4.1 Article

Biochemical and Structural Studies of Conserved Maf Proteins Revealed Nucleotide Pyrophosphatases with a Preference for Modified Nucleotides

期刊

CHEMISTRY & BIOLOGY
卷 20, 期 11, 页码 1386-1398

出版社

CELL PRESS
DOI: 10.1016/j.chembiol.2013.09.011

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资金

  1. Government of Canada through Genome Canada
  2. Ontario Genomics Institute [2009-OGI-ABC-1405, OGI-055]
  3. Ontario Research Fund [ORFGL2-01-004]
  4. COMBREX
  5. UK Medical Research Council [MC_U105192716]
  6. Natural Sciences and Engineering Research Council
  7. Canadian Institutes of Health Research
  8. National Institutes of Health [P50GM071508, 1R01CA16359-01A1]
  9. Canada Foundation for Innovation
  10. Eli Lilly Canada
  11. GlaxoSmithKline
  12. Ontario Ministry of Economic Development and Innovation
  13. Novartis Research Foundation
  14. Pfizer
  15. AbbVie
  16. Takeda
  17. Janssen
  18. Boehringer Ingelheim
  19. Wellcome Trust
  20. Medical Research Council [MC_U105192716] Funding Source: researchfish
  21. MRC [MC_U105192716] Funding Source: UKRI

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Maf (for multicopy associated filamentation) proteins represent a large family of conserved proteins implicated in cell division arrest but whose biochemical activity remains unknown. Here, we show that the prokaryotic and eukaryotic Maf proteins exhibit nucleotide pyrophosphatase activity against 5-methyl-UTP, pseudo-UTP, 5-methyl-CTP, and 7-methyl-GTP, which represent the most abundant modified bases in all organisms, as well as against canonical nucleotides dTTP, UTP, and CTP. Overexpression of the Maf protein YhdE. in E. coli cells increased intracellular levels of dTMP and UMP, confirming that dTTP and UTP are the in vivo substrates of this protein. Crystal structures and site-directed mutagenesis of Maf proteins revealed the determinants of their activity and substrate specificity. Thus, pyrophosphatase activity of Maf proteins toward canonical and modified nucleotides might provide the molecular mechanism for a dual role of these proteins in cell division arrest and house cleaning.

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