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豚鼠结肠平滑肌中的钙离子调节:钠钙交换体和肌浆网的作用

Ca(2+) regulation in guinea-pig colonic smooth muscle: the role of the Na(+)-Ca(2+) exchanger and the sarcoplasmic reticulum.

作者信息

Bradley Karen N, Flynn Elaine R M, Muir Thomas C, McCarron John G

机构信息

Institute of Biomedical and Life Sciences, Neuroscience and Biomedical Systems, West Medical Building, University of Glasgow, Glasgow G12 8QQ, UK.

出版信息

J Physiol. 2002 Jan 15;538(Pt 2):465-82. doi: 10.1113/jphysiol.2001.013039.

Abstract

To study the contribution of the Na(+)-Ca(2+) exchanger to Ca(2+) regulation and its interaction with the sarcoplasmic reticulum (SR), changes in cytoplasmic Ca(2+) concentration (Ca(2+)) were measured in single, voltage clamped, smooth muscle cells. Increases in Ca(2+) were evoked by either depolarisation (-70 mV to 0 mV) or by release from the SR by caffeine (10 mM) or flash photolysis of caged InsP(3) (InsP(3)). Depletion of the SR of Ca(2+) (verified by the absence of a response to caffeine and InsP(3)) by either ryanodine (50 microM), to open the ryanodine receptors (RyRs), or thapsigargin (500 nM) or cyclopiazonic acid (CPA, 10 microM), to inhibit the SR Ca(2+) pumps, reduced neither the magnitude of the Ca(2+) transient nor the relationship between the influx of and the rise in Ca(2+) evoked by depolarisation. This suggested that Ca(2+)-induced Ca(2+) release (CICR) from the SR did not contribute significantly to the depolarisation-evoked rise in Ca(2+). However, although Ca(2+) was not released from it, the SR accumulated the ion following depolarisation since ryanodine and thapsigargin each slowed the rate of decline of the depolarisation-evoked Ca(2+) transient. Indeed, the SR Ca(2+) content increased following depolarisation as assessed by the increased magnitude of the Ca(2+) levels evoked each by InsP(3) and caffeine, relative to controls. The increased SR Ca(2+) content following depolarisation returned to control values in approximately 12 min via Na(+)-Ca(2+) exchanger activity. Thus inhibition of the Na(+)-Ca(2+) exchanger by removal of external Na(+) (by either lithium or choline substitution) prevented the increased SR Ca(2+) content from returning to control levels. On the other hand, the Na(+)-Ca(2+) exchanger did not appear to regulate bulk average Ca(2+) directly since the rates of decline in Ca(2+), following either depolarisation or the release of Ca(2+) from the SR (by either InsP(3) or caffeine), were neither voltage nor Na(+) dependent. Thus, no evidence for short term (seconds) control of Ca(2+) by the Na(+)-Ca(2+) exchanger was found. Together, the results suggest that despite the lack of CICR, the SR removes Ca(2+) from the cytosol after its elevation by depolarisation. This Ca(2+) is then removed from the SR to outside the cell by the Na(+)-Ca(2+) exchanger. However, the exchanger does not contribute significantly to the decline in bulk average Ca(2+) following transient elevations in the ion produced either by depolarisation or by release from the store.

摘要

为研究钠钙交换体对钙离子调节的作用及其与肌浆网(SR)的相互作用,在单个电压钳制的平滑肌细胞中测量了细胞质钙离子浓度([Ca²⁺]c)的变化。[Ca²⁺]c的升高可通过去极化(从 -70 mV 到 0 mV)或通过咖啡因(10 mM)从 SR 释放钙离子或通过笼锁肌醇三磷酸(InsP₃)的闪光光解来诱发。通过使用ryanodine(50 μM)打开ryanodine受体(RyRs),或使用毒胡萝卜素(500 nM)或环匹阿尼酸(CPA,10 μM)抑制 SR 钙泵,使 SR 中的钙离子耗尽(通过对咖啡因和 InsP₃ 无反应来验证),这既没有降低钙离子瞬变的幅度,也没有改变去极化诱发的[Ca²⁺]c 升高与钙离子内流之间的关系。这表明 SR 的钙诱导钙释放(CICR)对去极化诱发的[Ca²⁺]c 升高没有显著贡献。然而,尽管没有从 SR 释放钙离子,但去极化后 SR 积累了离子,因为 ryanodine 和毒胡萝卜素各自减慢了去极化诱发的钙离子瞬变的下降速率。实际上,通过 InsP₃ 和咖啡因诱发的[Ca²⁺]c 水平升高幅度相对于对照增加,表明去极化后 SR 钙含量增加。去极化后增加的 SR 钙含量通过钠钙交换体活性在大约 12 分钟内恢复到对照值。因此,通过去除外部钠离子(用锂或胆碱替代)抑制钠钙交换体可阻止增加的 SR 钙含量恢复到对照水平。另一方面,钠钙交换体似乎并不直接调节总体平均钙离子浓度,因为去极化或 SR 释放钙离子(通过 InsP₃ 或咖啡因)后[Ca²⁺]c 的下降速率既不依赖电压也不依赖钠离子。因此,未发现钠钙交换体对[Ca²⁺]c 进行短期(秒级)控制的证据。总之,结果表明尽管缺乏 CICR,但 SR 在去极化使其升高后从细胞质中去除钙离子。然后该钙离子通过钠钙交换体从 SR 转运到细胞外。然而,在去极化或从储存库释放离子导致钙离子短暂升高后,该交换体对总体平均[Ca²⁺]c 的下降没有显著贡献。

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