Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.

Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.

Recent advances have made it possible to readily derive cardiac myocytes from human induced pluripotent stem cells (hiPSC-CMs). HiPSC-CMs represent a valuable new experimental model for studying human cardiac muscle physiology and disease. Many laboratories have devoted substantial effort to examini...

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Main Authors: Matthew Wheelwright, Zaw Win, Jennifer L Mikkila, Kamilah Y Amen, Patrick W Alford, Joseph M Metzger
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2018-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC5884520?pdf=render
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spelling doaj-caf9cb36c65b4daba1edc969b79984a82020-11-25T00:04:27ZengPublic Library of Science (PLoS)PLoS ONE1932-62032018-01-01134e019490910.1371/journal.pone.0194909Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.Matthew WheelwrightZaw WinJennifer L MikkilaKamilah Y AmenPatrick W AlfordJoseph M MetzgerRecent advances have made it possible to readily derive cardiac myocytes from human induced pluripotent stem cells (hiPSC-CMs). HiPSC-CMs represent a valuable new experimental model for studying human cardiac muscle physiology and disease. Many laboratories have devoted substantial effort to examining the functional properties of isolated hiPSC-CMs, but to date, force production has not been adequately characterized. Here, we utilized traction force microscopy (TFM) with micro-patterning cell printing to investigate the maximum force production of isolated single hiPSC-CMs under varied culture and assay conditions. We examined the role of length of differentiation in culture and the effects of varied extracellular calcium concentration in the culture media on the maturation of hiPSC-CMs. Results show that hiPSC-CMs developing in culture for two weeks produced significantly less force than cells cultured from one to three months, with hiPSC-CMs cultured for three months resembling the cell morphology and function of neonatal rat ventricular myocytes in terms of size, dimensions, and force production. Furthermore, hiPSC-CMs cultured long term in conditions of physiologic calcium concentrations were larger and produced more force than hiPSC-CMs cultured in standard media with sub-physiological calcium. We also examined relationships between cell morphology, substrate stiffness and force production. Results showed a significant relationship between cell area and force. Implementing directed modifications of substrate stiffness, by varying stiffness from embryonic-like to adult myocardium-like, hiPSC-CMs produced maximal forces on substrates with a lower modulus and significantly less force when assayed on increasingly stiff adult myocardium-like substrates. Calculated strain energy measurements paralleled these findings. Collectively, these findings further establish single cell TFM as a valuable approach to illuminate the quantitative physiological maturation of force in hiPSC-CMs.http://europepmc.org/articles/PMC5884520?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Matthew Wheelwright
Zaw Win
Jennifer L Mikkila
Kamilah Y Amen
Patrick W Alford
Joseph M Metzger
spellingShingle Matthew Wheelwright
Zaw Win
Jennifer L Mikkila
Kamilah Y Amen
Patrick W Alford
Joseph M Metzger
Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.
PLoS ONE
author_facet Matthew Wheelwright
Zaw Win
Jennifer L Mikkila
Kamilah Y Amen
Patrick W Alford
Joseph M Metzger
author_sort Matthew Wheelwright
title Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.
title_short Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.
title_full Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.
title_fullStr Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.
title_full_unstemmed Investigation of human iPSC-derived cardiac myocyte functional maturation by single cell traction force microscopy.
title_sort investigation of human ipsc-derived cardiac myocyte functional maturation by single cell traction force microscopy.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2018-01-01
description Recent advances have made it possible to readily derive cardiac myocytes from human induced pluripotent stem cells (hiPSC-CMs). HiPSC-CMs represent a valuable new experimental model for studying human cardiac muscle physiology and disease. Many laboratories have devoted substantial effort to examining the functional properties of isolated hiPSC-CMs, but to date, force production has not been adequately characterized. Here, we utilized traction force microscopy (TFM) with micro-patterning cell printing to investigate the maximum force production of isolated single hiPSC-CMs under varied culture and assay conditions. We examined the role of length of differentiation in culture and the effects of varied extracellular calcium concentration in the culture media on the maturation of hiPSC-CMs. Results show that hiPSC-CMs developing in culture for two weeks produced significantly less force than cells cultured from one to three months, with hiPSC-CMs cultured for three months resembling the cell morphology and function of neonatal rat ventricular myocytes in terms of size, dimensions, and force production. Furthermore, hiPSC-CMs cultured long term in conditions of physiologic calcium concentrations were larger and produced more force than hiPSC-CMs cultured in standard media with sub-physiological calcium. We also examined relationships between cell morphology, substrate stiffness and force production. Results showed a significant relationship between cell area and force. Implementing directed modifications of substrate stiffness, by varying stiffness from embryonic-like to adult myocardium-like, hiPSC-CMs produced maximal forces on substrates with a lower modulus and significantly less force when assayed on increasingly stiff adult myocardium-like substrates. Calculated strain energy measurements paralleled these findings. Collectively, these findings further establish single cell TFM as a valuable approach to illuminate the quantitative physiological maturation of force in hiPSC-CMs.
url http://europepmc.org/articles/PMC5884520?pdf=render
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AT kamilahyamen investigationofhumanipscderivedcardiacmyocytefunctionalmaturationbysinglecelltractionforcemicroscopy
AT patrickwalford investigationofhumanipscderivedcardiacmyocytefunctionalmaturationbysinglecelltractionforcemicroscopy
AT josephmmetzger investigationofhumanipscderivedcardiacmyocytefunctionalmaturationbysinglecelltractionforcemicroscopy
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