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激活减慢的G蛋白调节性钙电流不会改变动作电位诱发的钙电流的动力学。

G-protein-modulated Ca(2+) current with slowed activation does not alter the kinetics of action potential-evoked Ca(2+) current.

作者信息

Artim D E, Meriney S D

机构信息

Department of Neuroscience, University of Pittsburgh, Pittsburgh, Pennsylvania 15260, USA.

出版信息

J Neurophysiol. 2000 Nov;84(5):2417-25. doi: 10.1152/jn.2000.84.5.2417.

Abstract

We have studied voltage-dependent inhibition of N-type calcium currents to investigate the effects of G-protein modulation-induced alterations in channel gating on action potential-evoked calcium current. In isolated chick ciliary ganglion neurons, GTPgammaS produced voltage-dependent inhibition that exhibited slowed activation kinetics and was partially relieved by a conditioning prepulse. Using step depolarizations to evoke calcium current, we measured tail current amplitudes on abrupt repolarization to estimate the time course of calcium channel activation from 1 to 30 ms. GTPgammaS prolonged significantly channel activation, consistent with the presence of kinetic slowing in the modulated whole cell current evoked by 100-ms steps. Since kinetic slowing is caused by an altered voltage dependence of channel activation (such that channels require stronger or longer duration depolarization to open), we asked if GTPgammaS-induced modulation would alter the time course of calcium channel activation during an action potential. Using an action potential waveform as a voltage command to evoke calcium current, we abruptly repolarized to -80 mV at various time points during the repolarization phase of the action potential. The resulting tail current was used to estimate the relative number of calcium channels that were open. Using action potential waveforms of either 2.2- or 6-ms duration at half-amplitude, there were no differences in the time course of calcium channel activation, or in the percent activation at any time point tested during the repolarization, when control and modulated currents were compared. It is also possible that modulated channels might open briefly and that these reluctant openings would effect the time course of action potential-evoked calcium current. However, when control and modulated currents were scaled to the same peak amplitude and superimposed, there was no difference in the kinetics of the two currents. Thus voltage-dependent inhibition did not alter the kinetics of action potential-evoked current. These results suggest that G-protein-modulated channels do not contribute significantly to calcium current evoked by a single action potential.

摘要

我们研究了电压依赖性N型钙电流抑制,以探讨G蛋白调节引起的通道门控改变对动作电位诱发钙电流的影响。在分离的鸡睫状神经节神经元中,GTPγS产生电压依赖性抑制,其表现为激活动力学减慢,并被一个条件性预脉冲部分缓解。使用阶跃去极化诱发钙电流,我们在突然复极化时测量尾电流幅度,以估计1至30毫秒内钙通道激活的时间进程。GTPγS显著延长了通道激活时间,这与100毫秒阶跃诱发的调制全细胞电流中存在动力学减慢一致。由于动力学减慢是由通道激活电压依赖性的改变引起的(即通道需要更强或更长持续时间的去极化才能打开),我们询问GTPγS诱导的调制是否会改变动作电位期间钙通道激活的时间进程。使用动作电位波形作为电压指令诱发钙电流,我们在动作电位复极化阶段的不同时间点突然复极化到 -80 mV。由此产生的尾电流用于估计开放的钙通道的相对数量。当比较对照电流和调制电流时,使用半幅度持续时间为2.2毫秒或6毫秒的动作电位波形,钙通道激活的时间进程或复极化期间任何测试时间点的激活百分比均无差异。调制通道也可能短暂开放,而这些勉强的开放可能会影响动作电位诱发钙电流的时间进程。然而,当对照电流和调制电流按比例缩放至相同的峰值幅度并叠加时,两种电流的动力学没有差异。因此,电压依赖性抑制不会改变动作电位诱发电流的动力学。这些结果表明,G蛋白调制的通道对单个动作电位诱发的钙电流贡献不大。

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