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大鼠肿瘤生长激素细胞的内源性起搏活动。

Endogenous pacemaker activity of rat tumour somatotrophs.

作者信息

Kwiecien R, Robert C, Cannon R, Vigues S, Arnoux A, Kordon C, Hammond C

机构信息

Unite de Dynamique des Systemes Neuroendocriniens, INSERM U159, 2 ter rue d'Alesia, 75014 Paris, France.

出版信息

J Physiol. 1998 May 1;508 ( Pt 3)(Pt 3):883-905. doi: 10.1111/j.1469-7793.1998.883bp.x.

DOI:10.1111/j.1469-7793.1998.883bp.x
PMID:9518740
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2230921/
Abstract
  1. Cells derived from a rat pituitary tumour (GC cell line) that continuously release growth hormone behave as endogenous pacemakers. In simultaneous patch clamp recordings and cytosolic Ca2+ concentration ([Ca2+]i) imaging, they displayed rhythmic action potentials (44.7 +/- 2.7 mV, 178 +/- 40 ms, 0.30 +/- 0.04 Hz) and concomitant [Ca2+]i transients (374 +/- 57 nM, 1.0 +/- 0.2 s, 0.27 +/- 0.03 Hz). 2. Action potentials and [Ca2+]i transients were reversibly blocked by removal of external Ca2+, addition of nifedipine (1 microM) or Ni2+ (40 microM), but were insensitive to TTX (1 microM). An L-type Ca2+ current activated at -33.6 +/- 0.4 mV (holding potential (Vh), -40 mV), peaked at -1.8 +/- 1.3 mV, was reduced by nifedipine and enhanced by S-(+)-SDZ 202 791. A T/R-type Ca2+ current activated at -41.7 +/- 2.7 mV (Vh, -80 or -60 mV), peaked at -9.2 +/- 3.0 mV, was reduced by low concentrations of Ni2+ (40 microM) or Cd2+ (10 microM) and was toxin resistant. Parallel experiments revealed the expression of the class E calcium channel alpha1-subunit mRNA. 3. The K+ channel blockers TEA (25 mM) and charybdotoxin (10-100 nM) enhanced spike amplitude and/or duration. Apamin (100 nM) also strongly reduced the after-spike hyperpolarization. The outward K+ tail current evoked by a depolarizing step that mimicked an action potential reversed at -69. 8 +/- 0.3 mV, presented two components, lasted 2-3 s and was totally blocked by Cd2+ (400 microM). 4. The slow pacemaker depolarization (3.5 +/- 0.4 s) that separated consecutive spikes corresponded to a 2- to 3-fold increase in membrane resistance, was strongly Na+ sensitive but TTX insensitive. 5. Computer simulations showed that pacemaker activity can be reproduced by a minimum of six currents: an L-type Ca2+ current underlies the rising phase of action potentials that are repolarized by a delayed rectifier and Ca2+-activated K+ currents. In between spikes, the decay of Ca2+-activated K+ currents and a persistent inward cationic current depolarize the membrane, activate the T/R-type Ca2+ current and initiate a new cycle.
摘要
  1. 源自大鼠垂体肿瘤(GC细胞系)且持续释放生长激素的细胞表现为内源性起搏器。在同时进行的膜片钳记录和胞质Ca2+浓度([Ca2+]i)成像中,它们显示出有节律的动作电位(44.7±2.7 mV,178±40 ms,0.30±0.04 Hz)以及伴随的[Ca2+]i瞬变(374±57 nM,1.0±0.2 s,0.27±0.03 Hz)。2. 去除细胞外Ca2+、添加硝苯地平(1 μM)或Ni2+(40 μM)可使动作电位和[Ca2+]i瞬变可逆性阻断,但对TTX(1 μM)不敏感。一种L型Ca2+电流在-33.6±0.4 mV(钳制电位(Vh),-40 mV)时被激活,在-1.8±1.3 mV时达到峰值,可被硝苯地平降低并被S-(+)-SDZ 202 791增强。一种T/R型Ca2+电流在-41.7±2.7 mV(Vh,-80或-60 mV)时被激活,在-9.2±3.0 mV时达到峰值,可被低浓度的Ni2+(40 μM)或Cd2+(10 μM)降低且对毒素有抗性。平行实验揭示了E类钙通道α1亚基mRNA的表达。3. K+通道阻滞剂TEA(25 mM)和蝎毒素(10 - 100 nM)可增强动作电位幅度和/或持续时间。蜂毒明肽(100 nM)也能强烈降低动作电位后的超极化。由模拟动作电位的去极化步骤诱发的外向K+尾电流在-69.8±0.3 mV时反转,呈现两个成分,持续2 - 3 s且完全被Cd2+(400 μM)阻断。4. 分隔连续动作电位的缓慢起搏器去极化(3.5±0.4 s)对应膜电阻增加2至3倍,对Na+高度敏感但对TTX不敏感。5. 计算机模拟表明,至少六种电流可重现起搏器活动:L型Ca2+电流是动作电位上升相的基础,动作电位由延迟整流器和Ca2+激活的K+电流复极化。在动作电位之间,Ca2+激活的K+电流的衰减和持续内向阳离子电流使膜去极化,激活T/R型Ca2+电流并启动新的周期。

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