to be addressed. Here, we investigated the roles of Syt1 and Syt2 at two types of fast-releasing inhibitory connections in the mammalian CNS: the medial nucleus of the trapezoid body to lateral superior olive glycinergic synapse, and the basket/stellate cell-Purkinje GABAergic synapse in the cerebellum. We used conditional and conventional knock-out (KO) mouse lines, with viral expression of Cre-recombinase and a light-activated ion channel for optical stimulation of the transduced fibers, to produce Syt1-Syt2 double KO synapses in vivo. Surprisingly, we found that KO of Syt2 alone had only minor effects on evoked transmitter release, despite the clear presence of the protein in inhibitory nerve terminals revealed by immunohistochemistry. We show that Syt1 is weakly coexpressed at these inhibitory synapses and must be genetically inactivated together with Syt2 to achieve a significant reduction and desynchronization of fast release. Thus, our work identifies the functionally relevant Ca2+ sensor(s) at fast-releasing inhibitory synapses and shows that two major Syt isoforms can cooperate to mediate release at a given synaptic connection.

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