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细胞贴附式与外翻式膜片中钙激活钾通道电流的比较。

A comparison of calcium-activated potassium channel currents in cell-attached and excised patches.

作者信息

Pallotta B S, Hepler J R, Oglesby S A, Harden T K

出版信息

J Gen Physiol. 1987 Jun;89(6):985-97. doi: 10.1085/jgp.89.6.985.

Abstract

Single channel currents from Ca-activated K channels were recorded from cell-attached patches, which were then excised from 1321N1 human astrocytoma cells. Cells were depolarized with K (110 mM) so that the membrane potential was known in both patch configurations, and the Ca ionophore A23187 or ionomycin (20-100 microM) was used to equilibrate intracellular and extracellular [Ca] (0.3 or 1 microM). Measurements of intracellular [Ca] with the fluorescent Ca indicator quin2 verified that [Ca] equilibration apparently occurred in our experiments. Under these conditions, where both membrane potential and intracellular [Ca] were known, we found that the dependence of the channel percent open time on membrane potential and [Ca] was similar in both the cell-attached and excised patch configuration for several minutes after excision. Current-voltage relations were also similar, and autocorrelation functions constructed from the single channel currents revealed no obvious change in channel gating upon patch excision. These findings suggest that the results of studies that use excised membrane patches can be extrapolated to the K-depolarized cell-attached configuration, and that the relation between [Ca] and channel activity can be used to obtain a quantitative measure of [Ca] near the membrane intracellular surface.

摘要

从1321N1人星形细胞瘤细胞上记录钙激活钾通道的单通道电流,记录采用细胞贴附式膜片钳模式,之后将膜片从细胞上分离下来。用110 mM的钾使细胞去极化,这样在两种膜片钳模式下膜电位都是已知的,使用钙离子载体A23187或离子霉素(20 - 100 μM)来平衡细胞内和细胞外的[Ca](0.3或1 μM)。用荧光钙指示剂quin2测量细胞内[Ca],证实我们的实验中[Ca]平衡明显发生。在这些膜电位和细胞内[Ca]都已知的条件下,我们发现,在分离后的几分钟内,细胞贴附式和分离式膜片钳模式下,通道开放时间百分比对膜电位和[Ca]的依赖性相似。电流 - 电压关系也相似,由单通道电流构建的自相关函数显示,膜片分离后通道门控没有明显变化。这些发现表明,使用分离膜片的研究结果可以外推到钾去极化的细胞贴附式模式,并且[Ca]与通道活性之间的关系可用于定量测量膜内表面附近的[Ca]。

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