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豚鼠电压钳制海马神经元中的钙激活外向电流。

Calcium-activated outward current in voltage-clamped hippocampal neurones of the guinea-pig.

作者信息

Brown D A, Griffith W H

出版信息

J Physiol. 1983 Apr;337:287-301. doi: 10.1113/jphysiol.1983.sp014624.

DOI:10.1113/jphysiol.1983.sp014624
PMID:6875931
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1199107/
Abstract

Slow clamp currents were recorded from CA1 and CA3 pyramidal neurones in slices of guinea-pig hippocampus maintained in vitro, using a single micro-electrode sample-and-hold technique. Depolarizing voltage commands evoked a time- and voltage-dependent outward current which was suppressed by removing external Ca or by adding Cd (0.5 mM) or Mn (5 mM). This Ca-dependent current (Ic) was not reduced by muscarinic agonists (unlike IM) but was greatly reduced by 5-20 mM-tetraethylammonium (TEA). Repolarizing IC tail currents reversed at -73 +/- 5 mV in 3 mM-K solution. The reversal potential became about 30 mV more positive on raising [K]o to 15 mM. No clear change in current amplitude or tail-current reversal potential occurred on adding Cs (2 mM), reducing [Cl]o from 128 to 10 mM, or replacing external Na with Tris. The underlying conductance GC was activated at membrane potentials positive to -45 mV. At -32 mV GC showed an approximately exponential increase with time, with a time constant of approximately 0.6 sec at 26 degrees C. Repolarizing tail currents declined exponentially with time, the time constant becoming shorter with increasing negative post-pulse potentials. When the clamp was switched off at the end of a depolarizing command of sufficient amplitude and duration to activate IC, a membrane hyperpolarization to -73 mV ensued, of similar amplitude and decay time to that following spontaneous action potentials. It is concluded that the clamp current observed in these experiments is probably the Ca-activated K current thought to contribute to the post-activation after-hyperpolarization in hippocampal neurones.

摘要

采用单微电极采样保持技术,在体外维持的豚鼠海马切片中,记录CA1和CA3锥体神经元的慢钳制电流。去极化电压指令诱发了一种时间和电压依赖性外向电流,去除细胞外钙或添加镉(0.5 mM)或锰(5 mM)可抑制该电流。这种钙依赖性电流(Ic)不受毒蕈碱激动剂的影响(与IM不同),但可被5 - 20 mM的四乙铵(TEA)显著降低。在3 mM - K溶液中,复极化的Ic尾电流在-73±5 mV处反转。将[K]o提高到15 mM时,反转电位变得更正约30 mV。添加铯(2 mM)、将[Cl]o从128 mM降至10 mM或用Tris替代细胞外钠时,电流幅度或尾电流反转电位均无明显变化。基础电导GC在膜电位正向至-45 mV时被激活。在-32 mV时,GC随时间呈近似指数增加,在26℃时时间常数约为0.6秒。复极化尾电流随时间呈指数下降,时间常数随负向脉冲后电位增加而缩短。当在足够幅度和持续时间的去极化指令结束时关闭钳制,会随之出现膜超极化至-73 mV,其幅度和衰减时间与自发动作电位后的相似。结论是,在这些实验中观察到的钳制电流可能是钙激活钾电流,被认为有助于海马神经元激活后超极化。

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