合胞体中hSC CM的静息膜电位比分离细胞的静息膜电势更为超极化。

Dieter V Van de Sande, Ivan Kopljar, Alaerts Maaike, Ard Teisman, David J Gallacher, Loeys Bart, Dirk J Snyders, Luc Leybaert, Hua Rong Lu, Alain J Labro
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摘要

人诱导多能干细胞(hiPSC)和干细胞(hSC)衍生的心肌细胞(CM)作为心脏病学和药理学研究的体外模型越来越受欢迎。如单细胞电生理学特征所示,这些细胞的一个剩余缺陷是与天然CM相比,静息膜电位(RMP)更去极化。大多数报道将其归因于产生IK1电流的Kir2.1钾通道的低表达。然而,大多数RMP记录是从分离的hSC/hiPSC CM中获得的,而在更天然的环境中,这些细胞通过基于连接蛋白的间隙连接与相邻细胞互连,形成合胞体。由此,这些细胞被电连接并且IK1的总池增加。因此,互连电池的输入电阻(Ri)低于分离电池的输入阻抗。在膜片钳实验中,移液管需要很好地附着或密封到细胞上,这反映在密封电阻(Rs)中,因为非特异性离子电流可以通过移液管与细胞的接触或密封泄漏,并平衡细胞内的小电流,如IK1。通过记录分离的hSC CMs和在小单层中培养的hSC CM的动作电位,我们发现单层中的hSC CMs的RMP比分离的细胞高出约-20mV的超极化。因此,加入连接蛋白通道阻断剂碳烯酮,将被膜片钳的细胞与单层的相邻细胞分离,并使RMP去极化。所提供的数据显示,合胞体中hSC CM的记录RMP比从分离的hSC/hiPSC CM中确定的RMP更负,很可能是因为Kir2.1通道的活性池增加了。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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The resting membrane potential of hSC-CM in a syncytium is more hyperpolarised than that of isolated cells.

Human-induced pluripotent stem cell (hiPSC) and stem cell (hSC) derived cardiomyocytes (CM) are gaining popularity as in vitro model for cardiology and pharmacology studies. A remaining flaw of these cells, as shown by single-cell electrophysiological characterization, is a more depolarized resting membrane potential (RMP) compared to native CM. Most reports attribute this to a lower expression of the Kir2.1 potassium channel that generates the IK1 current. However, most RMP recordings are obtained from isolated hSC/hiPSC-CMs whereas in a more native setting these cells are interconnected with neighboring cells by connexin-based gap junctions, forming a syncytium. Hereby, these cells are electrically connected and the total pool of IK1 increases. Therefore, the input resistance (Ri) of interconnected cells is lower than that of isolated cells. During patch clamp experiments pipettes need to be well attached or sealed to the cell, which is reflected in the seal resistance (Rs), because a nonspecific ionic current can leak through this pipette-cell contact or seal and balance out small currents within the cell such as IK1. By recording the action potential of isolated hSC-CMs and that of hSC-CMs cultured in small monolayers, we show that the RMP of hSC-CMs in monolayer is approximately -20 mV more hyperpolarized compared to isolated cells. Accordingly, adding carbenoxolone, a connexin channel blocker, isolates the cell that is patch clamped from its neighboring cells of the monolayer and depolarizes the RMP. The presented data show that the recorded RMP of hSC-CMs in a syncytium is more negative than that determined from isolated hSC/hiPSC-CMs, most likely because the active pool of Kir2.1 channels increased.

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