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大鼠脑片室旁大细胞神经元的电生理特性:血管紧张素 II 对 IA 电流的调制作用

Electrophysiological properties of paraventricular magnocellular neurons in rat brain slices: modulation of IA by angiotensin II.

作者信息

Li Z, Ferguson A V

机构信息

Department of Physiology, Queen's University, Kingston, Ontario, Canada.

出版信息

Neuroscience. 1996 Mar;71(1):133-45. doi: 10.1016/0306-4522(95)00434-3.

DOI:10.1016/0306-4522(95)00434-3
PMID:8834397
Abstract

Whole-cell patch-clamp recordings obtained from magnocellular neurons of the hypothalamic paraventricular nucleus in brain slice preparations of adult Sprague-Dawley rats have been utilized to examine three outward potassium conductances and the ionic mechanisms through which angiotensin II exerts its neurotransmitter actions within this region. Lucifer Yellow fills showed that neurons from which we recorded had large ovoid cell bodies 11-17 microns wide and 22-35 microns long, as well as 1-3 minimally branched processes, anatomical features in accordance with those previously described for magnocellular neuroendocrine neurons. These neurons had an average resting membrane potential of -58.3 +/- 0.9 (mean +/- S.E.M.) mV, spike amplitude of 92.8 +/- 1.4 mV, and input resistance of 788.9 +/- 50.4 M omega. Most of these cells displayed irregular or continuous spontaneous activity with a mean frequency of 2.44 +/- 0.33 Hz. Voltage-clamp recordings revealed three outward potassium currents; (1) a delayed outward current (IK), (2) a Ca(2+)-dependent outward current (IK(Ca)) and (3) a transient outward current (IA). These currents were classified according to their voltage dependence, inactivation, Ca2+ dependence and pharmacology. The IK was activated by depolarization beyond -40 mV and its amplitude consistently increased with depolarizing steps. The membrane conductance underlying this current was 27.3 +/- 3.8 nS for depolarization to +50 mV. In medium containing 2 mM Ca2+, depolarization to above -20 mV evoked a slowly-activating IK(Ca) which showed minimal inactivation. This current was suppressed in Ca(2+)-free/Co2+ medium and its membrane conductance was also smaller (19.4 +/- 3.5 nS at +50 mV) than that of IK. The IA demonstrated both fast activation and inactivation and was evoked only if depolarizing pulse steps were preceded by conditioning hyperpolarization. The activation threshold was approximately -65 mV and IA amplitude increased in non-linear fashion as test voltage steps became more positive. The 90% maximum of IA conductance was 15.7 +/- 1.1 nS, and was observed at membrane potentials around -15 mV. The reversal potentials of these currents were in accordance with the K+ equilibrium potential. Tetra-ethylammonium reversibly inhibited both the peak and steady-state currents of the IK, while 4-aminopyridine suppressed the IA. Replacement of 2 mM Ca2+ with 2 mM Co2+ in our bath solution or addition of Co2+ into Ca(2+)-free medium reduced the magnitude of IA, revealing the existence of a Co(2+)-sensitive IA. Bath administration of 10(-7) M angiotensin was without significant effect on IK, but resulted in a statistically significant reduction in IA (-31.0 +/- 4.1%) in 12 of 14 paraventricular nucleus cells tested, effects which were not observed following pretreatment with the AT1 receptor antagonist losartan. We conclude that in paraventricular nucleus magnocellular cells, like other CNS neurons, at least three sets of potassium channels contribute to the outward current evoked by depolarization. Our data also demonstrate ionic mechanisms through which angiotensin may act at AT1 receptors to influence the excitability of hypothalamic neuroendocrine cells.

摘要

从成年Sprague-Dawley大鼠脑片制备物中下丘脑室旁核的大细胞神经元获得的全细胞膜片钳记录,已被用于研究三种外向钾离子电导以及血管紧张素II在该区域发挥其神经递质作用的离子机制。荧光黄填充显示,我们记录的神经元具有大的卵圆形细胞体,宽11 - 17微米,长22 - 35微米,以及1 - 3个分支极少的突起,这些解剖特征与先前描述的大细胞神经内分泌神经元一致。这些神经元的平均静息膜电位为 -58.3 ± 0.9(平均值 ± 标准误)mV,动作电位幅度为92.8 ± 1.4 mV,输入电阻为788.9 ± 50.4 MΩ。这些细胞中的大多数表现出不规则或连续的自发活动,平均频率为2.44 ± 0.33 Hz。电压钳记录显示出三种外向钾电流;(1)延迟外向电流(IK),(2)钙依赖性外向电流(IK(Ca))和(3)瞬时外向电流(IA)。这些电流根据其电压依赖性、失活、钙依赖性和药理学特性进行分类。IK在去极化超过 -40 mV时被激活,其幅度随着去极化步骤持续增加。对于去极化到 +50 mV,该电流的膜电导为27.3 ± 3.8 nS。在含有2 mM钙的培养基中,去极化到 -20 mV以上会诱发缓慢激活的IK(Ca),其显示出最小的失活。该电流在无钙/钴培养基中被抑制,并且其膜电导(在 +50 mV时为19.4 ± 3.5 nS)也比IK小。IA表现出快速激活和失活,并且仅在去极化脉冲步骤之前进行预处理超极化时才被诱发。激活阈值约为 -65 mV,并且随着测试电压步骤变得更正,IA幅度以非线性方式增加。IA电导的90%最大值为15.7 ± 1.1 nS,并且在膜电位约为 -15 mV时观察到。这些电流的反转电位与钾离子平衡电位一致。四乙铵可逆地抑制IK的峰值和稳态电流,而4 - 氨基吡啶抑制IA。在我们的浴液中用2 mM钴替代2 mM钙或在无钙培养基中添加钴会降低IA的幅度,揭示了存在对钴敏感的IA。浴液中给予10(-7) M血管紧张素对IK没有显著影响,但在测试的14个室旁核细胞中的12个中导致IA有统计学意义地降低(-31.0 ± 4.1%),在用AT1受体拮抗剂氯沙坦预处理后未观察到这些效应。我们得出结论,在室旁核大细胞中,与其他中枢神经系统神经元一样,至少三组钾通道对去极化诱发的外向电流有贡献。我们的数据还证明了血管紧张素可能通过离子机制作用于AT1受体以影响下丘脑神经内分泌细胞的兴奋性。

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