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. 2015 Jul 3;5:11749. doi: 10.1038/srep11749

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Copyright © 2015, Macmillan Publishers Limited

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3 cell lines (SKOV3, OVCAR3, and CaOV3) were treated with HGF, HGF + INC280, or left untreated, for 10 min (A), 360 min (B), or 24 hrs (D). c-MET phosphorylation was assessed in these cell lines using antibodies against phosphorylated Y1234/1235 c-MET (P c-MET), and total c-MET (T c-MET). C) Signaling downstream of c-MET activation was assessed (shown here 360 minutes post treatment using antibodies against phosphorylated S473 AKT (P AKT), total AKT (T AKT), phosphorylated Y202/204 ERK 1/2 (P ERK), and total ERK. β-actin was used as a loading control. HOSE 6.3 normal ovarian surface epithelium cells were also treated with HGF, HGF + INC280, or left untreated, for 10 min (E), 360 min (F) or 24 hrs (G). Full length gels containing the cropped images above are shown in Supplementary Figures 4 (A and B), 5 (C), and 6 (D–G).