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Abstract
The mechanism by which extracellular ATP stimulates insulin secretion was investigated in RINm5F cells. ATP depolarized the cells as demonstrated both by using the patch-clamp technique and a fluorescent probe. The depolarization is due to closure of ATP-sensitive K+ channels as shown directly in outside-out membrane patches. ATP also raised cytosolic Ca2+ [( Ca2+]i). At the single cell level the latency of the [Ca2+]i response was inversely related to ATP concentration. The [Ca2+]i rise is due both to inositol trisphosphate mediated Ca2+ mobilization and to Ca2+ influx. The former component, as well as inositol trisphosphate generation, were inhibited by phorbol myristate acetate which uncouples agonist receptors from phospholipase C. This manoeuvre did not block Ca2+ influx or membrane depolarization. Diazoxide, which opens ATP-sensitive K+ channels, attenuated membrane depolarization and part of the Ca2+ influx stimulated by ATP. However, the main Ca2+ influx component was unaffected by L-type channel blockers, suggesting the activation of other Ca2+ conductance pathways. ATP increased the rate of insulin secretion by more than 12-fold but the effect was transient. Prolonged exposure to EGTA dissociated the [Ca2+]i rise from ATP-induced insulin secretion, since the former was abolished and the latter only decreased by about 60%. In contrast, vasopressin-evoked insulin secretion was more sensitive to Ca2+ removal than the accompanying [Ca2+]i rise. Inhibition of phospholipase C stimulation by phorbol myristate acetate abrogated vasopressin but only reduced ATP-induced insulin secretion by 34%. These results suggest that ATP stimulates insulin release by both phospholipase C dependent and distinct mechanisms. The Ca2+)-independent component of insulin secretion points to a direct triggering of exocytosis by ATP.
Highlights
The mechanism by which extracellular ATP stimu- Extracellular ATP can be considered as a neurotransmitter, lates insulin secretion was investigated in RINm5F since it is released from nerve endings of different types [1]
The Ca2+-independentcomponent of inpresent work we have investigated the mechanism involved in ATP-induced insulin secretion in the RINmSF cell line
The stimulation of insulin secretion is mediated by several intracellular messenger pathways
Summary
Tinuousstretches of data(filtered a t 1 kHz (low pass)),lasting between and 20 s. When ATP was added 2 min their effects on [Ca2+]iwere measured at various times after after PMA, there was still a clear albeit small increase in the addition of EGTA to thecell suspensions (Fig. 6). All cells responded to the agonist, albeit with different pat- action of ATP, we employed diazoxide, whichattenuates the terns.In general, at low concentrations ATP provoked a membrane depolarization (cf Fig. 3c). In view of the failure for 10, 50, and 250 p~ ATP, respectively) and ATP caused a of diazoxide to lower the [CaZ+]r,ise due to ATP measured in [Ca"'], rise which was characterized by a broadening of the cell suspensions (Table I), it can be concluded that the voltpeak with a tendency of increasing amplitude Single [Ca2+Itiransients lastingless than 20 s with peak values To examine the dependence of ATP induced insulin secrenot exceeding 300nM (not shown)
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