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大鼠神经垂体神经末梢中一种新型的大电导钙激活钾通道及电流

A novel large-conductance Ca(2+)-activated potassium channel and current in nerve terminals of the rat neurohypophysis.

作者信息

Wang G, Thorn P, Lemos J R

机构信息

Worcester Foundation for Experimental Biology, Shrewsbury, MA 01545.

出版信息

J Physiol. 1992 Nov;457:47-74. doi: 10.1113/jphysiol.1992.sp019364.

DOI:10.1113/jphysiol.1992.sp019364
PMID:1284313
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1175717/
Abstract
  1. Nerve terminals of the rat posterior pituitary were acutely dissociated and identified using a combination of morphological and immunohistochemical techniques. Terminal membrane currents were studied using the 'whole-cell' patch clamp technique and channels were studied using inside-out and outside-out patches. 2. In physiological solutions, but with 7 mM 4-aminopyridine (4-AP), depolarizing voltage clamp steps from different holding potentials (-90 or -50 mV) elicited a fast, inward current followed by a slow, sustained, outward current. This outward current did not appear to show any steady-state inactivation. 3. The threshold for activation of the outward current was -30 mV and the current-voltage relation was 'bell-shaped'. The amplitude increased with increasingly depolarized potential steps. The outward current reversal potential was measured using tail current analysis and was consistent with that of a potassium current. 4. The sustained potassium current was determined to be dependent on the concentration of intracellular calcium. Extracellular Cd2+ (80 microM), a calcium channel blocker, also reversibly abolished the outward current. 5. The current was delayed in onset and was sustained over the length of a 150 ms-duration depolarizing pulse. The outward current reached a peak plateau and then decayed slowly. The decay was fitted by a single exponential with a time constant of 9.0 +/- 2.2 s. The decay constants did not show a dependence on voltage but rather on intracellular Ca2+. The time course of recovery from this decay was complex with full recovery taking > 190 s. 6. 4-AP (7 mM), dendrotoxin (100 nM), apamin (40-80 nM), and charybdotoxin (10-100 nM) had no effect on the sustained outward current. In contrast Ba2+ (200 microM) and tetraethylammonium inhibited the current, the latter in a dose-dependent manner (apparent concentration giving 50% of maximal inhibition (IC50) = 0.51 mM). 7. The neurohypophysial terminal outward current recorded here corresponds most closely to a Ca(2+)-activated K+ current (IK(Ca)) and not to a delayed rectifier or IA-like current. It also has properties different from that of the Ca(2+)-dependent outward current described in the magnocellular neuronal cell bodies of the hypothalamus. 8. A large conductance channel is often observed in isolated rat neurohypophysial nerve terminals. The channel had a unit conductance of 231 pS in symmetrical 150 mM K+.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 运用形态学和免疫组织化学技术相结合的方法,对大鼠垂体后叶的神经末梢进行急性分离并鉴定。采用“全细胞”膜片钳技术研究终末膜电流,运用内面向外和外面向内的膜片研究通道。2. 在生理溶液中,但含有7 mM 4 - 氨基吡啶(4 - AP)时,从不同的钳制电位(-90或-50 mV)进行去极化电压钳制步骤,会引发一个快速的内向电流,随后是一个缓慢、持续的外向电流。该外向电流似乎未表现出任何稳态失活。3. 外向电流激活的阈值为-30 mV,电流-电压关系呈“钟形”。随着去极化电位阶跃增加,电流幅度增大。使用尾电流分析测量外向电流反转电位,其与钾电流的反转电位一致。4. 确定持续的钾电流依赖于细胞内钙的浓度。细胞外Cd2 +(80 microM),一种钙通道阻滞剂,也能可逆地消除外向电流。5. 电流起始有延迟,并在150 ms持续时间的去极化脉冲期间持续存在。外向电流达到一个峰值平台,然后缓慢衰减。衰减过程用单指数拟合,时间常数为9.0±2.2 s。衰减常数不依赖于电压,而是依赖于细胞内Ca2 +。从这种衰减中恢复的时间进程很复杂,完全恢复需要>190 s。6. 4 - AP(7 mM)、树突毒素(100 nM)、蜂毒明肽(40 - 80 nM)和蝎毒素(10 - 100 nM)对持续的外向电流无影响。相比之下,Ba2 +(200 microM)和四乙铵抑制该电流,后者呈剂量依赖性(产生50%最大抑制的表观浓度(IC50)= 0.51 mM)。7. 此处记录的神经垂体终末外向电流最符合钙激活钾电流(IK(Ca)),而不是延迟整流电流或IA样电流。它也具有与下丘脑大细胞神经元胞体中描述的钙依赖性外向电流不同的特性。8. 在分离的大鼠神经垂体神经末梢中经常观察到一个大电导通道。在对称的150 mM K +中,该通道的单位电导为231 pS。(摘要截断于400字)

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