Synaptic vesicle release during ribbon synapse formation of cone photoreceptors.

Front Cell Neurosci

Division of Animal Physiology/Neurobiology, Department of Biology, Friedrich-Alexander-Universität Erlangen-Nürnberg, Erlangen, Germany.

Published: November 2022

AI Article Synopsis

  • Mammalian cone photoreceptors rely on synaptic ribbons to effectively transmit visual signals to second-order retinal neurons, though their precise role is still unclear.
  • In developing mice, synaptic ribbons start as free-floating structures that elongate and attach to the active zone in photoreceptor terminals over time.
  • Research indicates that while synaptic ribbons don't influence voltage-sensitive Ca channels or release probability, they enhance synaptic vesicle density, increase readily releasable vesicle pools, promote vesicle replenishment, and improve the Ca-sensitivity of glutamate release.

Article Abstract

Mammalian cone photoreceptors enable through their sophisticated synapse the high-fidelity transfer of visual information to second-order neurons in the retina. The synapse contains a proteinaceous organelle, called the synaptic ribbon, which tethers synaptic vesicles (SVs) at the active zone (AZ) close to voltage-gated Ca channels. However, the exact contribution of the synaptic ribbon to neurotransmission is not fully understood, yet. In mice, precursors to synaptic ribbons appear within photoreceptor terminals shortly after birth as free-floating spherical structures, which progressively elongate and then attach to the AZ during the following days. Here, we took advantage of the process of synaptic ribbon maturation to study their contribution to SV release. We performed whole-cell patch-clamp recordings from cone photoreceptors at three postnatal (P) development stages (P8-9, P12-13, >P30) and measured evoked SV release, SV replenishment rate, recovery from synaptic depression, domain organization of voltage-sensitive Ca channels, and Ca-sensitivity of exocytosis. Additionally, we performed electron microscopy to determine the density of SVs at ribbon-free and ribbon-occupied AZs. Our results suggest that ribbon attachment does not organize the voltage-sensitive Ca channels into nanodomains or control SV release probability. However, ribbon attachment increases SV density at the AZ, increases the pool size of readily releasable SVs available for evoked SV release, facilitates SV replenishment without changing the SV pool refilling time, and increases the Ca- sensitivity of glutamate release.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC9672513PMC
http://dx.doi.org/10.3389/fncel.2022.1022419DOI Listing

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