Literature DB >> 29053918

Active Site Interactions Impact Phosphoryl Transfer during Replication of Damaged and Undamaged DNA by Escherichia coli DNA Polymerase I.

A S Prakasha Gowda1, Thomas E Spratt1.   

Abstract

Replicative DNA polymerases are able to discriminate between very similar substrates with high accuracy. One mechanism by which E. coli DNA polymerase I checks for Watson-Crick geometry is through a hydrogen bonding fork between Arg668 and the incoming dNTP and the minor groove of the primer terminus. The importance of the Arg-fork was examined by disrupting it with either a guanine to 3-deazaguanine substitution at the primer terminus or the use of a carbocyclic deoxyribose analog of dUTP. Using thio-substituted dNTPs and differential quench techniques, we determined that when the Arg-fork was disrupted, the rate-limiting step changed from a conformational change to phosphodiester bond formation. This result indicates that Arg668 is involved in the phosphoryl transfer step. We examined the role of the Arg-fork in the replication of four DNA damaged templates, O6-methylguanine (O6-mG), 8-oxo-7,8-dihydroguanine (oxoG), O2-[4-(3-pyridyl)-4-oxobutyl]thymine (O2-POB-T), and N2-[(7S,8R,9S,10R)-7,8,9,10-tetrahydro-8,9,10-trihydroxybenzo[a]pyren-7-yl]-guanine (N2-BP-G). In general, the guanine to 3-deazaguanine substitution caused a decrease in kpol that was proportional to kpol over five orders of magnitude. The linear relationship indicates that the Arg668-fork helps catalyze phosphoryl transfer by the same mechanism with all the substrates. Exceptions to the linear relationship were the incorporations of dTTP opposite G, oxoG, and O6mG, which showed large decreases in kpol, similar to that exhibited by the Watson-Crick base pairs. It was proposed that the incorporation of dTTP opposite G, oxoG, and O6mG occurred via Watson-Crick-like structures.

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Year:  2017        PMID: 29053918      PMCID: PMC5696056          DOI: 10.1021/acs.chemrestox.7b00257

Source DB:  PubMed          Journal:  Chem Res Toxicol        ISSN: 0893-228X            Impact factor:   3.739


  93 in total

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5.  Error-free and error-prone lesion bypass by human DNA polymerase kappa in vitro.

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6.  Misincorporation and stalling at O(6)-methylguanine and O(6)-benzylguanine: evidence for inactive polymerase complexes.

Authors:  Adrienne M Woodside; F Peter Guengerich
Journal:  Biochemistry       Date:  2002-01-22       Impact factor: 3.162

7.  Analysis of pyridyloxobutyl DNA adducts in F344 rats chronically treated with (R)- and (S)-N'-nitrosonornicotine.

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Journal:  Chem Res Toxicol       Date:  2007-02       Impact factor: 3.739

8.  Protonated base pairs explain the ambiguous pairing properties of O6-methylguanine.

Authors:  L D Williams; B R Shaw
Journal:  Proc Natl Acad Sci U S A       Date:  1987-04       Impact factor: 11.205

9.  Kinetics of extension of O6-methylguanine paired with cytosine or thymine in defined oligonucleotide sequences.

Authors:  M K Dosanjh; G Galeros; M F Goodman; B Singer
Journal:  Biochemistry       Date:  1991-12-10       Impact factor: 3.162

10.  How a homolog of high-fidelity replicases conducts mutagenic DNA synthesis.

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Journal:  Nat Struct Mol Biol       Date:  2015-03-16       Impact factor: 15.369

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