4.7 Article

Structural Insights into the Recognition of Mono- and Diacetylated Histones by the ATAD2B Bromodomain

Journal

JOURNAL OF MEDICINAL CHEMISTRY
Volume 63, Issue 21, Pages 12799-12813

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.jmedchem.0c01178

Keywords

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Funding

  1. National Institutes of Health [R01GM129338, R44GM116584, R44GM117683, R15GM104865]
  2. NIH [P41GM103399, S10RR02781, S10RR08438, S10RR023438, S10RR025062, S10RR029220]
  3. University of Wisconsin.Madison
  4. NSF [DMB-8415048, OIA-9977486, BIR9214394]
  5. USDA
  6. National Institutes of Health - National Cancer Institute [P01CA098993, R01CA52040]
  7. National Cancer Institute [ACB-12002]
  8. National Institute of General Medical Sciences [AGM-12006]
  9. DOE Office of Science [DE-AC02-06CH11357]
  10. University of Vermont Cancer Center
  11. Lake Champlain Cancer Research Organization
  12. UVM Larner College of Medicine
  13. NIH (NIGMS) [P20GM103449]

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Bromodomains exhibit preferences for specific patterns of post-translational modifications on core and variant histone proteins. We examined the ligand specificity of the ATAD2B bromodomain and compared it to its closely related paralogue in ATAD2. We show that the ATAD2B bromodomain recognizes mono- and diacetyllysine modifications on histones H4 and H2A. A structure-function approach was used to identify key residues in the acetyllysine-binding pocket that dictate the molecular recognition process, and we examined the binding of an ATAD2 bromodomain inhibitor by ATAD2B. Our analysis demonstrated that critical contacts required for bromodomain inhibitor coordination are conserved between the ATAD2/B bromodomains, with many residues playing a dual role in acetyllysine recognition. We further characterized an alternative splice variant of ATAD2B that results in a loss of function. Our results outline the structural and functional features of the ATAD2B bromodomain and identify a novel mechanism regulating the interaction of the ATAD2B protein with chromatin.

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