Long-term changes in transmembrane voltage after electroporation are governed by the interplay between nonselective leak current and ion channel activation

去极化 电穿孔 膜电位 超极化(物理学) 生物物理学 离子通道 化学 钾通道 门控 细胞内 膜透性 跨膜蛋白 静息电位 生物化学 生物 受体 有机化学 核磁共振波谱 基因
作者
Anja Blažič,Manon Guinard,Tomaž Leskovar,Rodney P. O’Connor,Lea Rems
出处
期刊:Bioelectrochemistry [Elsevier]
卷期号:161: 108802-108802
标识
DOI:10.1016/j.bioelechem.2024.108802
摘要

Electroporation causes a temporal increase in cell membrane permeability and leads to prolonged changes in transmembrane voltage (TMV) in both excitable and non-excitable cells. However, the mechanisms of these TMV changes remain to be fully elucidated. To this end, we monitored TMV over 30 min after exposing two different cell lines to a single 100 µs electroporation pulse using the FLIPR Membrane Potential dye. In CHO-K1 cells, which express very low levels of endogenous ion channels, membrane depolarization following pulse exposure could be explained by nonselective leak current, which persists until the membrane reseals, enabling the cells to recover their resting TMV. In U-87 MG cells, which express many different ion channels, we unexpectedly observed membrane hyperpolarization following the initial depolarization phase, but only at 33 °C and not at 25 °C. We developed a theoretical model, supported by experiments with ion channel inhibitors, which indicated that hyperpolarization could largely be attributed to the activation of calcium-activated potassium channels. Ion channel activation, coupled with changes in TMV and intracellular calcium, participates in various physiological processes, including cell proliferation, differentiation, migration, and apoptosis. Therefore, our study suggests that ion channels could present a potential target for influencing the biological response after electroporation.

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