Literature DB >> 20122942

Crystal structure of the first eubacterial Mre11 nuclease reveals novel features that may discriminate substrates during DNA repair.

Debanu Das1, Davide Moiani, Herbert L Axelrod, Mitchell D Miller, Daniel McMullan, Kevin K Jin, Polat Abdubek, Tamara Astakhova, Prasad Burra, Dennis Carlton, Hsiu-Ju Chiu, Thomas Clayton, Marc C Deller, Lian Duan, Dustin Ernst, Julie Feuerhelm, Joanna C Grant, Anna Grzechnik, Slawomir K Grzechnik, Gye Won Han, Lukasz Jaroszewski, Heath E Klock, Mark W Knuth, Piotr Kozbial, S Sri Krishna, Abhinav Kumar, David Marciano, Andrew T Morse, Edward Nigoghossian, Linda Okach, Jessica Paulsen, Ron Reyes, Christopher L Rife, Natasha Sefcovic, Henry J Tien, Christine B Trame, Henry van den Bedem, Dana Weekes, Qingping Xu, Keith O Hodgson, John Wooley, Marc-André Elsliger, Ashley M Deacon, Adam Godzik, Scott A Lesley, John A Tainer, Ian A Wilson.   

Abstract

Mre11 nuclease plays a central role in the repair of cytotoxic and mutagenic DNA double-strand breaks. As X-ray structural information has been available only for the Pyrococcus furiosus enzyme (PfMre11), the conserved and variable features of this nuclease across the domains of life have not been experimentally defined. Our crystal structure and biochemical studies demonstrate that TM1635 from Thermotoga maritima, originally annotated as a putative nuclease, is an Mre11 endo/exonuclease (TmMre11) and the first such structure from eubacteria. TmMre11 and PfMre11 display similar overall structures, despite sequence identity in the twilight zone of only approximately 20%. However, they differ substantially in their DNA-specificity domains and in their dimeric organization. Residues in the nuclease domain are highly conserved, but those in the DNA-specificity domain are not. The structural differences likely affect how Mre11 from different organisms recognize and interact with single-stranded DNA, double-stranded DNA and DNA hairpin structures during DNA repair. The TmMre11 nuclease active site has no bound metal ions, but is conserved in sequence and structure with the exception of a histidine that is important in PfMre11 nuclease activity. Nevertheless, biochemical characterization confirms that TmMre11 possesses both endonuclease and exonuclease activities on single-stranded and double-stranded DNA substrates, respectively. Copyright 2010 Elsevier Ltd. All rights reserved.

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Year:  2010        PMID: 20122942      PMCID: PMC2839085          DOI: 10.1016/j.jmb.2010.01.049

Source DB:  PubMed          Journal:  J Mol Biol        ISSN: 0022-2836            Impact factor:   5.469


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