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Publication : Enzyme mechanism-based, oxidative DNA-protein cross-links formed with DNA polymerase β in vivo.

First Author  Quiñones JL Year  2015
Journal  Proc Natl Acad Sci U S A Volume  112
Issue  28 Pages  8602-7
PubMed ID  26124145 Mgi Jnum  J:223801
Mgi Id  MGI:5660425 Doi  10.1073/pnas.1501101112
Citation  Quinones JL, et al. (2015) Enzyme mechanism-based, oxidative DNA-protein cross-links formed with DNA polymerase beta in vivo. Proc Natl Acad Sci U S A 112(28):8602-7
abstractText  Free radical attack on the C1' position of DNA deoxyribose generates the oxidized abasic (AP) site 2-deoxyribonolactone (dL). Upon encountering dL, AP lyase enzymes such as DNA polymerase beta (Polbeta) form dead-end, covalent intermediates in vitro during attempted DNA repair. However, the conditions that lead to the in vivo formation of such DNA-protein cross-links (DPC), and their impact on cellular functions, have remained unknown. We adapted an immuno-slot blot approach to detect oxidative Polbeta-DPC in vivo. Treatment of mammalian cells with genotoxic oxidants that generate dL in DNA led to the formation of Polbeta-DPC in vivo. In a dose-dependent fashion, Polbeta-DPC were detected in MDA-MB-231 human cells treated with the antitumor drug tirapazamine (TPZ; much more Polbeta-DPC under 1% O2 than under 21% O2) and even more robustly with the "chemical nuclease" 1,10-copper-ortho-phenanthroline, Cu(OP)2. Mouse embryonic fibroblasts challenged with TPZ or Cu(OP)2 also incurred Polbeta-DPC. Nonoxidative agents did not generate Polbeta-DPC. The cross-linking in vivo was clearly a result of the base excision DNA repair pathway: oxidative Polbeta-DPC depended on the Ape1 AP endonuclease, which generates the Polbeta lyase substrate, and they required the essential lysine-72 in the Polbeta lyase active site. Oxidative Polbeta-DPC had an unexpectedly short half-life ( approximately 30 min) in both human and mouse cells, and their removal was dependent on the proteasome. Proteasome inhibition under Cu(OP)2 treatment was significantly more cytotoxic to cells expressing wild-type Polbeta than to cells with the lyase-defective form. That observation underscores the genotoxic potential of oxidative Polbeta-DPC and the biological pressure to repair them.
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