Cell density and phosphorylation control the subcellular localization of adenomatous polyposis coli protein. Mol Cell Biol. 2001; 21:8143–8156. [PubMed: 11689703] Zeineldin et al. Page 17 Oncogene. Author manuscript; available

Loss of functional adenomatous polyposis coli protein (APC) leads to uncontrolled proliferation of colonic epithelial cells, as evidenced by polyp formation, a prelude to carcinogenesis. As a tumor suppressor, APC targets the oncogene -catenin for proteasome-mediated cytoplasmic degradation. Recently, it was demon-strated that APC also interacts with nuclear -catenin, thereby reducing -catenin’s activity as a transcription cofactor and enhancing its nuclear export. The first objective of this study was to analyze how cellular context affected APC distribution. We determined that cell density but not cell cycle influenced APC’s subcellular distribution, with predominantly nuclear APC found in subconfluent MDCK and intestinal epithelial cells but both cytoplasmic and nuclear APC in superconfluent cells. Redistribution of APC protein did not depend on continual nuclear export. Focusing on the two defined nuclear localization signals in the C-terminal third of APC (NLS1APC and NLS2APC), we found that phosphorylation at the CK2 site increased and phosphorylation at the PKA site decreased NLS2APC-mediated nuclear translocation. Cell density-mediated redistribution of -galactosidase was achieved by fusion to NLS2APC but not to NLS1APC. Both the CK2 and PKA sites were important for this density-mediated redistribution, and pharmacological agents that target CK2 and PKA instigated relocalization of endogenous APC. Our data provide evidence that physiological signals such as cell density regulate APC’s nuclear distribution, with phosphorylation sites near NLS2APC being critical for thi