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稳定转染细胞中的连接蛋白32间隙连接通道:单通道电导

Connexin32 gap junction channels in stably transfected cells: unitary conductance.

作者信息

Moreno A P, Eghbali B, Spray D C

机构信息

Department of Neuroscience, Albert Einstein College of Medicine, Bronx, New York 10461.

出版信息

Biophys J. 1991 Nov;60(5):1254-66. doi: 10.1016/S0006-3495(91)82159-2.

Abstract

Pairs of SKHep1 cells, which are derived from a highly metastatic human hepatoma, were studied using the whole cell voltage clamp technique with patch-type electrodes containing CsCl as the major ionic species. In 12 of 81 cell pairs, current flow through junctional membranes was detectable; in the remaining 69 cell pairs, junctional conductance was less than the noise limit of our recording apparatus (worst case: 10 pS). Macroscopic junctional conductance (gj) in the small percentage of pairs where it was detectable ranged from 100 to 600 pS. Unitary junctional conductance (gamma j) determined in the lowest conductance pairs or after reducing conductance with a short exposure to the uncoupling agent halothane was 25-35 pS. To study properties of gap junction channels formed of connexin32, the parental SKHep1 cell line was stably transfected with a plasmid containing cDNA that encodes connexin32, the major gap junction protein of rat liver cells. In 85 of 98 pairs of voltage clamped connexin32-transfected SKHep1 cells, macroscopic gj was greater than 1 nS; gj increased with time after dissociation (from 1.8 +/- 0.6 [mean +/- SE; n = 7] nS at 2 h after plating to 9.3 +/- 2.2 [n = 9] nS, the maximal value, at 24 h). Unitary conductance of gap junction channels between pairs of transfected SKHep1 cells was measured in low conductance pairs and after reducing gj by exposure to halothane or heptanol. Histograms of gamma j values in transfected cells, in 10 experiments where greater than 100 transitions were measurable, displayed two peaks; 120-130 pS and 25-35 pS. The smaller size corresponded to channels that were occasionally detected in the parental cells. We therefore conclude that connexin32 forms gap junctions channels of the 120-130 pS size class.

摘要

采用全细胞电压钳技术,使用以CsCl作为主要离子成分的膜片型电极,对源自高转移性人肝癌的SKHep1细胞对进行了研究。在81对细胞中,有12对可检测到通过连接膜的电流;在其余69对细胞中,连接电导小于我们记录设备的噪声极限(最坏情况:10 pS)。在可检测到连接电导的小部分细胞对中,宏观连接电导(gj)范围为100至600 pS。在电导最低的细胞对中或用解偶联剂氟烷短暂处理降低电导后测定的单位连接电导(γj)为25 - 35 pS。为了研究由连接蛋白32形成的间隙连接通道的特性,将亲本SKHep1细胞系用含有编码连接蛋白32(大鼠肝细胞的主要间隙连接蛋白)的cDNA的质粒进行稳定转染。在98对电压钳制的转染连接蛋白32的SKHep1细胞中,有85对宏观gj大于1 nS;gj在解离后随时间增加(从接种后2小时的1.8±0.6[平均值±标准误;n = 7] nS增加到接种后24小时的9.3±2.2[n = 9] nS,最大值)。在低电导细胞对中以及通过暴露于氟烷或庚醇降低gj后,测量了转染的SKHep1细胞对之间间隙连接通道的单位电导。在10次可测量超过100次转变的实验中,转染细胞中γj值的直方图显示出两个峰值;120 - 130 pS和25 - 35 pS。较小的尺寸对应于在亲本细胞中偶尔检测到的通道。因此,我们得出结论,连接蛋白32形成120 - 130 pS尺寸类别的间隙连接通道。

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