Figure 2.

Analysis of mitochondrial gene expression and genome copy number. Expression analysis of mitochondrial encoded genes (A) and nuclear encoded mitochondrial transcription factors (B). Total RNA isolated from control and SIN3-deficient cells (KD1, black bars, and KD2, gray bars) was used to generate cDNA. qPCR was performed using the cDNA as a template and primer pairs for the genes indicated along the X-axis. Relative levels of gene expression are indicated. Error bars represent standard error. A, n = 7 for KD1 and n = 5 for KD2, p < 0.05 for all data. B, n = 4, *p < 0.05. (C) Mitochondrial DNA copy number is unaltered following loss of SIN3. DNA was isolated from control and SIN3-deficient cells. qPCR was performed using the DNA as a template and primer pairs for both nuclear and mitochondrial genome sequences as indicated along the X-axis. Pro-cyt-c-p amplifies the promoter region of Cyt-c-p. Relative copy number is indicated. The nuclear gene glutathione transferase (CG11784) was used for normalization. Error bars represent standard error (n = 3).