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管腔Ca2+在大鼠心室肌细胞Ca2+波产生中的作用。

The role of luminal Ca2+ in the generation of Ca2+ waves in rat ventricular myocytes.

作者信息

Lukyanenko V, Subramanian S, Gyorke I, Wiesner T F, Gyorke S

机构信息

Department of Physiology, University Health Sciences Center, Texas Tech University, Lubbock, TX, USA.

出版信息

J Physiol. 1999 Jul 1;518(Pt 1):173-86. doi: 10.1111/j.1469-7793.1999.0173r.x.

Abstract
  1. We used confocal Ca2+ imaging and fluo-3 to investigate the transition of localized Ca2+ releases induced by focal caffeine stimulation into propagating Ca2+ waves in isolated rat ventricular myocytes. 2. Self-sustaining Ca2+ waves could be initiated when the cellular Ca2+ load was increased by elevating the extracellular [Ca2+] ([Ca2+]o) and they could also be initiated at normal Ca2+ loads when the sensitivity of the release sites to cytosolic Ca2+ was enhanced by low doses of caffeine. When we prevented the accumulation of extra Ca2+ in the luminal compartment of the sarcoplasmic reticulum (SR) with thapsigargin, focal caffeine pulses failed to trigger self-sustaining Ca2+ waves on elevation of [Ca2+]o. Inhibition of SR Ca2+ uptake by thapsigargin in cells already preloaded with Ca2+ above normal levels did not prevent local Ca2+ elevations from triggering propagating waves. Moreover, wave velocity increased by 20 %. Tetracaine (0.75 mM) caused transient complete inhibition of both local and propagating Ca2+ signals, followed by full recovery of the responses due to increased SR Ca2+ accumulation. 3. Computer simulations using a numerical model with spatially distinct Ca2+ release sites suggested that increased amounts of releasable Ca2+ might not be sufficient to generate self-sustaining Ca2+ waves under conditions of Ca2+ overload unless the threshold of release site Ca2+ activation was set at relatively low levels (< 1.5 microM). 4. We conclude that the potentiation of SR Ca2+ release channels by luminal Ca2+ is an important factor in Ca2+ wave generation. Wave propagation does not require the translocation of Ca2+ from the spreading wave front into the SR. Instead, it relies on luminal Ca2+ sensitizing Ca2+ release channels to cytosolic Ca2+.
摘要
  1. 我们使用共聚焦钙成像和荧光素-3来研究在分离的大鼠心室肌细胞中,由局部咖啡因刺激诱导的局部钙释放向传播性钙波的转变。2. 当通过提高细胞外钙离子浓度([Ca2+]o)增加细胞内钙负荷时,能够引发自我维持的钙波;当低剂量咖啡因增强释放位点对胞质钙离子的敏感性时,在正常钙负荷下也能引发自我维持的钙波。当我们用毒胡萝卜素阻止额外的钙离子在肌浆网(SR)腔室中积累时,局部咖啡因脉冲在升高[Ca2+]o时未能触发自我维持的钙波。在已经预加载高于正常水平钙离子的细胞中,毒胡萝卜素抑制SR对钙离子的摄取并不能阻止局部钙离子升高触发传播波。此外,波速增加了20%。丁卡因(0.75 mM)导致局部和传播性钙信号短暂完全抑制,随后由于SR中钙离子积累增加,反应完全恢复。3. 使用具有空间上不同钙释放位点的数值模型进行的计算机模拟表明,在钙超载条件下,除非将释放位点钙激活的阈值设定在相对较低水平(<1.5 microM),否则可释放钙量的增加可能不足以产生自我维持的钙波。4. 我们得出结论,腔内钙离子对SR钙释放通道的增强作用是钙波产生的一个重要因素。波的传播不需要钙离子从传播的波前转运到SR中。相反,它依赖于腔内钙离子使钙释放通道对胞质钙离子敏感。

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