(A) Relative expression levels of the top most down-regulated genes in LATS2L breast tumors (TCGA-BRCA dataset, see Fig 1) in the panel of breast cancer.

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(A) Relative expression levels of the top most down-regulated genes in LATS2L breast tumors (TCGA-BRCA dataset, see Fig 1) in the panel of breast cancer cell lines included in the Cancer Cell Line Encyclopedia. (A) Relative expression levels of the top most down-regulated genes in LATS2L breast tumors (TCGA-BRCA dataset, see Fig 1) in the panel of breast cancer cell lines included in the Cancer Cell Line Encyclopedia. Representative luminal cell lines are marked. (B) Upper panel: schematic representation of the LATS2 genomic locus. Positions of CpG island and methylation probes with differential methylation (P-value < 0.05) between LATS2L and LATS2H lumB tumors are shown. Lower panel: mean methylation of each probe in LATS2L versus LATS2H tumors. Line thickness corresponds to the P-value of the difference in methylation levels of the indicated probe between the two groups. For each probe, Pearson's correlation coefficient between expression and methylation in all lumB tumors is listed. (C) Left panel: ZR75-1 cells were transiently transfected with the indicated expression plasmids and harvested 72 h later. Cell extracts were subjected to Western blot analysis of LATS1, LATS2, and GAPDH as loading control. Right panel: ZR75-1 cells were transduced with MYC-LATS2 expression plasmid or vector control and selected with blasticidin to obtain stable expression. Cell extracts were subjected to Western blot analysis with the indicated antibodies. (D) MDA-MB-468 cells were transfected with the indicated expression plasmids and subjected 48 h later to PI exclusion analysis followed by flow cytometry analysis. “Relative cell death” represents the ratio between the percentages of dead (PI+) cells in the GFP-positive population versus the GFP-negative population. Values within each experiment were normalized to GFP transfected sample; mean ± SEM of two independent experiments. Noa Furth et al. LSA 2018;1:e201800171 © 2018 Furth et al.