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大鼠心室肌细胞中L型钙电流与单个肌浆网钙释放事件之间的关系。

Relationship between L-type Ca2+ current and unitary sarcoplasmic reticulum Ca2+ release events in rat ventricular myocytes.

作者信息

Collier M L, Thomas A P, Berlin J R

机构信息

Department of Physiology, Allegheny University of the Health Sciences, Philadelphia, PA, USA.

出版信息

J Physiol. 1999 Apr 1;516 ( Pt 1)(Pt 1):117-28. doi: 10.1111/j.1469-7793.1999.117aa.x.

Abstract
  1. The time courses of Ca2+ current and Ca2+ spark occurrence were determined in single rat ventricular myocytes voltage clamped with patch pipettes containing 0.1 microM fluo-3. Acquisition of line-scan images on a laser scanning confocal microscope was synchronized with measurement of Cd2+-sensitive Ca2+ currents. In most cells, individual Ca2+ sparks were observed by reducing Ca2+ current density with nifedipine (0.1-8 microM). 2. Ca2+ sparks elicited by depolarizing voltage-clamp pulses had a peak [Ca2+] amplitude of 289 +/- 3 nM with a decay half-time of 20.8 +/- 0.2 ms and a full width at half-maximum of 1.40 +/- 0.03 microm (mean +/- s. e.m., n = 345), independent of the membrane potential. 3. The time between the beginning of a depolarization and the initiation of each Ca2+ spark was calculated and data were pooled to construct waiting time histograms. Exponential functions were fitted to these histograms and to the decaying phase of the Ca2+ current. This analysis showed that the time constants describing Ca2+ current and Ca2+ spark occurrence at membrane potentials between -30 mV and +30 mV were not significantly different. At +50 mV, in the absence of nifedipine, the time constant describing Ca2+ spark occurrence was significantly larger than the time constant of the Ca2+ current. 4. A simple model is developed using Poisson statistics to relate macroscopic Ca2+ current to the opening of single L-type Ca2+ channels at the dyad junction and to the time course of Ca2+ spark occurrence. The model suggests that the time courses of macroscopic Ca2+ current and Ca2+ spark occurrence should be closely related when opening of a single L-type Ca2+ channel initiates a Ca2+ spark. By comparison with the data, the model suggests that Ca2+ sparks are initiated by the opening of a single L-type Ca2+ channel at all membrane potentials encountered during an action potential.
摘要
  1. 在使用含0.1微摩尔荧光素-3的膜片吸管进行电压钳制的单个大鼠心室肌细胞中,测定了Ca2+电流和Ca2+闪烁发生的时间进程。在激光扫描共聚焦显微镜上采集线扫描图像与测量Cd2+敏感的Ca2+电流同步。在大多数细胞中,通过用硝苯地平(0.1 - 8微摩尔)降低Ca2+电流密度来观察单个Ca2+闪烁。2. 去极化电压钳制脉冲引发的Ca2+闪烁的峰值[Ca2+]幅度为289±3纳摩尔,衰减半衰期为20.8±0.2毫秒,半高宽为1.40±0.03微米(平均值±标准误,n = 345),与膜电位无关。3. 计算去极化开始到每个Ca2+闪烁起始之间的时间,并汇总数据以构建等待时间直方图。将指数函数拟合到这些直方图以及Ca2+电流的衰减阶段。该分析表明,在 - 30毫伏至 + 30毫伏之间的膜电位下,描述Ca2+电流和Ca2+闪烁发生的时间常数没有显著差异。在 + 50毫伏时,在没有硝苯地平的情况下,描述Ca2+闪烁发生的时间常数显著大于Ca2+电流的时间常数。4. 使用泊松统计建立了一个简单模型,以将宏观Ca2+电流与二联体连接处单个L型Ca2+通道的开放以及Ca2+闪烁发生的时间进程联系起来。该模型表明,当单个L型Ca2+通道的开放引发Ca2+闪烁时,宏观Ca2+电流和Ca2+闪烁发生的时间进程应该密切相关。通过与数据比较,该模型表明在动作电位期间遇到的所有膜电位下,Ca2+闪烁都是由单个L型Ca2+通道的开放引发的。

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