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单个新鲜分离的平滑肌细胞膜的被动特性。

Passive properties of the membrane of single freshly isolated smooth muscle cells.

作者信息

Singer J J, Walsh J V

出版信息

Am J Physiol. 1980 Nov;239(5):C153-61. doi: 10.1152/ajpcell.1980.239.5.C153.

DOI:10.1152/ajpcell.1980.239.5.C153
PMID:6776818
Abstract

Single, smooth muscle cells were isolated from the stomach muscularis of the toad Bufo marinus and studied on the same day as isolation using standard electrophysiological techniques and direct microscopic observation at high magnification. Following penetration a period of hyperpolarization occurred that appeared to be caused by an increase in K+ conductance activated by Ca2+ entering the cell upon penetration. Ion substitution studies showed that the stable steady-state resting potential was dependent on both [Na+]0 and [K+]0. At [Ca2+]0 = 1.8 mM, active responses could be elicited which, at the higher [Ca2+]0 (< 8mM) generally employed, became action potentials with overshoots. Calculations employing the equations for a short cable and the observed change of membrane potential as a single exponential in response to a small hyperpolarizing current step both indicated that the length constant (lambda) was sufficiently greater than the cell length so that the cell behaved as an isopotential surface during subthreshold perturbations. From photomicrographic measurements of each cell studied and the input resistance, values of specific membrane resistance (Rm) were obtained that ranged as high as 152 k omega x cm2 depending on the ionic environment, most notably on [Ca2+]0. The membrane capacity (Cm) referred to the surface area measured with light microscopy was 1.3 +/- 0.3 microF/cm2 (mean +/- SD). When the best estimate of caveolar membrane area was included, Cm referred to total membrane area (caveolar plus noncaveolar) was approximately 0.8 microF/cm2.

摘要

从海蟾蜍(Bufo marinus)的胃肌层中分离出单个平滑肌细胞,并在分离当天使用标准电生理技术和高倍直接显微镜观察进行研究。刺入细胞后会出现一段超极化期,这似乎是由于刺入时Ca2+进入细胞激活了K+电导增加所致。离子替代研究表明,稳定的稳态静息电位取决于[Na+]0和[K+]0两者。在[Ca2+]0 = 1.8 mM时,可引发主动反应,在通常使用的较高[Ca2+]0(<8 mM)时,会变成具有超射的动作电位。使用短电缆方程以及观察到的膜电位作为对小超极化电流阶跃响应的单指数变化进行的计算均表明,长度常数(lambda)足够大于细胞长度,因此在阈下扰动期间细胞表现为等电位表面。根据对每个研究细胞的显微照片测量和输入电阻,获得了比膜电阻(Rm)值,其范围高达152 k omega x cm2,这取决于离子环境,最显著的是取决于[Ca2+]0。根据光学显微镜测量的表面积计算的膜电容(Cm)为1.3 +/- 0.3 microF/cm2(平均值 +/- 标准差)。当包括小窝膜面积的最佳估计值时,相对于总膜面积(小窝膜加非小窝膜)的Cm约为0.8 microF/cm2。

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