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Some kinetic and steady-state properties of sodium channels after removal of inactivation

机译:灭活后钠通道的一些动力学和稳态性质

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摘要

To study the kinetic and steady-state properties of voltage-dependent sodium conductance activation, squid giant axons were perfused internally with either pronase or N-bromoacetamide and voltage clamped. Parameters of activation, tau m and gNa(V), and deactivation, tau Na, were measured and compared with those obtained from control axons under the assumption that gNa oc m3h of the Hodgkin-Huxley scheme. tau m(V) values obtained from the turn-on of INa agree well with control axons and previous determinations by others. tau Na(V) values derived from Na tail currents were also unchanged by pronase treatment and matched fairly well previously published values. tau m(V) obtained from 3 x tau Na(V) were much larger than tau m(V) obtained from INa turn-on at the same potentials, resulting in a discontinuous distribution. Steady- state In (gNa/gNa max - gNa) vs. voltage was not linear and had a limiting logarithmic slope of 5.3 mV/e-fold gNa. Voltage step procedures that induce a second turn-on of INa during various stages of the deactivation (Na tail current) process reveal quasiexponential activation at early stages that becomes increasingly sigmoid as deactivation progresses. For moderate depolarizations, primary and secondary activation kinetics are superimposable. These data suggest that, although m3 can describe the shape of INa turn-on, it cannot quantitatively account for the kinetics of gNa after repolarization. Kinetic schemes for gNa in which substantial deactivation occurs by a unique pathway between conducting and resting states are shown to be unlikely. It appears that the rate-limiting step in linear kinetic models of activation may be between a terminal conducting state and the adjacent nonconducting intermediate.
机译:为了研究电压依赖性钠电导活化的动力学和稳态特性,鱿鱼巨型轴突在内部用链霉蛋白酶或N-溴乙酰胺灌注并钳位电压。在霍奇金-赫克斯利(Hodgkin-Huxley)方案的gNa oc m3h的假设下,测量激活参数tau m和gNa(V)以及失活参数tau Na,并将其与从对照轴突获得的参数进行比较。从INa开启获得的tau m(V)值与控制轴突和其他人先前的确定非常吻合。通过链霉蛋白酶处理,从Na尾流得到的tau Na(V)值也没有变化,并且与以前发表的值相当吻合。在相同的电势下,从3 x tau Na(V)获得的tau m(V)远远大于从INa导通获得的tau m(V),导致不连续分布。稳态In(gNa / gNa max-gNa)与电压呈非线性关系,极限对数斜率为5.3 mV / e倍gNa。在失活过程的各个阶段(Na尾电流)引起INa的第二次导通的电压阶跃程序显示出在早期阶段的准指数激活,随着失活的进行,其逐渐呈S形。对于适度的去极化,一级和二级活化动力学是可叠加的。这些数据表明,尽管m3可以描述INa导通的形状,但它不能定量说明复极化后gNa的动力学。 gNa的动力学方案不太可能发生,在该方案中,通过传导状态和静止状态之间的唯一途径发生大量失活。似乎在线性活化动力学模型中的限速步骤可能在末端导电状态和相邻的非导电中间体之间。

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