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钠钙交换通过改变细胞内钙储存量来调节人血小板的钙处理。

Na(+)-Ca2+ exchange modulates Ca2+ handling of human platelets by altering intracellular Ca2+ store size.

作者信息

Ishida T, Matsuura H, Ishida-Kainouchi M, Ozono R, Watanabe M, Kajiyama G, Oshima T

机构信息

First Department of Internal Medicine, Hiroshima University School of Medicine, Japan.

出版信息

J Hypertens. 1993 Oct;11(10):1089-95. doi: 10.1097/00004872-199310000-00013.

Abstract

OBJECTIVE

In order to elucidate the role of Na(+)-Ca2+ exchange in regulating cytosolic free Ca2+ concentration in human platelets, we investigated the relationship between cytosolic free Na+ and Ca2+ concentrations in human platelets.

METHODS

Sodium-binding benzofuran isophthalate and fura-2 were used to monitor cytosolic free Na+ and Ca2+ concentrations, respectively.

RESULTS

Ouabain at a concentration of 100 mumol/l induced an increase in cytosolic free Na+ concentration within 5 min, followed by increases in resting cytosolic free Ca2+ concentration and intracellular Ca2+ store. These three parameters were increased in a time-dependent manner significantly above the timed control over a period of 60 min. Pre-incubation of platelets with 100 mumol/l ouabain for 30 min significantly enhanced the cytosolic free Ca2+ response to thrombin and arginine vasopressin in the absence of extracellular Ca2+. The decrease from peak cytosolic free Ca2+ concentration in response to ionomycin in the absence of extracellular Ca2+ was significantly slower in low-Na+ buffer than in standard buffer. In addition, 5 mumol/ionomycin increased the cytosolic free Na+ concentration markedly in the presence of 0.1 mmol/l extracellular Ca2+, but the rise in cytosolic free Na+ concentration was suppressed by 2 mmol/l Ni2+ (NiCl2) or by removal of extracellular Ca2+.

CONCLUSIONS

These results suggest that Na(+)-Ca2+ exchange is important in extruding Ca2+ from the cytosol in human platelets, and inhibition of this exchange leads to the accumulation of intracellular Ca2+ store, which may be responsible for the enhanced responsiveness of cytosolic free Ca2+ to agonists.

摘要

目的

为了阐明钠钙交换在调节人血小板胞浆游离钙浓度中的作用,我们研究了人血小板胞浆游离钠浓度与钙浓度之间的关系。

方法

分别使用钠结合苯并呋喃间苯二甲酸酯和fura-2监测胞浆游离钠浓度和钙浓度。

结果

浓度为100μmol/l的哇巴因在5分钟内可诱导胞浆游离钠浓度升高,随后静息胞浆游离钙浓度和细胞内钙储存增加。在60分钟内,这三个参数均呈时间依赖性增加,显著高于同期的时间对照。在无细胞外钙的情况下,将血小板与100μmol/l哇巴因预孵育30分钟可显著增强对凝血酶和精氨酸加压素的胞浆游离钙反应。在无细胞外钙的情况下,低钠缓冲液中离子霉素引起的胞浆游离钙浓度峰值下降明显慢于标准缓冲液。此外,在存在0.1mmol/l细胞外钙的情况下,5μmol/离子霉素可显著增加胞浆游离钠浓度,但2mmol/l Ni2+(NiCl2)或去除细胞外钙可抑制胞浆游离钠浓度的升高。

结论

这些结果表明钠钙交换在人血小板中将钙从胞浆中挤出的过程中很重要,抑制这种交换会导致细胞内钙储存积累,这可能是胞浆游离钙对激动剂反应增强的原因。

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