Figure 6. CD44 and CDH1 protein expression in Hs578t and HCT116 RNAi stable clones.

Total cellular protein was extracted from the Hs578t and HCT116 parental cell lines and representative vector and RNAi stable clones using either urea (CD44) or high salt RIPA (CDH1) buffers, separated by SDS-PAGE and immunoblotted for CD44 (A & B) or CDH1 (C). β-actin served as a loading control.