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青蛙离体骨骼肌纤维中慢钙电流的快速门控动力学

Fast gating kinetics of the slow Ca2+ current in cut skeletal muscle fibres of the frog.

作者信息

Feldmeyer D, Melzer W, Pohl B, Zöllner P

机构信息

Department of Cell Physiology, Ruhr-University Bochum, FRG.

出版信息

J Physiol. 1990 Jun;425:347-67. doi: 10.1113/jphysiol.1990.sp018107.

Abstract
  1. Calcium currents and intramembrane charge movements were measured in cut twitch muscle fibres of the frog and the time course of activation of the current was studied using various conditioning pulse protocols. 2. When a conditioning activation was produced by a depolarizing pulse which ended before inactivation occurred, a subsequent depolarization led to a faster onset of activation, indicating that the system had not completely returned to the initial state during the interval between the two pulses. 3. The interval between conditioning and test pulse was varied at different subthreshold potentials to study the time course of restoring the steady-state conditions. Complete restoration required a waiting period of about 1 min at the holding potential of -80 mV due to a very slow process but partial recovery was reached within 100 ms. This initial recovery process was strongly voltage dependent and became considerably slower when the interval potential approached the threshold for current activation. 4. Stepping to a roughly 10 mV subthreshold potential without applying a conditioning activation caused no change in the time course of the current produced by a subsequent test depolarization. Depolarizing just to the current threshold caused a slowly progressing acceleration of test current activation. 5. The peak current-voltage relation in the fast gating regime caused by a conditioning activation coincided with the current-voltage relation measured under steady-state conditions, indicating not that a new channel population had become activated but that the same channels showed a different gating behaviour. 6. Intramembrane charge movements measured in 2 mM-Cd2+ and tested at potentials between -40 and +40 mV showed negligible changes when preceded by a strong depolarization. 7. We discuss several possible models which can explain the fact that the current is speeded up by a conditioning activation while the charge movements remain unchanged. It is possible that the fast voltage-dependent transition which becomes visible after conditioning pulses reflects a rapid conformational change of the Ca2+ channel molecule which also occurs during its normal gating mode but remains undetectable in terms of conductance. In view of the hypothesis that the Ca2+ channel molecule forms a voltage sensor for excitation-contraction coupling this fast transition could be coupled to the control of Ca2+ release from the sarcoplasmic reticulum.
摘要
  1. 在青蛙的离体单收缩肌纤维中测量了钙电流和膜内电荷移动,并使用各种条件脉冲方案研究了电流激活的时间进程。2. 当由在失活发生之前结束的去极化脉冲产生条件激活时,随后的去极化导致激活的起始更快,这表明在两个脉冲之间的间隔期间系统尚未完全恢复到初始状态。3. 在不同的阈下电位下改变条件脉冲和测试脉冲之间的间隔,以研究恢复稳态条件的时间进程。由于一个非常缓慢的过程,在 -80 mV 的 holding 电位下完全恢复需要约 1 分钟的等待期,但在 100 ms 内达到部分恢复。这个初始恢复过程强烈依赖电压,并且当间隔电位接近电流激活阈值时变得相当缓慢。4. 不施加条件激活而跃升至大致 10 mV 的阈下电位不会导致随后的测试去极化产生的电流的时间进程发生变化。仅去极化至电流阈值会导致测试电流激活的缓慢进展加速。5. 由条件激活引起的快速门控状态下的峰值电流 - 电压关系与在稳态条件下测量的电流 - 电压关系一致,这表明不是新的通道群体被激活,而是相同的通道表现出不同的门控行为。6. 在 2 mM - Cd2+ 中测量并在 -40 至 +40 mV 之间的电位下测试的膜内电荷移动,在强去极化之前显示出可忽略不计的变化。7. 我们讨论了几种可能的模型,这些模型可以解释这样一个事实,即电流通过条件激活而加速,而电荷移动保持不变。有可能在条件脉冲后可见的快速电压依赖性转变反映了 Ca2+ 通道分子的快速构象变化,这种变化在其正常门控模式期间也会发生,但就电导率而言仍然无法检测到。鉴于 Ca2+ 通道分子形成用于兴奋 - 收缩偶联的电压传感器这一假设,这种快速转变可能与肌浆网中 Ca2+ 释放的控制相关联。

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