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利用 FluoVolt 染料研究 200 纳秒脉冲电场对神经元的激发和穿孔:光学膜电位。

Neuronal excitation and permeabilization by 200-ns pulsed electric field: An optical membrane potential study with FluoVolt dye.

机构信息

Frank Reidy Research Center for Bioelectrics, Old Dominion University, Norfolk, VA, USA.

Frank Reidy Research Center for Bioelectrics, Old Dominion University, Norfolk, VA, USA.

出版信息

Biochim Biophys Acta Biomembr. 2017 Jul;1859(7):1273-1281. doi: 10.1016/j.bbamem.2017.04.016. Epub 2017 Apr 18.

Abstract

Electric field pulses of nano- and picosecond duration are a novel modality for neurostimulation, activation of Ca signaling, and tissue ablation. However it is not known how such brief pulses activate voltage-gated ion channels. We studied excitation and electroporation of hippocampal neurons by 200-ns pulsed electric field (nsPEF), by means of time-lapse imaging of the optical membrane potential (OMP) with FluoVolt dye. Electroporation abruptly shifted OMP to a more depolarized level, which was reached within <1ms. The OMP recovery started rapidly (τ=8-12ms) but gradually slowed down (to τ>10s), so cells remained above the resting OMP level for at least 20-30s. Activation of voltage-gated sodium channels (VGSC) enhanced the depolarizing effect of electroporation, resulting in an additional tetrodotoxin-sensitive OMP peak in 4-5ms after nsPEF. Omitting Ca in the extracellular solution did not reduce the depolarization, suggesting no contribution of voltage-gated calcium channels (VGCC). In 40% of neurons, nsPEF triggered a single action potential (AP), with the median threshold of 3kV/cm (range: 1.9-4kV/cm); no APs could be evoked by stimuli below the electroporation threshold (1.5-1.9kV/cm). VGSC opening could already be detected in 0.5ms after nsPEF, which is too fast to be mediated by the depolarizing effect of electroporation. The overlap of electroporation and AP thresholds does not necessarily reflect the causal relation, but suggests a low potency of nsPEF, as compared to conventional electrostimulation, for VGSC activation and AP induction.

摘要

纳秒和皮秒时长的电场脉冲是一种新型的神经刺激、钙信号激活和组织消融模式。然而,目前尚不清楚如此短暂的脉冲如何激活电压门控离子通道。我们通过 FluoVolt 染料对海马神经元进行延时成像,研究了 200 纳秒脉冲电场(nsPEF)的激发和电穿孔作用。电穿孔会突然将膜电位(OMP)移至更去极化的水平,这一过程在 <1ms 内完成。OMP 的恢复迅速开始(τ=8-12ms),但逐渐减慢(至 τ>10s),因此细胞在至少 20-30s 内保持在高于静息 OMP 水平的状态。电压门控钠离子通道(VGSC)的激活增强了电穿孔的去极化效应,导致在 nsPEF 后 4-5ms 出现额外的河豚毒素敏感的 OMP 峰。在细胞外液中去除 Ca 并没有减少去极化,这表明电压门控钙通道(VGCC)没有贡献。在 40%的神经元中,nsPEF 触发单个动作电位(AP),其阈值中位数为 3kV/cm(范围:1.9-4kV/cm);低于电穿孔阈值(1.5-1.9kV/cm)的刺激不能引发 AP。在 nsPEF 后 0.5ms 即可检测到 VGSC 的开放,这一速度太快,不可能是由电穿孔的去极化效应介导的。电穿孔和 AP 阈值的重叠不一定反映因果关系,但表明与传统电刺激相比,nsPEF 对 VGSC 激活和 AP 诱导的效力较低。

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