Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart

KEY POINTS: A robust cardiac slicing approach was developed for optical mapping of transmural gradients in transmembrane potential (V (m)) and intracellular Ca(2+) transient (CaT) of murine heart. Significant transmural gradients in V (m) and CaT were observed in the left ventricle. Frequency‐depend...

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Autores principales: Wen, Q., Gandhi, K., Capel, Rebecca A., Hao, G., O'Shea, C., Neagu, G., Pearcey, S., Pavlovic, D., Terrar, Derek A., Wu, J., Faggian, G., Camelliti, Patrizia, Lei, M.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley and Sons Inc. 2018
Materias:
Cardiovascular
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6117587/
https://www.ncbi.nlm.nih.gov/pubmed/29928770
http://dx.doi.org/10.1113/JP276239
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author Wen, Q.
Gandhi, K.
Capel, Rebecca A.
Hao, G.
O'Shea, C.
Neagu, G.
Pearcey, S.
Pavlovic, D.
Terrar, Derek A.
Wu, J.
Faggian, G.
Camelliti, Patrizia
Lei, M.
author_facet Wen, Q.
Gandhi, K.
Capel, Rebecca A.
Hao, G.
O'Shea, C.
Neagu, G.
Pearcey, S.
Pavlovic, D.
Terrar, Derek A.
Wu, J.
Faggian, G.
Camelliti, Patrizia
Lei, M.
author_sort Wen, Q.
collection PubMed
description KEY POINTS: A robust cardiac slicing approach was developed for optical mapping of transmural gradients in transmembrane potential (V (m)) and intracellular Ca(2+) transient (CaT) of murine heart. Significant transmural gradients in V (m) and CaT were observed in the left ventricle. Frequency‐dependent action potentials and CaT alternans were observed in all ventricular regions with rapid pacing, with significantly greater incidence in the endocardium than epicardium. The observations demonstrate the feasibility of our new approach to cardiac slicing for systematic analysis of intrinsic transmural and regional gradients in V (m) and CaT. ABSTRACT: Transmural and regional gradients in membrane potential and Ca(2+) transient in the murine heart are largely unexplored. Here, we developed and validated a robust approach which combines transverse ultra‐thin cardiac slices and high resolution optical mapping to enable systematic analysis of transmural and regional gradients in transmembrane potential (V (m)) and intracellular Ca(2+) transient (CaT) across the entire murine ventricles. The voltage dye RH237 or Ca(2+) dye Rhod‐2 AM were loaded through the coronary circulation using a Langendorff perfusion system. Short‐axis slices (300 μm thick) were prepared from the entire ventricles (from the apex to the base) by using a high‐precision vibratome. Action potentials (APs) and CaTs were recorded with optical mapping during steady‐state baseline and rapid pacing. Significant transmural gradients in V (m) and CaT were observed in the left ventricle, with longer AP duration (APD(50) and APD(75)) and CaT duration (CaTD(50) and CaTD(75)) in the endocardium compared with that in the epicardium. No significant regional gradients were observed along the apico‐basal axis of the left ventricle. Interventricular gradients were detected with significantly shorter APD(50), APD(75) and CaTD(50) in the right ventricle compared with left ventricle and ventricular septum. During rapid pacing, AP and CaT alternans were observed in most ventricular regions, with significantly greater incidence in the endocardium in comparison with epicardium. In conclusion, these observations demonstrate the feasibility of our new approach to cardiac slicing for systematic analysis of intrinsic transmural and regional gradients in V (m) and CaT in murine ventricular tissue.
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spelling pubmed-61175872018-09-05 Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart Wen, Q. Gandhi, K. Capel, Rebecca A. Hao, G. O'Shea, C. Neagu, G. Pearcey, S. Pavlovic, D. Terrar, Derek A. Wu, J. Faggian, G. Camelliti, Patrizia Lei, M. J Physiol Cardiovascular KEY POINTS: A robust cardiac slicing approach was developed for optical mapping of transmural gradients in transmembrane potential (V (m)) and intracellular Ca(2+) transient (CaT) of murine heart. Significant transmural gradients in V (m) and CaT were observed in the left ventricle. Frequency‐dependent action potentials and CaT alternans were observed in all ventricular regions with rapid pacing, with significantly greater incidence in the endocardium than epicardium. The observations demonstrate the feasibility of our new approach to cardiac slicing for systematic analysis of intrinsic transmural and regional gradients in V (m) and CaT. ABSTRACT: Transmural and regional gradients in membrane potential and Ca(2+) transient in the murine heart are largely unexplored. Here, we developed and validated a robust approach which combines transverse ultra‐thin cardiac slices and high resolution optical mapping to enable systematic analysis of transmural and regional gradients in transmembrane potential (V (m)) and intracellular Ca(2+) transient (CaT) across the entire murine ventricles. The voltage dye RH237 or Ca(2+) dye Rhod‐2 AM were loaded through the coronary circulation using a Langendorff perfusion system. Short‐axis slices (300 μm thick) were prepared from the entire ventricles (from the apex to the base) by using a high‐precision vibratome. Action potentials (APs) and CaTs were recorded with optical mapping during steady‐state baseline and rapid pacing. Significant transmural gradients in V (m) and CaT were observed in the left ventricle, with longer AP duration (APD(50) and APD(75)) and CaT duration (CaTD(50) and CaTD(75)) in the endocardium compared with that in the epicardium. No significant regional gradients were observed along the apico‐basal axis of the left ventricle. Interventricular gradients were detected with significantly shorter APD(50), APD(75) and CaTD(50) in the right ventricle compared with left ventricle and ventricular septum. During rapid pacing, AP and CaT alternans were observed in most ventricular regions, with significantly greater incidence in the endocardium in comparison with epicardium. In conclusion, these observations demonstrate the feasibility of our new approach to cardiac slicing for systematic analysis of intrinsic transmural and regional gradients in V (m) and CaT in murine ventricular tissue. John Wiley and Sons Inc. 2018-07-26 2018-09-01 /pmc/articles/PMC6117587/ /pubmed/29928770 http://dx.doi.org/10.1113/JP276239 Text en © 2018 The Authors. The Journal of Physiology published by John Wiley & Sons Ltd on behalf of The Physiological Society This is an open access article under the terms of the http://creativecommons.org/licenses/by/4.0/ License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.
spellingShingle Cardiovascular
Wen, Q.
Gandhi, K.
Capel, Rebecca A.
Hao, G.
O'Shea, C.
Neagu, G.
Pearcey, S.
Pavlovic, D.
Terrar, Derek A.
Wu, J.
Faggian, G.
Camelliti, Patrizia
Lei, M.
Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart
title Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart
title_full Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart
title_fullStr Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart
title_full_unstemmed Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart
title_short Transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and Ca(2+) transients in murine heart
title_sort transverse cardiac slicing and optical imaging for analysis of transmural gradients in membrane potential and ca(2+) transients in murine heart
topic Cardiovascular
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6117587/
https://www.ncbi.nlm.nih.gov/pubmed/29928770
http://dx.doi.org/10.1113/JP276239
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