应用Patchliner Dynamite8实时模拟人诱导多能干细胞衍生心肌细胞IK1的自动动态钳

Q2 Pharmacology, Toxicology and Pharmaceutics

Current Protocols in Pharmacology Pub Date : 2020-03-01 DOI:10.1002/cpph.70

Nadine Becker, András Horváth, Teun De Boer, Alan Fabbri, Christian Grad, Niels Fertig, Michael George, Alison Obergrussberger

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引用次数: 16

摘要

目前的体外检测通常很难预测心脏倾向，因为它们关注的是细胞系中过度表达的单离子通道。另一方面，人类诱导多能干细胞衍生的心肌细胞(hiPSC-CMs)为使用高通量系统对人类心肌细胞进行药物测试提供了独特的机会。然而，这些细胞在离子通道表达和电生理特性上与成人心肌细胞不同。hiPSC-CMs的主要挑战之一是离子通道的生理表达，如向内整流器(例如Kir2.1-2.3)，其传导心脏向内整流器钾电流(IK1)。IK1是维持心脏细胞静息膜电位稳定的主要贡献者之一，这对兴奋性至关重要。膜片钳研究表明，在hiPSC-CMs中，这种蛋白仅以低水平表达，有时根本不表达。动态箝位是一种将离子电流(例如IK1)引入细胞以补偿内源性表达缺失的方法，从而提供了在hiPSC-CMs中记录更稳定动作电位的潜力。在本文中，我们描述了在自动膜片钳装置(Patchliner)上使用hiPSC-CMs的方法，该方法与自动动态钳附件(Dynamite8)相结合。我们描述了在Patchliner上使用的优化细胞处理和收获的协议，以及在动态夹紧模式下自动执行实验和数据分析所需的步骤。©2019 by John Wiley & Sons, Inc。基本方案:在自动膜片钳结合动态钳中记录人类诱导多能干细胞衍生的心肌细胞的动作电位药理学，以引入模拟IK1和补偿密封阻力支持方案1:心肌细胞电镀和培养支持方案2:细胞收获和解离备用方案:在生理温度下记录动作电位药理学。

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Automated Dynamic Clamp for Simulation of I_K1 in Human Induced Pluripotent Stem Cell-Derived Cardiomyocytes in Real Time Using Patchliner Dynamite⁸.

Current in vitro assays typically poorly predict cardiac liability as they focus on single ion channels overexpressed in cell lines. Human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs), on the other hand, provide a unique opportunity for drug testing on human cardiomyocytes using high-throughput systems. However, these cells can differ from adult cardiomyocytes in their ion channel expression and, therefore, electrophysiologic properties. One of the main challenges of hiPSC-CMs is the physiologic expression of ion channels such as the inward rectifiers (e.g., Kir2.1-2.3), which conduct the cardiac inward rectifier potassium current (I_K1 ). I_K1 is one of the primary contributors in maintaining a stable resting membrane potential in cardiac cells, which is essential for excitability. This is only expressed in low levels, or sometimes not at all, in hiPSC-CMs as shown by patch clamp studies. Dynamic clamp is a method of electronically introducing ion currents (e.g., I_K1 ) into cells to compensate for the lack of endogenous expression, thus offering the potential to record more stable action potentials in hiPSC-CMs. In this article, we describe the method of using hiPSC-CMs on an automated patch clamp device (Patchliner) coupled with the automated dynamic clamp add-on (Dynamite⁸ ). We describe protocols for optimized cell handling and harvesting for use on the Patchliner and the steps required for automated execution of experiments and data analysis in dynamic clamp mode. © 2019 by John Wiley & Sons, Inc. Basic Protocol: Recording action potential pharmacology from human induced pluripotent stem cell-derived cardiomyocytes in automated patch clamp combined with dynamic clamp to introduce simulated I_K1 and compensate seal resistance Support Protocol 1: Cardiomyocyte plating and culture Support Protocol 2: Cell harvesting and dissociation Alternate Protocol: Recording action potential pharmacology at physiologic temperatures.

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Current Protocols in Pharmacology Pharmacology, Toxicology and Pharmaceutics-Pharmacology

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