Mapping the STK4/Hippo signaling network in prostate cancer cell
Fig 1
Expression of CL-STK4, LR-STK4, and NL-STK4 protein in Tet-inducible C4-2 prostate cancer cells.
(A) Time-dependent expression of CL-STK4, LR-STK4, and NL-STK4 protein in the engineered cells that were exposed to doxycycline (Dox) for 24 and 48h. Levels of ectopic STK4 proteins were assessed by Western blotting (WB) using the HA-tagged antibody. (B-D) Analysis of CL-STK4, LR-STK4, and NL-STK4 protein in cytoplasmic, lipid raft, and nuclear fractions, respectively. Expression of HA-STK4 protein was evaluated by WB with the HA-tag antibody at 48h after treatment with and without doxycycline (Dox, 4 μg/ml). Lam (lamin) A/C was used as a nuclear marker. Giα2 was used as a lipid raft marker. (E-G) Immunofluorescence (IF) analysis of CL-STK4, LR-STK4, and NL-STK4 protein in the C4-2/CL-STK4, C4-2/LR-STK4, and C4-2/NL-STK4 cells, respectively. IF was performed at 24h post Dox (4 μg/ml) treatment. Micrographs are the representation of two independent experiments. CTxB-FITC labeled lipid raft in C4-2/LR-STK4 cells. For both experiments, cells were grown in Tet-approved serum conditions. CL: Cytoplasmic localization, LR: Lipid raft; NL: nuclear localization, HA: Hemagglutinin.