Cooperative binding of two acetylation marks on a histone tail by a single bromodomain (original) (raw)

Nature volume 461, pages 664–668 (2009)Cite this article

Abstract

A key step in many chromatin-related processes is the recognition of histone post-translational modifications by effector modules such as bromodomains and chromo-like domains of the Royal family1,2. Whereas effector-mediated recognition of single post-translational modifications is well characterized3, how the cell achieves combinatorial readout of histones bearing multiple modifications is poorly understood. One mechanism involves multivalent binding by linked effector modules4. For example, the tandem bromodomains of human TATA-binding protein-associated factor-1 (TAF1) bind better to a diacetylated histone H4 tail than to monoacetylated tails, a cooperative effect attributed to each bromodomain engaging one acetyl-lysine mark5. Here we report a distinct mechanism of combinatorial readout for the mouse TAF1 homologue Brdt, a testis-specific member of the BET protein family6. Brdt associates with hyperacetylated histone H4 (ref. 7) and is implicated in the marked chromatin remodelling that follows histone hyperacetylation during spermiogenesis, the stage of spermatogenesis in which post-meiotic germ cells mature into fully differentiated sperm7,8,9,10. Notably, we find that a single bromodomain (BD1) of Brdt is responsible for selectively recognizing histone H4 tails bearing two or more acetylation marks. The crystal structure of BD1 bound to a diacetylated H4 tail shows how two acetyl-lysine residues cooperate to interact with one binding pocket. Structure-based mutagenesis that reduces the selectivity of BD1 towards diacetylated tails destabilizes the association of Brdt with acetylated chromatin in vivo. Structural analysis suggests that other chromatin-associated proteins may be capable of a similar mode of ligand recognition, including yeast Bdf1, human TAF1 and human CBP/p300 (also known as CREBBP and EP300, respectively). Our findings describe a new mechanism for the combinatorial readout of histone modifications in which a single effector module engages two marks on a histone tail as a composite binding epitope.

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Accession codes

Primary accessions

Protein Data Bank

Data deposits

Atomic coordinates and structure factors have been deposited with the Protein Data Bank under accession codes 2WP2 (BD1) and 2WP1 (BD2).

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Acknowledgements

We thank the ESRF and EMBL staff for beamline assistance, the Partnership for Structural Biology (PSB) for access to technical platforms, M. Jamin for MALLS experiments, G. Natrajan and V. Rybin for help with ITC, C. Soucier for help with FRAP, D. Panne and C. Clapier for comments on the manuscript, and S. Cusack for critical support. Work in the S.K. laboratory was supported by ANR blanche ‘EpiSperm’ and ‘Empreinte’, INCa and ‘ARECA’ (ARC) research programmes. J.Ga. was supported by a Ph.D. fellowship from the Rhône-Alpes region. J.M. was supported by an ‘E-STAR’ fellowship funded by EU FP6. C.P. acknowledges support from the ANRS/Fondation de France AIJC and CNRS ATIP programmes.

Author Contributions M.S.-L., D.J.H., S.K. and C.W.M. initiated the study. S.K., C.P. and C.W.M. coordinated the entire project and specific author contributions. J.M., S.R., U.S., M.S.-L., A.-L.V. and D.J.H. prepared constructs. J.M., U.S. and M.S.-L. expressed, purified and crystallized BD1 and BD2. J.M. and U.S. performed and analysed ITC and biophysical experiments. J.M., M.S.-L. and C.P. measured diffraction data and solved the crystal structures. C.P. and C.W.M. analysed structural and biochemical data. J.Go. performed immunoblot analysis and immunofluorescence microscopy. S.C. and S.R. performed FRAP and chromatin compaction experiments. J.Ga. prepared histones for MS/MS analysis. K.S. and J.K. performed the MS/MS analysis. C.P. wrote the manuscript. All authors discussed the results and commented on the manuscript.

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Author notes

  1. Montserrat Soler-López
    Present address: Present address: Institute for Research in Biomedicine (IRB Barcelona), Parc Científic de Barcelona, calle Baldiri Reixac 10–12, 08028 Barcelona, Spain.,

Authors and Affiliations

  1. European Molecular Biology Laboratory, Grenoble Outstation, 6 rue Jules Horowitz, BP 181, 38042 Grenoble Cedex 9, France ,
    Jeanne Morinière, Montserrat Soler-López & Darren J. Hart
  2. Unit of Virus Host-Cell Interactions, UMI 3265 Université Joseph Fourier-EMBL-CNRS, 6 rue Jules Horowitz, BP 181, 38042 Grenoble Cedex 9, France ,
    Jeanne Morinière, Montserrat Soler-López & Darren J. Hart
  3. INSERM, U823,
    Sophie Rousseaux, Sandrine Curtet, Anne-Laure Vitte, Jérôme Govin, Jonathan Gaucher, Karin Sadoul & Saadi Khochbin
  4. Université Joseph Fourier, Institut Albert Bonniot, F-38700 Grenoble, France
    Sophie Rousseaux, Sandrine Curtet, Anne-Laure Vitte, Jérôme Govin, Jonathan Gaucher, Karin Sadoul & Saadi Khochbin
  5. European Molecular Biology Laboratory, Meyerhofstrasse 1, D-69117 Heidelberg, Germany
    Ulrich Steuerwald, Jeroen Krijgsveld & Christoph W. Müller
  6. Institut de Biologie Structurale Jean-Pierre Ebel, UMR 5075 CEA-CNRS-Université Joseph Fourier, 41 Jules Horowitz, 38027 Grenoble Cedex 1, France ,
    Carlo Petosa

Authors

  1. Jeanne Morinière
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  2. Sophie Rousseaux
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  3. Ulrich Steuerwald
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  4. Montserrat Soler-López
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  5. Sandrine Curtet
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  6. Anne-Laure Vitte
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  7. Jérôme Govin
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  8. Jonathan Gaucher
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  9. Karin Sadoul
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  10. Darren J. Hart
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  11. Jeroen Krijgsveld
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Corresponding author

Correspondence toChristoph W. Müller.

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Morinière, J., Rousseaux, S., Steuerwald, U. et al. Cooperative binding of two acetylation marks on a histone tail by a single bromodomain.Nature 461, 664–668 (2009). https://doi.org/10.1038/nature08397

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Editorial Summary

Histone modification: tail spin

Brdt1 is a bromodomain-containing chromatin protein that can compact hyperacetylated chromatin and has important functions during spermiogenesis. Here, the crystal structure of a bromodomain of Brdt1 bound to an acetylated histone H4 tail reveals a combinatorial mode of binding to post-translational modifications where a single effector module engages two marks on a histone tail.