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FOXL2 and FOXA1 cooperatively assemble on the TP53 promoter in alternative dimer configurationsopen access

Authors
Choi, YuriLuo, YongyangLee, SeunghwaJin, HanyongYoon, Hye-JinHahn, YoonsooBae, JeehyeonLee, Hyung Ho
Issue Date
Aug-2022
Publisher
OXFORD UNIV PRESS
Citation
NUCLEIC ACIDS RESEARCH, v.50, no.15, pp 8929 - 8946
Pages
18
Journal Title
NUCLEIC ACIDS RESEARCH
Volume
50
Number
15
Start Page
8929
End Page
8946
URI
https://scholarworks.bwise.kr/cau/handle/2019.sw.cau/59627
DOI
10.1093/nar/gkac673
ISSN
0305-1048
1362-4962
Abstract
Although both the p53 and forkhead box (FOX) family proteins are key transcription factors associated with cancer progression, their direct relationship is unknown. Here, we found that FOX family proteins bind to the non-canonical homotypic cluster of the p53 promoter region (TP53). Analysis of crystal structures of FOX proteins (FOXL2 and FOXA1) bound to the p53 homotypic cluster indicated that they interact with a 2:1 stoichiometry accommodated by FOX-induced DNA allostery. In particular, FOX proteins exhibited distinct dimerization patterns in recognition of the same p53-DNA; dimer formation of FOXA1 involved protein-protein interaction, but FOXL2 did not. Biochemical and biological functional analyses confirmed the cooperative binding of FOX proteins to the TP53 promoter for the transcriptional activation of TP53. In addition, up-regulation of TP53 was necessary for FOX proteins to exhibit anti-proliferative activity in cancer cells. These analyses reveal the presence of a discrete characteristic within FOX family proteins in which FOX proteins regulate the transcription activity of the p53 tumor suppressor via cooperative binding to the TP53 promoter in alternative dimer configurations.
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자연과학대학 (생명과학과)
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