ffrench-Mullen J M, Rogawski M A
Laboratory of Neurophysiology, National Institute of Neurological Disorders and Stroke, Bethesda, Maryland 20892.
J Neurosci. 1989 Nov;9(11):4051-61. doi: 10.1523/JNEUROSCI.09-11-04051.1989.
Whole-cell voltage-clamp recording techniques were used to investigate the blockade of voltage-dependent K+ channels by phencyclidine (PCP) in cultured rat hippocampal neurons. All recordings were carried out in the presence of tetrodotoxin (1-2 microM) to eliminate Na+ currents. Step depolarization from a holding potential of -40 mV activated a slowly rising, minimally inactivating K+ current (IK). PCP (0.5-1000 microM) caused a reduction in the maximum conductance of IK [IC50(+30 mV), 22 microM] without altering its voltage dependency. The PCP block of IK diminished at depolarized potentials. Analysis according to the scheme of Woodhull (1973) suggested that block occurs via binding to an acceptor site (presumably within the channel pore) that senses 40-50% of the transmembrane electrostatic field. PCP had no effect on the kinetic properties of IK and the block failed to show use dependency, suggesting that PCP may bind to the IK channel via a hydrophobic mechanism not requiring open channels. For comparison, we also investigated the effect of PCP on the transient K+ current, IA, activated by step depolarization following a 200 msec prepulse to -90 mV (20 mM tetraethylammonium was present in the bathing solution to reduce IK). In contrast to the potent blocking action of PCP on IK, the drug only affected IA at high concentrations [IC50(+30 mV), 224 microM]. At concentrations causing substantial block (300-500 microM), PCP produced an acceleration in the IA inactivation rate, and, for brief (5-6 msec) depolarizing steps, the suppression of IA was use dependent. These observations suggest that PCP block of IA requires open channels. PCP reduced inward current responses induced by the excitatory amino acid agonist N-methyl-D-aspartate (NMDA) at substantially lower concentrations than those required for its effects on K+ channels [IC50(-60 mV), 0.45 microM]. The PCP-like dioxadrol stereoisomer dexoxadrol (10 microM) blocked NMDA-evoked inward current responses, while its behaviorally inactive enantiomer levoxadrol did not. Dexoxadrol and levoxadrol also blocked IK in a stereoselective fashion (IC50's, 73 and 260 microM, respectively), whereas the sigma ligands (+)- and (-)-SKF 10,047 and (+)-3-[3-hydroxyphenyl]-N-(1-propyl)piperidine [(+)-3-PPP] had little effect on the current (IC50's, greater than 300-500 microM). We conclude that PCP causes a selective, voltage-dependent block of IK in hippocampal neurons via a PCP- and not a sigma-type acceptor site.(ABSTRACT TRUNCATED AT 400 WORDS)
采用全细胞膜片钳记录技术,研究了苯环己哌啶(PCP)对培养的大鼠海马神经元中电压依赖性钾通道的阻断作用。所有记录均在河豚毒素(1 - 2 μM)存在的情况下进行,以消除钠电流。从 - 40 mV 的钳制电位进行阶跃去极化,激活了一个缓慢上升、极少失活的钾电流(IK)。PCP(0.5 - 1000 μM)导致 IK 的最大电导降低[IC50(+30 mV),22 μM],而不改变其电压依赖性。IK 的 PCP 阻断作用在去极化电位下减弱。根据伍德胡尔(1973 年)的方案进行分析表明,阻断是通过与一个受体位点(可能在通道孔内)结合发生的,该受体位点感知跨膜静电场的 40 - 50%。PCP 对 IK 的动力学特性没有影响,且阻断未表现出使用依赖性,这表明 PCP 可能通过一种不需要开放通道的疏水机制与 IK 通道结合。为作比较,我们还研究了 PCP 对瞬态钾电流 IA 的影响,IA 是在向 - 90 mV 进行 200 毫秒预脉冲后通过阶跃去极化激活的(浴液中存在 20 mM 四乙铵以减少 IK)。与 PCP 对 IK 的强效阻断作用相反,该药物仅在高浓度时影响 IA[IC50(+30 mV),224 μM]。在引起显著阻断的浓度(300 - 500 μM)下,PCP 使 IA 的失活速率加快,并且对于短暂(5 - 6 毫秒)的去极化步骤,IA 的抑制是使用依赖性的。这些观察结果表明,PCP 对 IA 的阻断需要开放通道。PCP 在比其对钾通道作用所需浓度低得多的浓度下,就能降低兴奋性氨基酸激动剂 N - 甲基 - D - 天冬氨酸(NMDA)诱导的内向电流反应[IC50(-60 mV),0.45 μM]。PCP 样二氧杂环己醇立体异构体右吗拉胺(10 μM)阻断 NMDA 诱发的内向电流反应,而其行为上无活性的对映体左吗拉胺则无此作用。右吗拉胺和左吗拉胺也以立体选择性方式阻断 IK(IC50 分别为 73 和 260 μM),而西格玛配体(+) - 和( - ) - SKF 10,047 以及(+) - 3 - [3 - 羟基苯基] - N - (1 - 丙基)哌啶[(+) - 3 - PPP]对电流影响很小(IC50 大于 300 - 500 μM)。我们得出结论,PCP 通过 PCP 型而非西格玛型受体位点,在海马神经元中对 IK 产生选择性的、电压依赖性阻断。(摘要截短于 400 字)