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Investigation of cardiac fibroblasts using myocardial slices.

Cardiovascular research (2017-10-11)
Filippo Perbellini, Samuel A Watson, Martina Scigliano, Samha Alayoubi, Sebastian Tkach, Ifigeneia Bardi, Nicholas Quaife, Christopher Kane, Neil P Dufton, André Simon, Markus B Sikkel, Giuseppe Faggian, Anna M Randi, Julia Gorelik, Sian E Harding, Cesare M Terracciano
RESUMEN

Cardiac fibroblasts (CFs) are considered the principal regulators of cardiac fibrosis. Factors that influence CF activity are difficult to determine. When isolated and cultured in vitro, CFs undergo rapid phenotypic changes including increased expression of α-SMA. Here we describe a new model to study CFs and their response to pharmacological and mechanical stimuli using in vitro cultured mouse, dog and human myocardial slices. Unloading of myocardial slices induced CF proliferation without α-SMA expression up to 7 days in culture. CFs migrating onto the culture plastic support or cultured on glass expressed αSMA within 3 days. The cells on the slice remained αSMA(-) despite transforming growth factor-β (20 ng/ml) or angiotensin II (200 µM) stimulation. When diastolic load was applied to myocardial slices using A-shaped stretchers, CF proliferation was significantly prevented at Days 3 and 7 (P < 0.001). Myocardial slices allow the study of CFs in a multicellular environment and may be used to effectively study mechanisms of cardiac fibrosis and potential targets.

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Sigma-Aldrich
Anti-α-actinina (sarcomérica) monoclonal antibody produced in mouse, clone EA-53, ascites fluid
Sigma-Aldrich
Goat Anti-Mouse IgG Antibody, Cy3 conjugate, Species Adsorbed, 1.3 mg/mL, Chemicon®