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1. A combination of patch-clamp, amperometric and fluorimetric methods were used to investigate the Ca2+ dependence and kinetics of secretion from pancreatic beta-cells elicited by voltage-gated Ca2+ entry. 2. Whether measured by the change in cell capacitance or by amperometric detection of 5-hydroxytryptamine (5-HT) release, the voltage dependence of the amount of secretion mirrored that of both the peak Ca2+ current and Ca2+ entry. 3. The magnitude of secretion elicited by a single pulse could be entirely accounted for by a readily releasable pool of approximately 200 vesicles. Neither depression nor potentiation of release was observed with 0.1 Hz pulse trains. 4. Transient amperometric currents were detected, which occurred independently of each other and were attributed to the fusion of single vesicles. 5. The time course of the macroscopic amperometric current could be accurately reconstructed by convolution of the all-events latency distribution and the unitary amperometric current. 6. In response to membrane depolarisation, secretion was initiated with a variable latency: approximately 95 % of the first secretory events occurred at least 50 ms after the start of the voltage pulse (and Ca2+ influx). Secretion fell rapidly on membrane repolarisation, even though the average intracellular calcium concentration ([Ca2+]i) was still elevated. 7. The [Ca2+] in the locality of the release site was estimated from the all-events latency distribution. [Ca2+] rose during a voltage pulse and secretion was elicited at > 0.4 microM and peaked at approximately 2-10 microM.

Type

Journal article

Journal

J Physiol

Publication Date

15/12/1999

Volume

521 Pt 3

Pages

651 - 664

Keywords

Algorithms, Animals, Calcium, Calcium Signaling, Electric Stimulation, Electrophysiology, Exocytosis, In Vitro Techniques, Islets of Langerhans, Kinetics, Membrane Potentials, Mice, Patch-Clamp Techniques, Serotonin