Tax overactivates replication origins. (A-B) JPX9 and JPX9i cells were extracted with CSK buffer, fixed, and stained for MCM2 or MCM3 and DNA content (4′,6-diamidino-2-phenylindole) before flow cytometric analysis. (A) Representative analyses of MCM2 staining and DNA content labeling. (B) MCM2 and MCM3 MFI in G₁ and M phases of the cell cycle normalized to the MFI of control cells in G1 (relative MFI). (C) JPX9 and JPX9i were treated with HU (2.5mM) to synchronize cells at G₁/S transition for 16 hours, and MCM2 occupancy at Myc, LaminB2, β-globin, and RNF185 replication origins was detected by ChIP. Results were expressed as a percentage of input DNA. (B) Representative results of one of 3 independent ChIP experiments are shown. (D) HeLa cells were transfected with a Tax expression vector, incubated during 3 hours, and synchronized at G₁/S transition with 2mM HU. After a short BrdU pulse (15 minutes) in HU-free medium, cells were processed for confocal microscopy. (E) Number of BrdU foci, (F) BrdU foci intensity, and (G) integrated BrdU intensity in control (Ctrl) and Tax-positive cells (n = 50). (H-I) Rat-1 cells stably transduced with control (Ctrl) or Tax-expressing viruses were treated or not with UCN-01 (100nM, 3 hours), pulsed with BrdU (33μM, 30 minutes). DNA was isolated, spread on slides, and the BrdU-labeled tracks were analyzed by confocal microscopy. Next, fork-to-fork distance and length of isolated tracks were measured. (J-K) JPX9 cells were stably transduced with lentiviruses encoding MCM3 shRNAs, stimulated (black bars) or not (open bars) with ZnCl₂ (120μM), and pulsed with BrdU for 30 minutes. (J) MFI of BrdU labeling and (K) duration of S phase were analyzed by flow cytometry (see supplemental Figure 4 for details). The results presented are the mean ± SD of 3 independent experiments. A.U. indicates arbitrary units; and NS, not significant. *P < .05, according to Kruskal-Wallis test. ***P < .001, according to Kruskal-Wallis test.