4.5 Article

Molecular Basis of C-N Bond Cleavage by the Glycyl Radical Enzyme Choline Trimethylamine-Lyase

Journal

CELL CHEMICAL BIOLOGY
Volume 23, Issue 10, Pages 1206-1216

Publisher

CELL PRESS
DOI: 10.1016/j.chembiol.2016.07.020

Keywords

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Funding

  1. HHMI International Student Research Fellowship
  2. National Science Foundation Graduate Research Fellowship [0645960]
  3. Richard and Susan Smith Family Foundatio
  4. Packard Fellowship for Science and Engineering
  5. National Center for Research Resources at the National Institute of Health [GM103403]
  6. Office of Research Infrastructure Programs High-End Instrumentation [S10 RR029205]
  7. U.S. Department of Energy, Office of Basic Energy Sciences [DE-AC02-06CH11357]

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Deamination of choline catalyzed by the glycyl radical enzyme choline trimethylamine-lyase (CutC) has emerged as an important route for the production of trimethylamine, a microbial metabolite associated with both human disease and biological methane production. Here, we have determined five high-resolution X-ray structures of wild-type CutC and mechanistically informative mutants in the presence of choline. Within an unexpectedly polar active site, CutC orients choline through hydrogen bonding with a putative general base, and through close interactions between phenolic and carboxylate oxygen atoms of the protein scaffold and the polarized methyl groups of the trimethylammonium moiety. These structural data, along with biochemical analysis of active site mutants, support a mechanism that involves direct elimination of trimethylamine. This work broadens our understanding of radical-based enzyme catalysis and will aid in the rational design of inhibitors of bacterial trimethylamine production.

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