Fig. 3

(a) Measurements of whole-cell L-type calcium currents in failing rat ARVCMs isolated from rat hearts after cryoinfarction, compared with non-failing (sham operated) controls at baseline or (b) after adenoviral Myoscape knockdown or (c) Myoscape overexpression, respectively (n=7-9, *P<0.05 (ANOVA)). (d) Summary of the L-type calcium currents under different experimental conditions, showing either restoration of calcium currents or a further reduction depending on Myoscape protein content. (n=7, *P<0.05 (ANOVA)) (e). To elucidate the functional consequences of myoscape downregulation on cardiomyocyte contractile function, again adult ventricular rat cardiomyocytes were utilized. On the first day of culture, ARVCMs where infected with AdMiRMyocape or control virus (AdMiRNeg). Fractional shortening was assessed by video edge detection evaluated by an observer blinded to experimental conditions. ARVCMs infected with AdMiRMyoscape showed a significant reduction in fractional shortening compared with ARVCM’s infected with control virus (21±1% versus 14±1%, in 60 assessed cells, and n=3 independent cell preparations, ***P<0.001 (ANOVA)). (f) Downregulation of Myoscape protein content was shown via western blot analyses in biopsies from patients suffering from end-stage heart failure due to dilated cardiomyopathy (DCM) and compared with control heart samples from individuals who died from a non-cardiovascular-cause (n=7-8). GAPDH served as a loading control (left panel). A statistical evaluation was done of all samples showing a significant decrease of Myoscape/GAPDH ratios. **P<0.01 (ANOVA). (g) Morpholino knockdown of zebrafish Myoscape results in severe contractile dysfunction. Myoscape knockdown morphants (lateral view) develop pericardial oedema and blood congestion due to low cardiac performance. By contrast, cardiac function of MO-control injected zebrafish embryos was unaffected after 48 or 72 h.p.f. (h) Quantitative evaluation showing 81.7% of Myoscape knockdown morphant zebrafish developing cardiac failure after injection. The presence of heart failure was assessed by evaluation of reduced ventricular function and development of pericardial oedema and precardial signs of blood congestion. Functional assessment of cardiac contractility was carried out by a Zeiss MCU II microscope with the help of the zebraFS software. (i) Fractional shortening (FS) of the ventricular chamber of wild-type and Myoscape-deficient embryos measured at different developmental stages (48 and 72 h.p.f.). *P<0.05; **P<0.01 (ANOVA). Scale bars, 25 µm.