| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2029646 | Structure | 2014 | 14 Pages |
•The crystal structure of the complete vaccinia virus capping enzyme is presented•TPase has a triphosphate tunnel metalloenzyme fold•The extensive TPase-GTase interface clamps GTase in a closed conformation•TPase-GTase interfacial mutations selectively cripple GTase activity
SummaryVaccinia virus capping enzyme is a heterodimer of D1 (844 aa) and D12 (287 aa) polypeptides that executes all three steps in m7GpppRNA synthesis. The D1 subunit comprises an N-terminal RNA triphosphatase (TPase)-guanylyltransferase (GTase) module and a C-terminal guanine-N7-methyltransferase (MTase) module. The D12 subunit binds and allosterically stimulates the MTase module. Crystal structures of the complete D1⋅D12 heterodimer disclose the TPase and GTase as members of the triphosphate tunnel metalloenzyme and covalent nucleotidyltransferase superfamilies, respectively, albeit with distinctive active site features. An extensive TPase-GTase interface clamps the GTase nucleotidyltransferase and OB-fold domains in a closed conformation around GTP. Mutagenesis confirms the importance of the TPase-GTase interface for GTase activity. The D1⋅D12 structure complements and rationalizes four decades of biochemical studies of this enzyme, which was the first capping enzyme to be purified and characterized, and provides new insights into the origins of the capping systems of other large DNA viruses.
Graphical AbstractFigure optionsDownload full-size imageDownload high-quality image (382 K)Download as PowerPoint slide
