4.3 Article

Role of the catalytic metal during polymerization by DNA polymerase lambda

Journal

DNA REPAIR
Volume 6, Issue 9, Pages 1333-1340

Publisher

ELSEVIER SCIENCE BV
DOI: 10.1016/j.dnarep.2007.03.005

Keywords

DNA polymerase lambda; DNA repair; nucleotidyl transfer; phosphoryl transfer; X-ray crystallography; crystal structure; divalent metal; catalysis; manganese; non-hydrolyzable nucleotide

Funding

  1. Intramural NIH HHS [Z01 ES065070-17] Funding Source: Medline

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The incorporation of dNMPs into DNA by polymerases involves a phosphoryl transfer reaction hypothesized to require two divalent metal ions. Here we investigate this hypothesis using as a model human DNA polymerase lambda (Pol lambda), an enzyme suggested to be activated in vivo by manganese. We report the crystal structures of four complexes of human Pol X. In a 1.9 angstrom structure of Pol lambda containing a 3'-OH and the non-hydrolyzable analog dUpnpp, a non-catalytic Na+ ion occupies the site for metal A and the ribose of the primer-terminal nucleotide is found in a conformation that positions the acceptor 3'-OH out of line with the a-phosphate and the bridging oxygen of the pyrophosphate leaving group. Soaking this crystal in MnCl2 yielded a 2.0 angstrom structure with Mn2+ occupying the site for metal A. In the presence of Mn2+, the conformation of the ribose is C3'-endo and the 3'-oxygen is in line with the leaving oxygen, at a distance from the phosphorus atom of the alpha-phosphate (3.69 angstrom) consistent with and supporting a catalytic mechanism involving two divalent metal ions. Finally, soaking with MnCl2 converted a pre-catalytic Pol lambda/Na+ complex with unreacted dCTP in the active site into a product complex via catalysis in the crystal. These data provide pre- and post-transition state information and outline in a single crystal the pathway for the phosphoryl transfer reaction carried out by DNA polymerases. Published by Elsevier B.V.

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