Electrophysiological properties of mouse bone marrow c-kit+ cells co-cultured onto neonatal cardiac myocytes

doi:10.1016/j.cardiores.2005.01.018

Cardiovascular Research 2005 66(3):482-492; doi:10.1016/j.cardiores.2005.01.018

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Electrophysiological properties of mouse bone marrow c-kit⁺ cells co-cultured onto neonatal cardiac myocytes

Laura Lagostena^a, Daniele Avitabile^b, Elena De Falco^a, Alessia Orlandi^a, Francesca Grassi^c, Maria Grazia Iachininoto^b, Gianluca Ragone^b, Sergio Fucile^c, Giulio Pompilio^a, Fabrizio Eusebi^c, Maurizio Pesce^a^,* and Maurizio C. Capogrossi^b

^aLaboratorio di Biologia Vascolare e Terapia Genica, Centro Cardiologico Monzino, Istituto di Ricovero e Cura a Carattere Scientifico, Milan, Italy
^bLaboratorio di Patologia Vascolare, Istituto Dermopatico dell'Immacolata, Istituto di Ricovero e Cura a Carattere Scientifico, Via dei Monti di Creta 104, 00167 Rome, Italy
^cLaboratorio di Biofisica, Dipartimento di Fisiologia Umana e Farmacologia "V. Erspamer", Centro di Eccellenza BEMM, Università La Sapienza, Rome, Italy

^* Corresponding author. Laboratorio di Patologia Vascolare, Istituto Dermopatico dell'Immacolata, Istituto di Ricovero e Cura a Carattere Scientifico, Via dei Monti di Creta 104, 00167 Rome, Italy. Tel.: +39 6 6646 2428; fax: +39 6 6646 2430. Email address: m.pesce{at}idi.it

Objective: Controversy about hematopoietic stem cells reprogramminginto cardiac myocytes is currently supported by positive andnegative findings. In fact, some reports have shown the abilityof stem cells from the bone marrow (BM) to differentiate intocardiac myocytes and to contribute to myocardium repair, whileothers have reported the opposite.

Methods: C-kit⁺ cells from mouse bone marrow were co-culturedonto neonatal cardiac myocytes. Hematopoietic stem cell-derivedcells were analyzed by investigating the expression of cardiacmarkers and ion channels and by single-cell electrophysiologicalrecordings.

Results: Groups of undifferentiated c-kit⁺ cells displayed onlyoutward currents. Co-cultured c-kit⁺ stem cells on neonatalcardiac myocytes expressed cardiac markers and Na⁺ and Ca²⁺voltage-gated ion channels. However, Na⁺ and Ca²⁺ currents werenot detected by electrophysiological patch-clamp recordingseven if caffeine and cyclopiazonic acid treatment showed thepresence of intracellular calcium stores. This suggests thatthese channels, although expressed, were not functional andthus do not allow the coupling between excitation and contractionthat is typical of cardiac myocytes. Nevertheless, co-culturedcells had a more hyperpolarized resting membrane potential and,at least in a subset of cells, displayed voltage-gated inwardrectifier currents and outward currents. Co-cultured c-kit⁺-derivedcells were not connected to surrounding cardiac myocytes throughgap junctions. To induce a more pronounced differentiation,co-cultured cells were treated with BMP-4 and TGF-β, twofactors that were shown to trigger a cardiac myocyte differentiationpathway in embryonic stem (ES) cells. Even under these conditions,c-kit⁺ cells did not differentiate into functionally activecardiac myocytes. However, TGF-β/BMP-4-treated cells werehyperpolarized and showed and increased inward rectifier currentdensity.

Conclusions: Our study shows that mouse BM hematopoietic stemcells exhibit a limited plasticity to transdifferentiate intocardiac myocytes in culture.

KEYWORDS Cardiac myocyte; Stem cell; Reprogramming; Electrophysiology; Bone marrow; C-kit; TGF-β; BMP-4

Time for primary review 26 days

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