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Ca2+、Mg2+和Na+在调节大鼠胰岛胰岛素释放中的相互作用。

Interactions of Ca2+, Mg2+, and Na+ in regulation of insulin release from rat islets.

作者信息

Janjic D, Wollheim C B

出版信息

Am J Physiol. 1983 Mar;244(3):E222-9. doi: 10.1152/ajpendo.1983.244.3.E222.

Abstract

The effects of glucose and ionic modifications on unidirectional Ca2+ efflux and insulin release has been studied. Rat pancreatic islets were isotopically equilibrated with 45Ca2+ for 2 days and then perifused at 10(-8) M Ca2+ to allow for strict interpretation of 45Ca2+ efflux. Under these conditions 16.7 mM glucose inhibited Ca2+ efflux but did not stimulate insulin release. Removal of Mg2+ from the buffer markedly stimulated Ca2+ efflux that was counteracted by glucose. The omission of Na+ decreased basal Ca2+ efflux by 30% at 10(-8) M Ca2+, thus demonstrating the importance of Na-Ca countertransport for Ca2+ extrusion. Like glucose, Na+ omission or the addition of ouabain attenuated Ca2+ efflux stimulated by Mg2+ removal. Glucose may interfere with Na-Ca countertransport because the actions of 16.7 mM glucose and Na+ omission were not additive. At 10(-8) M Ca2+, glucose elicited insulin release only when both 1) loss of cellular calcium was minimized by prior inhibition of Ca2+ efflux (Na+ omission or ouabain), and 2) Ca2+ mobilization was favored by Mg2+ removal. Under these conditions (in contrast to normal Ca2+), insulin release was not accompanied by increased Ca2+ efflux. Thus, unidirectional Ca2+ measurements do not permit the detection of Ca2+ mobilization in intact islets because glucose may concomitantly inhibit Ca2+ extrusion.

摘要

已经研究了葡萄糖和离子修饰对单向Ca2+外流及胰岛素释放的影响。将大鼠胰岛与45Ca2+进行同位素平衡2天,然后在10(-8)M Ca2+浓度下进行灌流,以便对45Ca2+外流进行严格的解释。在这些条件下,16.7 mM葡萄糖抑制Ca2+外流,但不刺激胰岛素释放。从缓冲液中去除Mg2+可显著刺激Ca2+外流,而葡萄糖可抵消这种刺激。在10(-8)M Ca2+浓度下,省略Na+可使基础Ca2+外流降低30%,从而证明了Na-Ca逆向转运对Ca2+外排的重要性。与葡萄糖一样,省略Na+或添加哇巴因可减弱因去除Mg2+而刺激的Ca2+外流。葡萄糖可能会干扰Na-Ca逆向转运,因为16.7 mM葡萄糖和省略Na+的作用并非相加的。在10(-8)M Ca2+浓度下,只有在以下两种情况同时存在时,葡萄糖才会引发胰岛素释放:1)通过事先抑制Ca2+外流(省略Na+或使用哇巴因)使细胞钙的流失最小化;2)去除Mg2+有利于Ca2+的动员。在这些条件下(与正常Ca2+情况相反),胰岛素释放并未伴随着Ca2+外流的增加。因此,单向Ca2+测量无法检测完整胰岛中的Ca2+动员情况,因为葡萄糖可能同时抑制Ca2+外排。

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