Sc 21731

We fixed raft cultures in 4% neutral buffered formalin and then embedded in paraffin for sectioning and hematoxylin and eosin (H&E) staining. Primary rabbit monoclonal antibodies to keratin 14 (ab51054, Abcam) and Ki-67 (ab16667, Abcam) and primary mouse monoclonal antibodies to K18 (ab7797, Abcam), pAkt1 (sc-293125, Santa Cruz) and MMP-1 (sc-21731, Santa Cruz) were used for immunohistochemistry on unstained sections. Secondary donkey anti-mouse antibody (ab150105, Abcam) with Alexa 488 tag and secondary goat anti-rabbit antibody (ab150080, Abcam) with an Alexa 594 tag were used for visualization. Negative controls consisted of irrelevant primary antibodies including rabbit monoclonal isotype control (ab172730, Abcam) and mouse monoclonal isotype control (ab170190, Abcam). The gain and exposure time of the fluorescence microscope were adjusted to show positively stained cells while negative control cells had no staining. Staining percentage was calculated by dividing the positively stained cell number by the total cell number. Staining intensity was measured by ImageJ and the negative control was used to subtract background.