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大鼠培养星形胶质细胞中的电压门控氯电导。

A voltage-gated chloride conductance in rat cultured astrocytes.

作者信息

Gray P T, Ritchie J M

出版信息

Proc R Soc Lond B Biol Sci. 1986 Aug 22;228(1252):267-88. doi: 10.1098/rspb.1986.0055.

Abstract

Large voltage-dependent outward currents are recorded with the whole-cell patch-clamp technique from rat cultured astrocytes under conditions where an outward movement of potassium ions is excluded (either by blockage of the potassium channels pharmacologically or by replacement of the internal potassium by the impermeant large organic cation N-methyl-(+)-glucamine). The current, which is activated at potentials more positive than -40 to -50 mV, is normally carried by an inward movement of chloride ions. Its reversal potential is the same as the chloride equilibrium potential. With depolarization to +60 mV (for 225 ms) little or no inactivation of the current occurs: with depolarizations to +90 to +110 mV a time-dependent decay is seen. The current, which is often not marked immediately after formation of the whole-cell clamp, generally increases over a period of a few minutes to a maximum (after which it usually declines), as if some as yet unknown intracellular factor keeping the channels closed were being washed away from the membrane. The time course of this phenomenon is not affected by changing of the internal free calcium concentration (from 10(-8)M to 10(-6)M) or by an intracellular mixture of cyclic AMP (1 mM), ATP (4 mM) and Mg+ (2 mM). The conductance is slightly increased when the chloride of the bathing medium is replaced by bromide; is much reduced on replacement by methylsulphate, sulphate, isethionate, or acetate; and is virtually abolished on replacement by the large anion gluconate. The outward current is inhibited by the disulphonate stilbenes DIDS and SITS; this blocking action was initially partly reversible, although never completely so. It is suggested that the chloride conductance plays a role in the spatial buffering of potassium by astrocytes.

摘要

采用全细胞膜片钳技术,在排除钾离子外流的条件下(通过药理学方法阻断钾通道,或用不透膜的大有机阳离子N-甲基-(+)-葡糖胺替代细胞内钾离子),从大鼠培养的星形胶质细胞中记录到了大的电压依赖性外向电流。该电流在比-40至-50mV更正的电位下被激活,通常由氯离子的内向移动携带。其反转电位与氯平衡电位相同。去极化至+60mV(持续225毫秒)时,电流几乎没有或没有失活:去极化至+90至+110mV时,可观察到时间依赖性衰减。该电流在全细胞膜片钳形成后通常不会立即明显出现,一般在几分钟内增加到最大值(之后通常会下降),就好像某种尚未知晓的使通道关闭的细胞内因子正从膜上被洗脱。这种现象的时间进程不受细胞内游离钙浓度变化(从10(-8)M至10(-6)M)或细胞内环状AMP(1mM)、ATP(4mM)和Mg+(2mM)混合物的影响。当灌流液中的氯离子被溴离子替代时,电导略有增加;被甲基硫酸根、硫酸根、羟乙基磺酸根或醋酸根替代时,电导大幅降低;被大阴离子葡萄糖酸根替代时,电导几乎完全消失。外向电流受到二磺酸盐类芪化合物DIDS和SITS的抑制;这种阻断作用最初部分可逆,尽管从未完全可逆。提示氯电导在星形胶质细胞对钾的空间缓冲中起作用。

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