Mutagenesis analysis of Ser350. A, phosphorylation-deficient mutation at Ser350 confers hPXR resistance to Cdk2. HepG2 cells were co-transfected with CYP3A4-luc, other plasmids as indicated (cyclin E, Cdk2, or hPXR), and CMV-Renilla luciferase plasmid (as a transfection control). Cells were treated with DMSO or 10 μm rifampicin 24 h post-transfection. Luciferase activities were measured 24 h after compound treatments. The relative luciferase units (RLUs) were determined by normalizing with the Renilla luciferase control. The values represent the means of six independent experiments, and the bars denote the standard deviation. In the absence of cyclin E and Cdk2 transfection (1st to 3rd lanes; 1st lane is the leftmost lane), the p value was ascertained using the Student's t test and expressed as follows: ***, p < 0.001, and ns (not significant; p > 0.05), as compared with samples that were transfected with wild-type FLAG-hPXR (1st lane), for either DMSO or rifampicin-treated samples, respectively. In the presence of cyclin E and Cdk2 transfection (4th to 6th lanes; 6th lane is the right-most lane), the p value was ascertained using the Student's t test and expressed as follows: ###, p < 0.001, as compared with samples that were not transfected with either cyclin E or Cdk2 (4th lane versus 1st lane, 5th lane versus 2nd lane, and 6th lane versus 3rd lane), for either DMSO or rifampicin-treated samples, respectively. Statistical significant differences between other samples (noted in brackets) are indicated by p < 0.001. B, expression levels of hPXR. Actin expression level is used to verify equal loading of lysates. α-FLAG, anti-FLAG; α-β-actin, anti-β-actin; Cdk2-WT, wild-type V5-Cdk2; cyclin E, V5-cyclin E. Data shown are from a representative experiment.