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利用膜片钳和荧光显微镜对单细胞电穿孔进行表征。

Characterization of single-cell electroporation by using patch-clamp and fluorescence microscopy.

作者信息

Ryttsén F, Farre C, Brennan C, Weber S G, Nolkrantz K, Jardemark K, Chiu D T, Orwar O

机构信息

Department of Chemistry, Göteborg University, Göteborg SE-412 96, Sweden.

出版信息

Biophys J. 2000 Oct;79(4):1993-2001. doi: 10.1016/S0006-3495(00)76447-2.

Abstract

Electroporation of single NG108-15 cells with carbon-fiber microelectrodes was characterized by patch-clamp recordings and fluorescence microscopy. To minimize adverse capacitive charging effects, the patch-clamp pipette was sealed on the cell at a 90(o) angle with respect to the microelectrodes where the applied potential reaches a minimum. From transmembrane current responses, we determined the electric field strengths necessary for ion-permeable pore formation and investigated the kinetics of pore opening and closing as well as pore open times. From both patch-clamp and fluorescence microscopy experiments, the threshold transmembrane potentials for dielectric breakdown of NG108-15 cells, using 1-ms rectangular waveform pulses, was approximately 250 mV. The electroporation pulse preceded pore formation, and analyte entry into the cells was dictated by concentration, and membrane resting potential driving forces. By stepwise moving a cell out of the focused field while measuring the transmembrane current response during a supramaximal pulse, we show that cells at a distance of approximately 30 microm from the focused field were not permeabilized.

摘要

使用碳纤维微电极对单个NG108 - 15细胞进行电穿孔,通过膜片钳记录和荧光显微镜进行表征。为了最小化不利的电容充电效应,膜片钳吸管相对于微电极以90°角密封在细胞上,此处施加的电位达到最小值。从跨膜电流响应中,我们确定了形成离子渗透孔所需的电场强度,并研究了孔打开和关闭的动力学以及孔开放时间。从膜片钳和荧光显微镜实验中,使用1毫秒矩形波形脉冲时,NG108 - 15细胞介电击穿的阈值跨膜电位约为250 mV。电穿孔脉冲先于孔的形成,分析物进入细胞由浓度和膜静息电位驱动力决定。通过在测量超最大脉冲期间的跨膜电流响应时逐步将细胞移出聚焦场,我们表明距离聚焦场约30微米处的细胞未被通透化。

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