Herrington J, Stern R C, Evers A S, Lingle C J
Department of Anesthesiology, Washington University School of Medicine, St. Louis, Missouri 63110.
J Neurosci. 1991 Jul;11(7):2226-40. doi: 10.1523/JNEUROSCI.11-07-02226.1991.
The effect of halothane on isolated calcium (Ca2+) current of clonal (GH3) pituitary cells was investigated using standard whole-cell clamp techniques at room temperature. Halothane (0.1-5.0 mM) reversibly reduced both the low-threshold, transient [low-voltage-activated (LVA)] component and the high-threshold [high-voltage-activated (HVA)] component of Ca2+ current. Halothane had little effect on the voltage dependence of activation or inactivation of either component of Ca2+ current. Inhibition of the peak high-threshold Ca2+ current was half-maximal at about 0.8 mM halothane, with maximal inhibition (100%) occurring with 5 mM halothane. When measured at the end of a 190-msec command step, half-maximal reduction of high-threshold current occurred at less than 0.5 mM halothane. The low-threshold transient current was less sensitive to halothane, with half-maximal inhibition of peak transient current activated at -30 mV occurring at approximately 1.3 mM. The effect of halothane on the HVA current was apparently not mediated by changes in intracellular Ca2+ concentration. The ability of halothane to inhibit Ca2+ current was unaffected by either the inclusion of the rapid Ca2+ buffer 1,2-bis(2-aminophenoxy)ethane N,N,N',N'-tetraacetic acid (BAPTA) in the recording pipette or exposure of the cell to 10 mM caffeine. To assess the selectivity of the effect of halothane, the actions of halothane on two components of voltage-activated potassium (K+) current observed in the absence of extracellular Ca2+ and on voltage-dependent sodium (Na+) current were also examined. Halothane had no effect on the voltage-dependent, inactivating K+ current of GH3 cells at concentrations up to 1.2 mM. In contrast, the non-inactivating K+ current, though less sensitive to halothane than either Ca2+ current, was reduced by about 40% by 1.2 mM halothane at +20 mV. Peak Na+ current was also blocked by halothane, but 50% block required around 2.6 mM halothane with little effect at 1.6 mM. Reduction of Na+ current was associated with a substantial negative shift in the steady-state inactivation curve. Although the results indicate that a number of voltage-dependent ionic currents are sensitive to halothane, both components of Ca2+ current exhibit a greater sensitivity to halothane than any of three other voltage-dependent currents in GH3 cells. These results show that GH3 cell Ca2+ currents are selectively inhibited by clinically appropriate concentrations of halothane and that the reduction of Ca2+ current can account for the inhibition by halothane of TRH- or KCl-induced prolactin secretion in GH3 cells.
在室温下,采用标准的全细胞钳技术研究了氟烷对克隆化垂体(GH3)细胞中分离的钙(Ca2+)电流的影响。氟烷(0.1 - 5.0 mM)可逆地降低了Ca2+电流的低阈值瞬态[低电压激活(LVA)]成分和高阈值[高电压激活(HVA)]成分。氟烷对Ca2+电流任何一个成分的激活或失活的电压依赖性几乎没有影响。高阈值Ca2+电流峰值的抑制在约0.8 mM氟烷时达到半数最大抑制,5 mM氟烷时出现最大抑制(100%)。在190毫秒指令步结束时测量,高阈值电流的半数最大降低在氟烷浓度低于0.5 mM时发生。低阈值瞬态电流对氟烷不太敏感,在 - 30 mV激活的瞬态电流峰值的半数最大抑制发生在约1.3 mM时。氟烷对HVA电流的影响显然不是由细胞内Ca2+浓度的变化介导的。氟烷抑制Ca2+电流的能力不受记录电极中加入快速Ca2+缓冲剂1,2 - 双(2 - 氨基苯氧基)乙烷N,N,N',N' - 四乙酸(BAPTA)或细胞暴露于10 mM咖啡因的影响。为了评估氟烷作用的选择性,还研究了氟烷在无细胞外Ca2+时对电压激活钾(K+)电流的两个成分以及电压依赖性钠(Na+)电流的作用。在浓度高达1.2 mM时,氟烷对GH3细胞的电压依赖性失活K+电流没有影响。相反,非失活K+电流虽然对氟烷的敏感性低于Ca2+电流中的任何一个,但在 + 20 mV时,1.2 mM氟烷使其降低了约40%。Na+电流峰值也被氟烷阻断,但50%阻断需要约2.6 mM氟烷,1.6 mM时几乎没有影响。Na+电流的降低与稳态失活曲线的显著负向移位有关。尽管结果表明许多电压依赖性离子电流对氟烷敏感,但Ca2+电流的两个成分对氟烷的敏感性高于GH3细胞中其他三个电压依赖性电流中的任何一个。这些结果表明,临床适当浓度的氟烷可选择性抑制GH3细胞的Ca2+电流,并且Ca2+电流的降低可以解释氟烷对GH3细胞中促甲状腺激素释放激素(TRH)或氯化钾(KCl)诱导的催乳素分泌的抑制作用。
