RESUMO
Abnormal accumulation of ß-catenin protein, a key transcriptional activator required for Wnt signaling, is the hallmark of many tumor types, including colon cancer. In normal cells, ß-catenin protein level is tightly controlled by a multiprotein complex through the proteosome pathway. Mutations in the components of the ß-catenin degradation complex, such as adenomatous polyposis coli (APC) and Axin, lead to ß-catenin stabilization and the constitutive activation of target genes. Since the signal transduction of Wnt/ß-catenin is mainly mediated by protein-protein interactions, this pathway has been particularly refractory to conventional target-based small-molecule screening. Here we designed a cellular high-content imaging assay to detect ß-catenin protein through immunofluorescent staining in the SW480 colon cancer cell line, which has elevated ß-catenin endogenously. We demonstrate that the assay is robust and specific to screen a focused biologically diverse chemical library set against known targets that play diverse cellular functions. We identified a number of hits that reduce ß-catenin levels without causing cell death. These hits may serve as tools to understand the dynamics of ß-catenin degradation. This study demonstrates that detecting cell-based ß-catenin protein stability is a viable approach to identifying novel mechanisms of ß-catenin regulation as well as small molecules of therapeutic potential.
