Fig. 3.
Fig. 3. Cell cycle–dependent regulation of exogenous FANCC but not exogenous luciferase expression. / (A) 293 FANCC E2 cells were treated with 1.3 mmol/L HU for 24 hours to synchronize cells at the G1/S boundary. Cells were then washed twice and fed with complete growth medium. Whole-cell lysates were prepared at the indicated times after release. A whole-cell extract was also prepared from a culture of asynchronous FANCC E2 cells (Control). The whole-cell extracts were subjected to Western blotting and probed using a murine anti-FANCC antibody (3A11). Identical results were obtained using a second monoclonal antibody (8F3; data not shown). Cell cycle kinetics in these experiments was identical to that shown in Figure 2B. (B) Whole-cell extracts of 293 LUC cells were prepared under similar experimental conditions. Extracts were analyzed for luciferase expression by Western blotting and probing with a rabbit anti-luciferase antiserum. The top band is a luciferase-specific band (LUC) detected only in 293 LUC cells and not in 293 WT, 293 NEO, 293 FANCC, or 293 L554P cells (data not shown). The lower 2 bands are nonspecific and are seen in 293 WT and derivative cells.

Cell cycle–dependent regulation of exogenous FANCC but not exogenous luciferase expression.

(A) 293 FANCC E2 cells were treated with 1.3 mmol/L HU for 24 hours to synchronize cells at the G1/S boundary. Cells were then washed twice and fed with complete growth medium. Whole-cell lysates were prepared at the indicated times after release. A whole-cell extract was also prepared from a culture of asynchronous FANCC E2 cells (Control). The whole-cell extracts were subjected to Western blotting and probed using a murine anti-FANCC antibody (3A11). Identical results were obtained using a second monoclonal antibody (8F3; data not shown). Cell cycle kinetics in these experiments was identical to that shown in Figure 2B. (B) Whole-cell extracts of 293 LUC cells were prepared under similar experimental conditions. Extracts were analyzed for luciferase expression by Western blotting and probing with a rabbit anti-luciferase antiserum. The top band is a luciferase-specific band (LUC) detected only in 293 LUC cells and not in 293 WT, 293 NEO, 293 FANCC, or 293 L554P cells (data not shown). The lower 2 bands are nonspecific and are seen in 293 WT and derivative cells.

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