Ge-specific stains (Fig. 6E). Typically, basal cells comprised approximately one out

September 8, 2017

Ge-specific stains (Fig. 6E). Typically, basal cells comprised approximately one out of four cultured epithelial cells, and the ratio of luminal/basal cells was 2.5. The addition of DMBA had a non-statistically significant effect on the survival ofFigure 5. DMBA-induced DDR is accompanied by loss of Wnt signaling in vitro and in vivo. (A) DMBA exposure reduces LRP activation in vivo, and this reduction in active Wnt signaling is durable. Mammary glands from DMBA-treated (and control) mice were snap-frozen, ground and lysed as described. Proteins were analyzed by Western blotting, and assayed for activation of LRP (p-LRP). Blots were normalized using a vinculin internal loading control. The relative signal was calculated for each pair of treated/control samples, for the timepoints indicated post-exposure. (B) DMBA exposure of MECs in vitro reduces Wnt ligand -induced (and basal) activation of Wnt signaling. MECs were transferred to culture for 24 h, treated with Wnt3a (100 ng/ml, or not) as described in the Methods section, and lysed for analysis of p-LRP, 24 and 48 hours later. (C, D) DMBA exposure of HC11 mammary epithelial cells reduces Wnt ligand -induced (and basal) activation of Wnt signaling. (C) HC11 cells were treated with DMBA and assayed for the appearance of cH2AX 24 hours later (by immunostaining as detailed for Fig. S3). (D) Lysates of similarly treated cells were analyzed by Western blotting for LRP activation (phosphor-LRP). doi:10.1371/journal.pone.0049902.gGenotoxins Inhibit Wnt-Dependent Mammary Stem CellFigure 6. The genotoxic response ablates Wnt-induced basal cell accumulation. (A) Castanospermine chemical information immunohistochemical analysis of lineage-specific responses to DMBA and Wnt3a. Cultured MECs were transferred to culture for 24 hours, and treated with DMBA (2 mg/ml), recombinant mouse Wnt3a (100 ngs/ml) or both for 24 hours, as indicated (Wnt alone, data not shown). Cells were either incubated with BrdU (for 60 mins) or not, then fixed and stained as 1676428 indicated. (B) Examples of images used for quantitative analysis. To obtain the fraction of cells of each lineage that showed activation of DNA damage, or cell division, the image of the lineage-specific marker 24272870 was overlaid on H2AX or BrdU. (C) Quantitation of immunohistochemical analysis of lineage-specific responses to DMBA and Wnt3a. The fraction of each of K5- or K8-positive cells was scored for expression of H2AX, or mitotic index, 24 or 48 hours after exposure to DMBA or Wnt3a (as indicated). (D) Assay of Wnt- and DDR-dependent transcriptional reporters. The Wnt reporter, Axin2, and the p53 target, p21, were measured by qPCR assay of RNA extracts of cell lysates. (E). Visualization of luminal and basal cells in Wnt-treated cultures. Cell cultures were fixed and stained with lineage-specific markers (K8, luminal; K5, basal) together with a nuclear counterstain. (F)Genotoxins Inhibit Wnt-Dependent Mammary Stem CellQuantitation of lineage-specific responses to DMBA and Wnt3a. Results were Iloprost site quantified (at least 1500 cells were counted in each sample; 3 experiments), and the relative differentiation of cultures expressed as K5 and K8-positive cells, and the luminal/basal ratio. * indicates significant difference from non-Wnt3a treated cultures, and ** indicates significant difference from both non-Wnt3a treated, and Wnt-treated cultures. doi:10.1371/journal.pone.0049902.gbasal cells in the absence of Wnt3a. Treated with Wnt3a, the relative frequency of basal cells increased (K8/K5 = 1.77).Ge-specific stains (Fig. 6E). Typically, basal cells comprised approximately one out of four cultured epithelial cells, and the ratio of luminal/basal cells was 2.5. The addition of DMBA had a non-statistically significant effect on the survival ofFigure 5. DMBA-induced DDR is accompanied by loss of Wnt signaling in vitro and in vivo. (A) DMBA exposure reduces LRP activation in vivo, and this reduction in active Wnt signaling is durable. Mammary glands from DMBA-treated (and control) mice were snap-frozen, ground and lysed as described. Proteins were analyzed by Western blotting, and assayed for activation of LRP (p-LRP). Blots were normalized using a vinculin internal loading control. The relative signal was calculated for each pair of treated/control samples, for the timepoints indicated post-exposure. (B) DMBA exposure of MECs in vitro reduces Wnt ligand -induced (and basal) activation of Wnt signaling. MECs were transferred to culture for 24 h, treated with Wnt3a (100 ng/ml, or not) as described in the Methods section, and lysed for analysis of p-LRP, 24 and 48 hours later. (C, D) DMBA exposure of HC11 mammary epithelial cells reduces Wnt ligand -induced (and basal) activation of Wnt signaling. (C) HC11 cells were treated with DMBA and assayed for the appearance of cH2AX 24 hours later (by immunostaining as detailed for Fig. S3). (D) Lysates of similarly treated cells were analyzed by Western blotting for LRP activation (phosphor-LRP). doi:10.1371/journal.pone.0049902.gGenotoxins Inhibit Wnt-Dependent Mammary Stem CellFigure 6. The genotoxic response ablates Wnt-induced basal cell accumulation. (A) Immunohistochemical analysis of lineage-specific responses to DMBA and Wnt3a. Cultured MECs were transferred to culture for 24 hours, and treated with DMBA (2 mg/ml), recombinant mouse Wnt3a (100 ngs/ml) or both for 24 hours, as indicated (Wnt alone, data not shown). Cells were either incubated with BrdU (for 60 mins) or not, then fixed and stained as 1676428 indicated. (B) Examples of images used for quantitative analysis. To obtain the fraction of cells of each lineage that showed activation of DNA damage, or cell division, the image of the lineage-specific marker 24272870 was overlaid on H2AX or BrdU. (C) Quantitation of immunohistochemical analysis of lineage-specific responses to DMBA and Wnt3a. The fraction of each of K5- or K8-positive cells was scored for expression of H2AX, or mitotic index, 24 or 48 hours after exposure to DMBA or Wnt3a (as indicated). (D) Assay of Wnt- and DDR-dependent transcriptional reporters. The Wnt reporter, Axin2, and the p53 target, p21, were measured by qPCR assay of RNA extracts of cell lysates. (E). Visualization of luminal and basal cells in Wnt-treated cultures. Cell cultures were fixed and stained with lineage-specific markers (K8, luminal; K5, basal) together with a nuclear counterstain. (F)Genotoxins Inhibit Wnt-Dependent Mammary Stem CellQuantitation of lineage-specific responses to DMBA and Wnt3a. Results were quantified (at least 1500 cells were counted in each sample; 3 experiments), and the relative differentiation of cultures expressed as K5 and K8-positive cells, and the luminal/basal ratio. * indicates significant difference from non-Wnt3a treated cultures, and ** indicates significant difference from both non-Wnt3a treated, and Wnt-treated cultures. doi:10.1371/journal.pone.0049902.gbasal cells in the absence of Wnt3a. Treated with Wnt3a, the relative frequency of basal cells increased (K8/K5 = 1.77).