首页> 美国卫生研究院文献>The Journal of Physiology >Voltage-dependent activation of the inward-rectifier potassium channel in the ventricular cell membrane of guinea-pig heart.
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Voltage-dependent activation of the inward-rectifier potassium channel in the ventricular cell membrane of guinea-pig heart.

机译:豚鼠心脏心室细胞膜内向整流钾通道的电压依赖性激活。

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摘要

The activation kinetics of the inward-rectifier K+ channel were studied by single-channel recording in isolated single cells of the guinea-pig ventricle with two different extracellular concentrations of K+ ([K+]o 150 and 75 mM). When voltage pulses were applied from a holding potential more positive than the potassium equilibrium potential (EK), to potentials more negative than EK, the probability of the channel being in the open state (Po) increased with time after the onset of the command pulse. The ensemble averaged current increased in its initial phase (activation). When the command potential was more negative than EK-40 mV, the current decreased after rapid activation due to the inactivation of the channel. The averaged current could be divided into an instantaneous and a time-dependent activation component; the latter was fitted by a single exponential function. The time constant of the time-dependent component became shorter, at more negative command potentials. When compared at the same command potential, the instantaneous component became smaller, as the patch membrane was held at more depolarized potential. This indicates that the steady-state Po of the channel decreases with depolarization at potentials more positive than EK. The Po of the activation gate of the channel was estimated by dividing the steady-state Po of the channel by the Po of the inactivation gate at each potential. It was about 0.1 at EK + 20 mV and increased sigmoidally with hyperpolarization. At potentials more negative than EK-40 mV, the Po of the activation gate saturated and was almost 1. The single-channel analysis and the noise analysis of the steady-state current fluctuations revealed that the activation gate of the channel follows first-order kinetics between the open and closed states. The activation kinetics shifted along the voltage axis in a similar way as EK when different [K+]o were used. Thus, the activation of the channel depends not only on the membrane potential but also on EK, when [K+]o is changed. The macroscopic current flowing through the inward-rectifier K+ channel during the activation process was calculated, assuming that the elementary conductance of the channel is not voltage dependent. The calculated current showed a prominent inward-rectifying property in the steady state and formed a negative conductance region at potentials positive to EK. It was, therefore, concluded that the properties of the inward-rectifier time-independent background K+ current (iK1) in the whole-cell current records (Noble, 1979) mainly depend on the activation kinetics of the inward-rectifier K+ channel in the cardiac myocyte membrane.
机译:通过在豚鼠心室的分离的单个细胞中以两种不同的细胞外浓度K +([K +] o 150和75 mM)进行单通道记录,研究了内向整流器K +通道的激活动力学。当电压脉冲从比钾平衡电势(EK)更正的保持电势施加到比EK更负电势时,在指令脉冲开始后,通道处于打开状态(Po)的可能性会随时间增加。整体平均电流在其初始阶段(激活)增加。当指令电势比EK-40 mV负电多时,由于通道的失活,快速激活后电流减小。平均电流可以分为瞬时和时间相关的激活分量。后者由单个指数函数拟合。时间相关组件的时间常数变得更短,命令电位更大。当在相同的命令电势下进行比较时,由于将补片膜保持在更多的去极化电势下,瞬时分量变小了。这表明在比EK更正的电势下,通道的稳态Po随着去极化而降低。通过在每个电势下将通道的稳态Po除以失活栅极的Po来估算通道的活化栅的Po。在EK + 20 mV时约为0.1,并随着超极化而呈S形增加。在比EK-40 mV更负的电位时,激活门的Po饱和并且接近1。单通道分析和稳态电流波动的噪声分析表明,通道的激活门遵循一阶打开状态和关闭状态之间的动力学。当使用不同的[K +] o时,活化动力学以类似于EK的方式沿电压轴移动。因此,当[K +] o改变时,通道的激活不仅取决于膜电位,而且取决于EK。假设通道的基本电导率与电压无关,则计算在激活过程中流过内部整流器K +通道的宏观电流。计算出的电流在稳态下显示出显着的内向整流特性,并在对EK呈正电位的情况下形成了一个负电导区域。因此,得出的结论是,全细胞电流记录(Noble,1979)中向内整流器与时间无关的背景K +电流(iK1)的性质主要取决于向内整流器K +通道在电池中的激活动力学。心肌细胞膜。

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