首页> 外文期刊>The Journal of general physiology >Kinetic and steady-state properties of Na+ channel and Ca2+ channel charge movements in ventricular myocytes of embryonic chick heart.
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Kinetic and steady-state properties of Na+ channel and Ca2+ channel charge movements in ventricular myocytes of embryonic chick heart.

机译:雏鸡心脏心室肌细胞中Na +通道和Ca2 +通道电荷运动的动力学和稳态特性。

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Nonlinear or asymmetric charge movement was recorded from single ventricular myocytes cultured from 17-d-old embryonic chick hearts using the whole-cell patch clamp method. The myocytes were exposed to the appropriate intracellular and extracellular solutions designed to block Na+, Ca2+, and K+ ionic currents. The linear components of the capacity and leakage currents during test voltage steps were eliminated by adding summed, hyperpolarizing control step currents. Upon depolarization from negative holding potentials the nonlinear charge movement was composed of two distinct and separable kinetic components. An early rapidly decaying component (decay time constant range: 0.12-0.50 ms) was significant at test potentials positive to -70 mV and displayed saturation above 0 mV (midpoint -35 mV; apparent valence 1.6 e-). The early ON charge was partially immobilized during brief (5 ms) depolarizing test steps and was more completely immobilized by the application of less negative holding potentials. A second slower-decaying component (decay time constant range: 0.88-3.7 ms) was activated at test potentials positive to -60 mV and showed saturation above +20 mV (midpoint -13 mV, apparent valence 1.9 e-). The second component of charge movement was immobilized by long duration (5 s) holding potentials, applied over a more positive voltage range than those that reduced the early component. The voltage dependencies for activation and inactivation of the Na+ and Ca2+ ionic currents were determined for myocytes in which these currents were not blocked. There was a positive correlation between the voltage dependence of activation and inactivation of the Na+ and Ca2+ ionic currents and the activation and immobilization of the fast and slow components of charge movement. These complementary kinetic and steady-state properties lead to the conclusion that the two components of charge movement are associated with the voltage-sensitive conformational changes that precede Na+ and Ca2+ channel openings.
机译:使用全细胞膜片钳方法记录了从17 d龄雏鸡心脏培养的单个心室肌细胞的非线性或不对称电荷运动。将心肌细胞暴露于适当的细胞内和细胞外溶液中,这些溶液旨在阻断Na +,Ca2 +和K +离子流。通过增加相加的超极化控制步骤电流,消除了测试电压步骤期间容量和泄漏电流的线性分量。从负保持电位除极化后,非线性电荷运动由两个不同且可分离的动力学分量组成。早期快速衰减成分(衰减时间常数范围:0.12-0.50 ms)在测试电位为-70 mV时显着,并且在0 mV以上(中点-35 mV;表观价为1.6 e-)时显示饱和。在短暂的去极化测试步骤(5毫秒)中,早期的ON电荷被部分固定,并通过施加较小的负保持电位而更加完全地固定。第二个较慢衰减的分量(衰减时间常数范围:0.88-3.7 ms)在正至-60 mV的测试电势下被激活,并显示出高于+20 mV的饱和度(中点-13 mV,表观价1.9 e-)。电荷移动的第二个成分是通过长时间(5 s)的保持电位固定的,该电位保持在比减少早期成分更正的电压范围内。对于其中未阻断这些电流的心肌细胞,确定了Na +和Ca2 +离子电流激活和失活的电压依赖性。 Na +和Ca2 +离子电流的激活和灭活与电压的依赖性与电荷移动的快慢成分的激活和固定之间存在正相关关系。这些互补的动力学和稳态特性得出这样的结论:电荷移动的两个分量与Na +和Ca2 +通道开口之前的电压敏感构象变化有关。

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