Sigmoidal and bell-shaped voltage dependence of Ca2+ transients in myotubes expressing the heterologous DHPR β2a-subunit. Ca2+ transients in ΔF/F units were measured in myotubes with the indicated phenotype (β1 KO, RyR3 KO, RyR1 KO and double RyR1/RyR3 KO) expressing β1a (top row) or β2a (bottom row). The depolarization duration was 50 ms (closed symbols) or 200 ms (open symbols) from a holding potential of −40 mV. The same myotube was subjected to the 50-ms and 200-ms depolarization protocols. Ca2+ transients were measured at the end of each depolarization from the time course of the integrated confocal line scan image fluorescence. The lines correspond to a Boltzmann fit of the population mean ΔF/F indicated in Table 2. All fluorescence vs. voltage curves were fit with Eq. 1 except those obtained with the 200 ms depolarization in myotubes overexpressing β2a, which were fit with Eq. 2. Parameters of the fitted lines (ΔF/Fmax in ΔF/F units, V1/2 in mV, and k in mV) for β1 KO overexpressing β1a are: 2.8, −6.1, 7.8 for 50 ms and 3.2, −10.2, 5.7 for 200 ms. Parameters for β1 KO overexpressing β2a are: 0.8, −2.5, 5.8 for 50 ms and 1.8, 9, 9.7 for 200 ms. Parameters for RyR3 KO overexpressing β1a are: 2.2, −7.2, 8.2 for 50 ms and 3.2, −9.9, 7.3 for 200 ms. Parameters for RyR3 KO overexpressing β2a are: 0.6, 8.5, 11.3 for 50 ms and 1.5, 3.6, 10 for 200 ms. Parameters for RyR1 KO overexpressing β2a are: 0.4, 9.8, 8.9 for 200 ms. Parameters for RyR1/RyR3 KO overexpressing β2a are: 0.2, 7.9, 10 for 200 ms.