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大鼠海马星形胶质细胞内的钠稳态

Intracellular sodium homeostasis in rat hippocampal astrocytes.

作者信息

Rose C R, Ransom B R

机构信息

Department of Neurology, Yale University School of Medicine, New Haven, CT 06520, USA.

出版信息

J Physiol. 1996 Mar 1;491 ( Pt 2)(Pt 2):291-305. doi: 10.1113/jphysiol.1996.sp021216.

DOI:10.1113/jphysiol.1996.sp021216
PMID:8866855
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1158726/
Abstract
  1. We determined the intracellular Na+ concentration ([Na+]i) and mechanisms of its regulation in cultured rat hippocampal astrocytes using fluorescence ratio imaging of the Na+ indicator SBFI-AM (acetoxymethylester of sodium-binding benzofuran isophthalate, 10 microM). Dye signal calibration within the astrocytes showed that the ratiometric dye signal changed monotonically with changes in [Na+]i from 0 to 140 nM. The K+ sensitivity of the dye was negligible; intracellular pH changes, however, slightly affected the 'Na+' signal. 2. Baseline [Na+]i was 14.6 +/- 4.9 mM (mean +/- S.D.) in CO2/HCO3(-)-containing saline with 3 mM K+. Removal of extracellular Na+ decreased [Na+]i in two phases: a rapid phase of [Na+]i reduction (0.58 +/- 0.32 mM min-1) followed by a slower phase (0.15 +/- 0.09 mM min-1). 3. Changing from CO2/HCO3(-)-free to CO2/HCO3(-)-buffered saline resulted in a transient increase in [Na+]i of approximately 5 mM, suggesting activation of inward Na(+)-HCO3- cotransport by CO2/HCO3-. During furosemide (frusemide, 1 mM) or bumetanide (50 microM) application, a slow decrease in [Na+]i of approximately 2 mM was observed, indicating a steady inward transport of Na+ via Na(+)-K(+)-2Cl- cotransport under control conditions. Tetrodotoxin (100 microM) did not influence [Na+]i in the majority of cells (85%), suggesting that influx of Na+ through voltage-gated Na+ channels contributed to baseline [Na+]i in only a small subpopulation of hippocampal astrocytes. 4. Blocking Na+, K(+)-ATPase activity with cardiac glycosides (ouabain or strophanthidin, 1 mM) or removal of extracellular K+ led to an increase in [Na+]i of about 2 and 4 mM min-1, respectively. This indicated that Na+, K(+)-ATPase activity was critical in maintaining low [Na+]i in the face of a steep electrochemical gradient, which would favour a much higher [Na+]i. 5. Elevation of extracellular K+ concentration ([K+]o) by as little as 1 mM (from 3 to 4 mM) resulted in a rapid and reversible decrease in [Na+]i. Both the slope and the amplitude of the [K+]o-induced reductions in [Na+]i were sensitive to bumetanide. A reduction of [K+]o by 1 mM increased [Na+]i by 3.0 +/- 2.3 mM. In contrast, changing extracellular Na+ concentration by 20 mM resulted in changes in [Na+]i of less than 3 mM. 6. These results implied that in hippocampal astrocytes low baseline [Na+]i is determined by the action of Na(+)-HCO3- cotransport, Na(+)-K(+)-2Cl- cotransport and Na+, K(+)-ATPase, and that both Na+, K(+)-ATPase and inward Na(+)-K(+)-2Cl cotransport are activated by small, physiologically relevant increases in [K+]o. These mechanisms are well suited to help buffer increases in [K+]o associated with neural activity.
摘要
  1. 我们使用钠离子指示剂SBFI-AM(钠结合苯并呋喃间苯二甲酸乙酰氧甲酯,10微摩尔)的荧光比率成像技术,测定了培养的大鼠海马星形胶质细胞内的钠离子浓度([Na⁺]i)及其调节机制。星形胶质细胞内的染料信号校准显示,比率染料信号随[Na⁺]i从0到140纳摩尔的变化而单调变化。染料对钾离子的敏感性可忽略不计;然而,细胞内pH值的变化对“Na⁺”信号有轻微影响。2. 在含3毫摩尔钾离子的二氧化碳/碳酸氢根(-)缓冲盐溶液中,基线[Na⁺]i为14.6±4.9毫摩尔(平均值±标准差)。去除细胞外钠离子会使[Na⁺]i分两个阶段降低:[Na⁺]i快速降低阶段(0.58±0.32毫摩尔/分钟),随后是较慢阶段(0.15±0.09毫摩尔/分钟)。3. 从无二氧化碳/碳酸氢根(-)的缓冲盐溶液换成二氧化碳/碳酸氢根(-)缓冲盐溶液,会使[Na⁺]i瞬时增加约5毫摩尔,这表明二氧化碳/碳酸氢根(-)激活了内向钠-碳酸氢根共转运。在应用呋塞米(速尿,1毫摩尔)或布美他尼(50微摩尔)期间,观察到[Na⁺]i缓慢降低约2毫摩尔,这表明在对照条件下,通过钠-钾-2氯共转运存在稳定的内向钠离子转运。河豚毒素(100微摩尔)对大多数细胞(85%)的[Na⁺]i没有影响,这表明通过电压门控钠离子通道的钠离子内流仅在一小部分海马星形胶质细胞中对基线[Na⁺]i有贡献。4. 用强心苷(哇巴因或毒毛花苷,1毫摩尔)阻断钠-钾-ATP酶活性或去除细胞外钾离子,分别导致[Na⁺]i以约2和4毫摩尔/分钟的速度增加。这表明在面对陡峭的电化学梯度时,钠-钾-ATP酶活性对于维持低[Na⁺]i至关重要,否则[Na⁺]i会高得多。5. 细胞外钾离子浓度([K⁺]o)仅升高1毫摩尔(从3毫摩尔升至4毫摩尔)就会导致[Na⁺]i迅速且可逆地降低。[K⁺]o诱导的[Na⁺]i降低的斜率和幅度对布美他尼都敏感。[K⁺]o降低1毫摩尔会使[Na⁺]i增加3.0±2.3毫摩尔。相比之下,细胞外钠离子浓度变化20毫摩尔导致[Na⁺]i变化小于3毫摩尔。6. 这些结果表明,在海马星形胶质细胞中,低基线[Na⁺]i由钠-碳酸氢根共转运、钠-钾-2氯共转运和钠-钾-ATP酶的作用决定,并且钠-钾-ATP酶和内向钠-钾-2氯共转运都会被生理相关的[K⁺]o小幅升高激活。这些机制非常适合帮助缓冲与神经活动相关的[K⁺]o升高。

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Astrocyte Na+ channels are required for maintenance of Na+/K(+)-ATPase activity.星形胶质细胞的钠离子通道是维持钠钾ATP酶活性所必需的。
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