Mechanisms of OCT4-SOX2 motif readout on nucleosomes

Alicia K. Michael(Friedrich Miescher Institute), Ralph S. Grand(Friedrich Miescher Institute), Luke Isbel(Friedrich Miescher Institute), Simone Cavadini(Friedrich Miescher Institute), Zuzanna Kozicka(University of Basel), Georg Kempf(Friedrich Miescher Institute), R.D. Bunker(Friedrich Miescher Institute), Andreas D. Schenk(Friedrich Miescher Institute), Alexandra Graff-Meyer(Friedrich Miescher Institute), G.R. Pathare(Friedrich Miescher Institute), Joscha Weiss(Friedrich Miescher Institute), S. Matsumoto(Friedrich Miescher Institute), Lukas Burger(SIB Swiss Institute of Bioinformatics), Dirk Schübeler(University of Basel), Nicolas H. Thomä(Friedrich Miescher Institute)
Science
April 23, 2020
10.1126/science.abb0074
Cited by 259

Abstract

Engaging the nucleosome Cell identity is defined by gene expression patterns that are established through the binding of specific transcription factors. However, nucleosomal units limit access of transcription factors to specific DNA motifs within the mammalian genome. To study how transcription factors bind such chromatinized, nucleosome-embedded motifs, Michael et al. focused on the pluripotency factors OCT4 and SOX2. They systematically quantified the relative affinities of these factors at different motif positions throughout the nucleosome, enabling structure determination of OCT4-SOX2–bound nucleosomes by cryo–electron microscopy. OCT4 and SOX2 bound cooperatively to strengthen DNA-binding affinity and resulted in DNA distortions that destabilized the nucleosome. This analysis reveals position-dependent binding modes that were validated in vivo, providing insights on how transcription factors read out chromatinized motifs. Science , this issue p. 1460

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