Heart rhythm in vitro: measuring stem cell-derived pacemaker cells on microelectrode arrays

Sophie Kussauer; Patrick Dilk; Moustafa Elleisy; Claudia Michaelis; Sarina Lichtwark; Christian Rimmbach; Robert David; Julia Jung

doi:10.3389/fcvm.2024.1200786

Heart rhythm in vitro: measuring stem cell-derived pacemaker cells on microelectrode arrays

Front Cardiovasc Med. 2024 Feb 21:11:1200786. doi: 10.3389/fcvm.2024.1200786. eCollection 2024.

Authors

Sophie Kussauer^{1

2}, Patrick Dilk^{1

2}, Moustafa Elleisy^{1

2}, Claudia Michaelis^{1

2}, Sarina Lichtwark^{1

2}, Christian Rimmbach^{1

2}, Robert David^{1

2}, Julia Jung^{1

2}

Affiliations

¹ Department of Cardiac Surgery, Rostock University Medical Centre, Rostock, Germany.
² Department of Life, Light, & Matter, University of Rostock, Rostock, Germany.

Abstract

Background: Cardiac arrhythmias have markedly increased in recent decades, highlighting the urgent need for appropriate test systems to evaluate the efficacy and safety of new pharmaceuticals and the potential side effects of established drugs.

Methods: The Microelectrode Array (MEA) system may be a suitable option, as it provides both real-time and non-invasive monitoring of cellular networks of spontaneously active cells. However, there is currently no commercially available cell source to apply this technology in the context of the cardiac conduction system (CCS). In response to this problem, our group has previously developed a protocol for the generation of pure functional cardiac pacemaker cells from mouse embryonic stem cells (ESCs). In addition, we compared the hanging drop method, which was previously utilized, with spherical plate-derived embryoid bodies (EBs) and the pacemaker cells that are differentiated from these.

Results: We described the application of these pacemaker cells on the MEA platform, which required a number of crucial optimization steps in terms of coating, dissociation, and cell density. As a result, we were able to generate a monolayer of pure pacemaker cells on an MEA surface that is viable and electromechanically active for weeks. Furthermore, we introduced spherical plates as a convenient and scalable method to be applied for the production of induced sinoatrial bodies.

Conclusion: We provide a tool to transfer modeling and analysis of cardiac rhythm diseases to the cell culture dish. Our system allows answering CCS-related queries within a cellular network, both under baseline conditions and post-drug exposure in a reliable and affordable manner. Ultimately, our approach may provide valuable guidance not only for cardiac pacemaker cells but also for the generation of an MEA test platform using other sensitive non-proliferating cell types.

Keywords: cardiomyocytes; conduction velocity; embryoid bodies; in vitro drug testing; microelectrode array; pacemaker cells.

Grants and funding

SK and RD are supported by the EU Structural Fund (ESF/14-BM-A55–0024/18), the German Federal Ministry for Economic Affairs and Climate Action (16KN083635) and German Federal Office for Agriculture and Food (281A819B21). In addition, SK is supported by the DFG (VA1797/1-1). JJ is supported by the BMBF (VIP+00240, 031L0106C) and the DFG (DA1296/6-1). Moreover, RD is supported by the DFG (DA1296/6-1), the DAMP Foundation, the German Heart Foundation (F/01/12) and the BMBF (VIP+00240).