Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy

Testing cardiac gene and cell therapies in vitro requires a tissue substrate that survives for several days in culture while maintaining its physiological properties. The purpose of this study was to test whether culture of intact cardiac tissue of neonatal rat ventricles (organ explant culture) may...

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Autores principales: den Haan, A. Dénise, Veldkamp, Marieke W., Bakker, Diane, Boink, Geert J. J., Janssen, Rob B., de Bakker, Jacques M. T., Tan, Hanno L.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2013
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3596330/
https://www.ncbi.nlm.nih.gov/pubmed/23516623
http://dx.doi.org/10.1371/journal.pone.0059290
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author den Haan, A. Dénise
Veldkamp, Marieke W.
Bakker, Diane
Boink, Geert J. J.
Janssen, Rob B.
de Bakker, Jacques M. T.
Tan, Hanno L.
author_facet den Haan, A. Dénise
Veldkamp, Marieke W.
Bakker, Diane
Boink, Geert J. J.
Janssen, Rob B.
de Bakker, Jacques M. T.
Tan, Hanno L.
author_sort den Haan, A. Dénise
collection PubMed
description Testing cardiac gene and cell therapies in vitro requires a tissue substrate that survives for several days in culture while maintaining its physiological properties. The purpose of this study was to test whether culture of intact cardiac tissue of neonatal rat ventricles (organ explant culture) may be used as a model to study gene and cell therapy. We compared (immuno) histology and electrophysiology of organ explant cultures to both freshly isolated neonatal rat ventricular tissue and monolayers. (Immuno) histologic studies showed that organ explant cultures retained their fiber orientation, and that expression patterns of α-actinin, connexin-43, and α-smooth muscle actin did not change during culture. Intracellular voltage recordings showed that spontaneous beating was rare in organ explant cultures (20%) and freshly isolated tissue (17%), but common (82%) in monolayers. Accordingly, resting membrane potential was -83.9±4.4 mV in organ explant cultures, −80.5±3.5 mV in freshly isolated tissue, and −60.9±4.3 mV in monolayers. Conduction velocity, measured by optical mapping, was 18.2±1.0 cm/s in organ explant cultures, 18.0±1.2 cm/s in freshly isolated tissue, and 24.3±0.7 cm/s in monolayers. We found no differences in action potential duration (APD) between organ explant cultures and freshly isolated tissue, while APD of monolayers was prolonged (APD at 70% repolarization 88.8±7.8, 79.1±2.9, and 134.0±4.5 ms, respectively). Organ explant cultures and freshly isolated tissue could be paced up to frequencies within the normal range for neonatal rat (CL 150 ms), while monolayers could not. Successful lentiviral (LV) transduction was shown via Egfp gene transfer. Co-culture of organ explant cultures with spontaneously beating cardiomyocytes increased the occurrence of spontaneous beating activity of organ explant cultures to 86%. We conclude that organ explant cultures of neonatal rat ventricle are structurally and electrophysiologically similar to freshly isolated tissue and a suitable new model to study the effects of gene and cell therapy.
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spelling pubmed-35963302013-03-20 Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy den Haan, A. Dénise Veldkamp, Marieke W. Bakker, Diane Boink, Geert J. J. Janssen, Rob B. de Bakker, Jacques M. T. Tan, Hanno L. PLoS One Research Article Testing cardiac gene and cell therapies in vitro requires a tissue substrate that survives for several days in culture while maintaining its physiological properties. The purpose of this study was to test whether culture of intact cardiac tissue of neonatal rat ventricles (organ explant culture) may be used as a model to study gene and cell therapy. We compared (immuno) histology and electrophysiology of organ explant cultures to both freshly isolated neonatal rat ventricular tissue and monolayers. (Immuno) histologic studies showed that organ explant cultures retained their fiber orientation, and that expression patterns of α-actinin, connexin-43, and α-smooth muscle actin did not change during culture. Intracellular voltage recordings showed that spontaneous beating was rare in organ explant cultures (20%) and freshly isolated tissue (17%), but common (82%) in monolayers. Accordingly, resting membrane potential was -83.9±4.4 mV in organ explant cultures, −80.5±3.5 mV in freshly isolated tissue, and −60.9±4.3 mV in monolayers. Conduction velocity, measured by optical mapping, was 18.2±1.0 cm/s in organ explant cultures, 18.0±1.2 cm/s in freshly isolated tissue, and 24.3±0.7 cm/s in monolayers. We found no differences in action potential duration (APD) between organ explant cultures and freshly isolated tissue, while APD of monolayers was prolonged (APD at 70% repolarization 88.8±7.8, 79.1±2.9, and 134.0±4.5 ms, respectively). Organ explant cultures and freshly isolated tissue could be paced up to frequencies within the normal range for neonatal rat (CL 150 ms), while monolayers could not. Successful lentiviral (LV) transduction was shown via Egfp gene transfer. Co-culture of organ explant cultures with spontaneously beating cardiomyocytes increased the occurrence of spontaneous beating activity of organ explant cultures to 86%. We conclude that organ explant cultures of neonatal rat ventricle are structurally and electrophysiologically similar to freshly isolated tissue and a suitable new model to study the effects of gene and cell therapy. Public Library of Science 2013-03-13 /pmc/articles/PMC3596330/ /pubmed/23516623 http://dx.doi.org/10.1371/journal.pone.0059290 Text en © 2013 den Haan et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
den Haan, A. Dénise
Veldkamp, Marieke W.
Bakker, Diane
Boink, Geert J. J.
Janssen, Rob B.
de Bakker, Jacques M. T.
Tan, Hanno L.
Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy
title Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy
title_full Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy
title_fullStr Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy
title_full_unstemmed Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy
title_short Organ Explant Culture of Neonatal Rat Ventricles: A New Model to Study Gene and Cell Therapy
title_sort organ explant culture of neonatal rat ventricles: a new model to study gene and cell therapy
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3596330/
https://www.ncbi.nlm.nih.gov/pubmed/23516623
http://dx.doi.org/10.1371/journal.pone.0059290
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