Figure 4.
Stable expression of dnFADD or dnDR5 in skeletal myoblasts results in decreased levels of MyoD mRNA and protein. In (A and C), cells were plated at 4×105 and the next day quantitative RT-PCR was used to assay for the relative levels of MyoD mRNA in total RNA samples derived from the indicated cell lines. The Ct values for the MyoD PCR product were normalized to the Ct values for a β-actin product, run in parallel, as described in Materials and methods. Error bars represent mean +/- SEM from triplicates. Statistical analysis was performed as described in Materials and methods. Each value obtained from lysates prepared from the clones is significantly different from the corresponding value obtained from lysates prepared from parental 23A2 myoblasts (P < 0.02). In (B and D) whole cell protein lysates were prepared and equal amounts of protein were subjected to SDS-PAGE followed by Western analysis with anti-MyoD (Pharmigen) or anti-actin and visualized by autoradiogaphy as described in Materials and Methods. Shown are the results of one experiment that is representative of three independent experiments.