β-catenin regulates FOXP2 transcriptional activity via multiple binding sites
Richter, Gesa; Gui, Tianshu; Bourgeois, Benjamin; Koyani, Chintan N.; Ulz, Peter; Heitzer, Ellen; von Lewinski, Dirk; Burgering, Boudewijn M.T.; Malle, Ernst; Madl, Tobias
(2021) FEBS Journal, volume 288, issue 10, pp. 3261 - 3284
(Article)
Abstract
The transcription factor forkhead box protein P2 (FOXP2) is a highly conserved key regulator of embryonal development. The molecular mechanisms of how FOXP2 regulates embryonal development, however, remain elusive. Using RNA sequencing, we identified the Wnt signaling pathway as key target of FOXP2-dependent transcriptional regulation. Using cell-based assays, we show
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that FOXP2 transcriptional activity is regulated by the Wnt coregulator β-catenin and that β-catenin contacts multiple regions within FOXP2. Using nuclear magnetic resonance spectroscopy, we uncovered the molecular details of these interactions. β-catenin contacts a disordered FOXP2 region with α-helical propensity via its folded armadillo domain, whereas the intrinsically disordered β-catenin N terminus and C terminus bind to the conserved FOXP2 DNA-binding domain. Using RNA sequencing, we confirmed that β-catenin indeed regulates transcriptional activity of FOXP2 and that the FOXP2 α-helical motif acts as a key regulatory element of FOXP2 transcriptional activity. Taken together, our findings provide first insight into novel regulatory interactions and help to understand the intricate mechanisms of FOXP2 function and (mis)-regulation in embryonal development and human diseases. Database: Expression data are available in the GEO database under the accession number GSE138938.
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Keywords: FOXP2, intrinsically disordered protein, signal transduction, transcriptional regulation, Wnt signaling, β-catenin, Biochemistry, Molecular Biology, Cell Biology
ISSN: 1742-464X
Publisher: Wiley-Blackwell
Note: Funding Information: This work was supported by the Austrian Science Foundation (P28854, I3792, DK‐MCD W1226 to TM), the Austrian Research Promotion Agency (FFG: 864690, 870454 to TM), the Integrative Metabolism Research Center Graz, the Austrian infrastructure program 2016/2017, the Styrian government (Zukunftsfonds), BioTechMed/Graz (Flagship Project), and the Austrian National Bank (P17600 to EM). Funding Information: This work was supported by the Austrian Science Foundation (P28854, I3792, DK-MCD W1226 to TM), the Austrian Research Promotion Agency (FFG: 864690, 870454 to TM), the Integrative Metabolism Research Center Graz, the Austrian infrastructure program 2016/2017, the Styrian government (Zukunftsfonds), BioTechMed/Graz (Flagship Project), and the Austrian National Bank (P17600 to EM). Publisher Copyright: © 2020 The Authors. The FEBS Journal published by John Wiley & Sons Ltd on behalf of Federation of European Biochemical Societies
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