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豚鼠嗅皮质神经元体外培养时的钙依赖性钾电导

Calcium-dependent potassium conductance in guinea-pig olfactory cortex neurones in vitro.

作者信息

Constanti A, Sim J A

机构信息

Department of Pharmacology, School of Pharmacy, London.

出版信息

J Physiol. 1987 Jun;387:173-94. doi: 10.1113/jphysiol.1987.sp016569.

DOI:10.1113/jphysiol.1987.sp016569
PMID:2443678
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1192500/
Abstract
  1. Guinea-pig olfactory cortex neurones in vitro (23-25 degrees C) were voltage clamped by means of a single-micro-electrode sample-and-hold technique. 2. Under current clamp at the resting potential (approximately -80 mV), brief depolarizing stimuli evoked trains of action potentials with little visible after-potential. However, in 90% of recorded cells held at membrane potentials between -70 and -45 mV, depolarizing current pulses evoked a slow after-hyperpolarization (a.h.p.) (approximately 8 mV) lasting several seconds and accompanied by an increase in input conductance. 3. The outward membrane current underlying the a.h.p. was revealed either by switching rapidly to voltage clamp at the end of a spike train ('hybrid' clamp) or by applying brief depolarizing commands from potentials between -60 to -45 mV. The tail current showed a distinct rising phase (time to peak approximately 1 s) and exponential decay (tau approximately 3 s) and was suppressed by removal of external Ca2+, or adding Co2+ (1-2 mM), Cd2+ (200 microM) or Mg2+ (6 mM). The a.h.p. current reversal potential was -96 mV in 3 mM-K+ medium. 4. Low concentrations (1-2 microM) of muscarine, carbachol, oxotremorine or the muscarinic ganglion stimulant, McN-A-343 (1-10 microM) reduced the a.h.p. current and leak conductance and induced a steady inward current, without affecting M-current (IM) relaxations. IM inhibition generally required higher (greater than 10 microM) agonist concentrations, although oxotremorine remained ineffective at up to 50 microM. 5. The a.h.p. current was reduced by noradrenaline and tetraethylammonium (TEA), but not by apamin or tubocurarine. Apart from TEA, these agents had no effect on IM. 6. Addition of tetrodotoxin (TTX, 1 microM) or removing external Na+ depressed the a.h.p. current amplitude recorded under voltage clamp. The residual tail current could be further reduced by adding Cd2+ or muscarinic agonists. 7. Repolarizing tail currents induced following positive voltage commands consisted mainly of IM and slow a.h.p. current with little evidence of a 'fast' Ca2+-activated K+ current (IC). 8. It is concluded that the slow a.h.p. current that underlies the post-burst after-hyperpolarization of olfactory neurones, is a Ca2+-dependent K+ current distinct from IM. It is suggested that the cholinergic modulation of this current (rather than IM) may provide a more subtle control of cell excitability in cortical neurones.
摘要
  1. 采用单微电极采样保持技术,在体外(23 - 25摄氏度)对豚鼠嗅觉皮层神经元进行电压钳制。2. 在静息电位(约 -80 mV)下进行电流钳制时,短暂的去极化刺激诱发动作电位序列,几乎没有可见的后电位。然而,在90%的记录细胞中,当膜电位保持在 -70至 -45 mV之间时,去极化电流脉冲诱发了持续数秒的缓慢超极化后电位(a.h.p.)(约8 mV),并伴有输入电导增加。3. 通过在一串动作电位结束时迅速切换到电压钳制(“混合”钳制),或者从 -60至 -45 mV的电位施加短暂的去极化指令,揭示了a.h.p. 背后的外向膜电流。尾电流呈现出明显的上升阶段(达到峰值的时间约1 s)和指数衰减(时间常数约3 s),并且通过去除细胞外Ca2+,或添加Co2+(1 - 2 mM)、Cd2+(200 microM)或Mg2+(6 mM)而受到抑制。在3 mM - K+ 培养基中,a.h.p. 电流反转电位为 -96 mV。4. 低浓度(1 - 2 microM)的毒蕈碱、卡巴胆碱、氧化震颤素或毒蕈碱型神经节兴奋剂McN - A - 343(1 - 10 microM)可降低a.h.p. 电流和漏电流,并诱导稳定的内向电流,而不影响M电流(IM)的松弛。IM抑制通常需要更高(大于10 microM)的激动剂浓度,尽管氧化震颤素在高达50 microM时仍无效。5. 去甲肾上腺素和四乙铵(TEA)可降低a.h.p. 电流,但蜂毒明肽或筒箭毒碱则无此作用。除了TEA外,这些药物对IM均无影响。6. 添加河豚毒素(TTX,1 microM)或去除细胞外Na+ 会降低电压钳制下记录的a.h.p. 电流幅度。通过添加Cd2+ 或毒蕈碱型激动剂,可进一步降低残余尾电流。7. 正电压指令后诱导的复极化尾电流主要由IM和缓慢的a.h.p. 电流组成,几乎没有证据表明存在“快速”的Ca2+ 激活K+ 电流(IC)。8. 得出结论,嗅觉神经元爆发后超极化背后的缓慢a.h.p. 电流是一种与IM不同的Ca2+ 依赖性K+ 电流。有人提出,该电流(而非IM)的胆碱能调制可能对皮层神经元的细胞兴奋性提供更精细的控制。

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