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激活的大鼠小胶质细胞中的电压依赖性钾通道

Voltage-dependent potassium channels in activated rat microglia.

作者信息

Nörenberg W, Gebicke-Haerter P J, Illes P

机构信息

Department of Pharmacology, University of Freiburg, FRG.

出版信息

J Physiol. 1994 Feb 15;475(1):15-32. doi: 10.1113/jphysiol.1994.sp020046.

DOI:10.1113/jphysiol.1994.sp020046
PMID:7514664
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1160352/
Abstract
  1. Voltage-dependent currents of untreated (proliferating) and lipopolysaccharide (LPS)-treated rat microglial cells in culture were recorded using the whole-cell patch-clamp technique. 2. Membrane potentials showed prominent peaks at -35 mV and -70 mV. Membrane potentials of LPS-treated cells alternated between the two values. This may be due to a negative slope region of the I-V relation resulting in two zero current potentials. 3. From a holding potential of -70 mV, hyperpolarizing steps evoked an inwardly rectifying current both in proliferating and in LPS-treated cells, while depolarizing steps below -50 mV evoked an outwardly rectifying current only in LPS-treated microglia. The currents were K+ selective, as indicated by their reversal potential of approximately 0 mV in symmetric K+ concentrations (150 mM both intra- and extracellularly) and the reversal potential of the outward tail currents of approximately -90 mV at a normal extracellular K+ concentration (4.5 mM). 4. The activation of the outward current could be fitted by Hodgkin-Huxley-type n4 kinetics. The time constant of activation depended on voltage. 5. The inactivation of the inward and outward currents could be fitted by a single exponential. The time constant of the inward current inactivation was dependent on voltage, whereas the time constant of the outward current inactivation was virtually independent of voltage, except near the threshold of activation. Recovery of the outward from inactivation was slow and could be fitted by two exponentials. Responses to depolarizing steps were stable at 0.125 Hz, but greatly decreased from the first to the second pulse at 1 Hz. 6. The inactivation of the inward, but not of the outward, current disappeared in a low Na(+)-containing medium (5 mM). The inward current was selectively inhibited by extracellular Cs+ and Ba2+. The outward current was selectively inhibited by Cd2+, 4-aminopyridine and charybdotoxin. Replacement of intracellular K+ by an equimolar concentration of Cs+, and the extracellular application of tetraethylammonium and quinine inhibited both currents. 7. An increase of extracellular Ca2+ from 2 to 20 mM resulted in outwardly rectifying K+ channels activating at more positive potentials. Omission of Ca2+ from the extracellular medium had the opposite effect. When the intracellular free Ca2+ was increased from 0.01 to 1 microM, the outward current amplitudes were depressed. The Ca2+ ionophore A23187 had a similar effect. 8. LPS-treated microglial cells possess inwardly and outwardly rectifying K+ channels. The physiological and pharmacological characteristics of these two channel populations are markedly different.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 使用全细胞膜片钳技术记录培养的未处理(增殖)和脂多糖(LPS)处理的大鼠小胶质细胞的电压依赖性电流。2. 膜电位在 -35 mV 和 -70 mV 处显示出明显的峰值。LPS 处理细胞的膜电位在这两个值之间交替。这可能是由于 I-V 关系的负斜率区域导致两个零电流电位。3. 从 -70 mV 的钳制电位开始,超极化步骤在增殖细胞和 LPS 处理的细胞中均诱发内向整流电流,而低于 -50 mV 的去极化步骤仅在 LPS 处理的小胶质细胞中诱发外向整流电流。这些电流对 K+ 具有选择性,在对称 K+ 浓度(细胞内和细胞外均为 150 mM)下其反转电位约为 0 mV,在正常细胞外 K+ 浓度(4.5 mM)下外向尾电流的反转电位约为 -90 mV 表明了这一点。4. 外向电流的激活可以用霍奇金 - 赫胥黎型 n4 动力学拟合。激活的时间常数取决于电压。5. 内向和外向电流的失活可以用单指数拟合。内向电流失活的时间常数取决于电压,而外向电流失活的时间常数实际上与电压无关,除了在激活阈值附近。外向电流从失活状态的恢复很慢,可以用两个指数拟合。对去极化步骤的反应在 0.125 Hz 时稳定,但在 1 Hz 时从第一个脉冲到第二个脉冲大大降低。6. 在低 Na+ 培养基(5 mM)中,内向电流的失活消失,但外向电流的失活没有消失。内向电流被细胞外 Cs+ 和 Ba2+ 选择性抑制。外向电流被 Cd2+、4 - 氨基吡啶和蝎毒素选择性抑制。用等摩尔浓度的 Cs+ 替代细胞内 K+,以及细胞外应用四乙铵和奎宁会抑制两种电流。7. 细胞外 Ca2+ 从 2 mM 增加到 20 mM 导致外向整流 K+ 通道在更正的电位下激活。从细胞外培养基中省略 Ca2+ 则产生相反的效果。当细胞内游离 Ca2+ 从 0.01 μM 增加到 1 μM 时,外向电流幅度降低。Ca2+ 离子载体 A23187 有类似的效果。8. LPS 处理的小胶质细胞具有内向和外向整流 K+ 通道。这两种通道群体的生理和药理特性明显不同。(摘要截断于 400 字)

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