Abstract

Mutational inactivation of BRCA1 confers a cumulative lifetime risk of breast and ovarian cancers. However, the underlying basis for the tissue-restricted tumor-suppressive properties of BRCA1 remains poorly defined. Here we show that BRCA1 mediates ligand-independent transcriptional repression of the estrogen receptor α (ERα), a principal determinant of the growth, differentiation, and normal functional status of breasts and ovaries. In Brca1-null mouse embryo fibroblasts and BRCA1-deficient human ovarian cancer cells, ERα exhibited ligand-independent transcriptional activity that was not observed in Brca1-proficient cells. Ectopic expression in Brca1-deficient cells of wild-type BRCA1, but not clinically validated BRCA1 missense mutants, restored ligand-independent repression of ERα in a manner dependent upon apparent histone deacetylase activity. In estrogen-dependent human breast cancer cells, chromatin immunoprecipitation analysis revealed the association of BRCA1 with ERα at endogenous estrogen-response elements before, but not after estrogen stimulation. Collectively, these results reveal BRCA1 to be a ligand-reversible barrier to transcriptional activation by unliganded promoter-bound ERα and suggest a possible mechanism by which functional inactivation of BRCA1 could promote tumorigenesis through inappropriate hormonal regulation of mammary and ovarian epithelial cell proliferation.

Keywords

BiologyChromatin immunoprecipitationEstrogen receptorCancer researchEstrogen receptor alphaEstrogen receptor betaEctopic expressionEstrogen-related receptor alphaEstrogenPsychological repressionTrichostatin ACell biologyHistone deacetylaseHistoneEndocrinologyGene expressionCell cultureCancerBreast cancerPromoterGeneticsGene

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Year
2001
Type
article
Volume
98
Issue
17
Pages
9587-9592
Citations
211
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Lei Zheng, Lois A. Annab, Cynthia A. Afshari et al. (2001). BRCA1 mediates ligand-independent transcriptional repression of the estrogen receptor. Proceedings of the National Academy of Sciences , 98 (17) , 9587-9592. https://doi.org/10.1073/pnas.171174298

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DOI
10.1073/pnas.171174298