4.0 Article

Endogenous Calcium Buffering at Photoreceptor Synaptic Terminals in Salamander Retina

期刊

SYNAPSE
卷 68, 期 11, 页码 518-528

出版社

WILEY
DOI: 10.1002/syn.21768

关键词

retina; photoreceptor; calcium buffering; added buffer; synapse; synaptic ribbon; calcium extrusion

资金

  1. NIH [EY10542]
  2. Senior Scientific Investigator Award from Research to Prevent Blindness, Fight for Sight

向作者/读者索取更多资源

Calcium operates by several mechanisms to regulate glutamate release at rod and cone synaptic terminals. In addition to serving as the exocytotic trigger, Ca2+ accelerates replenishment of vesicles in cones and triggers Ca2+-induced Ca2+ release (CICR) in rods. Ca2+ thereby amplifies sustained exocytosis, enabling photoreceptor synapses to encode constant and changing light. A complete picture of the role of Ca2+ in regulating synaptic transmission requires an understanding of the endogenous Ca2+ handling mechanisms at the synapse. We therefore used the added buffer approach to measure the endogenous Ca2+ binding ratio ((endo)) and extrusion rate constant () in synaptic terminals of photoreceptors in retinal slices from tiger salamander. We found that (endo) was similar in both cell types approximate to 25 and 50 in rods and cones, respectively. Using measurements of the decay time constants of Ca2+ transients, we found that was also similar, with values of approximate to 100 s(-1) and 160 s(-1) in rods and cones, respectively. The measurements of (endo) differ considerably from measurements in retinal bipolar cells, another ribbon-bearing class of retinal neurons, but are comparable to similar measurements at other conventional synapses. The values of are slower than at other synapses, suggesting that Ca2+ ions linger longer in photoreceptor terminals, supporting sustained exocytosis, CICR, and Ca2+-dependent ribbon replenishment. The mechanisms of endogenous Ca2+ handling in photoreceptors are thus well-suited for supporting tonic neurotransmission. Similarities between rod and cone Ca2+ handling suggest that neither buffering nor extrusion underlie differences in synaptic transmission kinetics. Synapse 68:518-528, 2014. (c) 2014 Wiley Periodicals, Inc.

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