Impact of Benzo[<i>a</i>]pyrene-2‘-deoxyguanosine Lesions On Methylation Of DNA by SssI and HhaI DNA Methyltransferases

Subach, Oksana M.; Baskunov, Vladimir B.; Дарий, М. В.; Maltseva, D. V.; Alexandrov, Dmitrii A.; Kirsanova, O. V.; Kolbanovskiy, Alexander; Kolbanovskiy, Marina; Johnson, Francis; Bonala, Radha; Geacintov, Nicholas E.; Громова, Е. С.

doi:10.1021/bi0511639

Cited by 27 publications

(44 citation statements)

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“…The impact of (+)- and (-)- trans -B[ a ]PDE- N 2 -dG adducts and (+)- cis -B[ a ]PDE- N 2 -dG adduct on methylation of 18-mer DNA duplexes by M.SssI was studied earlier [7, 8]. However, in the present work, we focused on the impact of two types of intercalative adducts that were not examined before.…”

Section: Resultsmentioning

confidence: 99%

“…The DNA substrates contained overlapping recognition sites of M.HhaI (5′-GCGC), M.SssI (5′-CG) and Dnmt3a (5′-CG). It was shown that the MTase binding affinities for 18-mer canonical DNA and 18-mer (+)- and (-)- trans -B[ a ]PDE-DNA decrease in the order M.HhaI > M.SssI > Dnmt3a-CD, with K d values in the range 10 pM – 70 nM [7, 8, 14]. The enhancement of fluorescence intensities (I 384 ) by a factor 45-50 relative to protein-free B[ a ]PDE-DNA duplexes was observed in the case of G C G t+ C/C GM G•М.SssI•AdoHcy, G t+ C G C/C GM G•M.HhaI•AdoHcy, and G C G t+ C/C GM G•M.HhaI•AdoHcy complexes with (+)- trans -B[ a ]PDE -N 2 -dG adducts positioned within the MTase recognition sites (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…In contrast, B[ a ]PDE-modified nucleotides that flank the CpG sequences on their 5′-side is crucial for the prokaryotic CpG-recognizing MTase M.SssI. In this case, methylation was either abolished in 18-mer duplexes containing B[ a ]PDE residues in the minor groove (motif A) [7], or strongly decreased in the case of 30-mer duplexes with the base-displaced intercalative (-)- cis -B[ a ]PDE- N 2 -dG adduct (motif B) (Table 3). The B[ a ]PDE- N 6 -dA adducts in the same position have less impact on the methylation rates of M.SssI.…”

Section: Resultsmentioning

confidence: 99%

“…These studies have shown that (1) the B[ a ]PDE lesions affect primarily the methylation reaction by decreasing the efficiency of the catalytic step rather than the binding of the enzymes to the carcinogen-DNA adducts, and that (2) the methylation efficiency is strongly dependent on adduct conformation and its position within the DNA substrate. For prokaryotic M.SssI, the most significant effect on the methylation efficiency was observed when DNA containing (+)- and (-)- trans -B[ a ]PDE- N 2 -dG adducts, that are known to be positioned in the minor groove [9], were positioned on the 5′-side of the CpG recognition site of the enzyme [7]. However, a number of important questions remain that have not been resolved.…”

Section: Introductionmentioning

confidence: 99%

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Probing murine methyltransfease Dnmt3a interactions with benzo[a]pyrene‐modified DNA by fluorescence methods

et al. 2012

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Summary The impact of bulky carcinogen-DNA adducts positioned at or near recognition sites (CpG) of eukaryotic DNA methyltransferases on their catalytic activities is poorly understood. In this work we have employed site-specifically modified 30-mer oligodeoxyribonucleotides containing stereoisomeric benzo[a]pyrene diol epoxide (B[a]PDE)-derived guanine (B[a]PDE-N2-dG) or adenine (B[a]PDE-N6-dA) adducts of different conformations as substrates of catalytic domain of murine Dnmt3a (Dnmt3a-CD). The fluorescence of these lesions was used to examine interactions between Dnmt3a-CD and DNA. In B[a]PDE-DNA•Dnmt3a-CD complexes the intensity of fluorescence of the covalently bound B[a]PDE residues is enhanced relative to the protein-free value when the B[a]PDE is positioned in the minor groove ((+)- and (−)-trans-B[a]PDE-N2-dG adducts in the CpG site) and when it is intercalated on the 5′-side of the CpG site ((+)-trans- B[a]PDE-N6-dA adduct). The fluorescence of B[a]PDE-modified DNA•Dnmt3a-CD complexes exhibits only small changes when the B[a]PDE is intercalated with base displacement in (+)- and (−)-cis- B[a]PDE-N2-dG adducts and without base displacement in the (−)-trans- B[a]PDE-N6-dA adduct. The initial rates of methylation were significantly reduced by the minor groove trans-B[a]PDE-N2-dG adducts regardless of their position in the substrate and by the intercalated cis-B[a]PDE-N2-dG adducts within the CpG site. The observed changes in fluorescence and methylation rates are consistent with the flipping of the target cytosine and a catalytic loop motion within the DNA•Dnmt3a-CD complexes. In the presence of the regulatory factor Dnmt3L, an enhancement of the methylation rates and fluorescence were observed which is consistent with a Dnmt3L-mediated displacement of the catalytic loop towards the CpG site.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Probing murine methyltransfease Dnmt3a interactions with benzo[a]pyrene‐modified DNA by fluorescence methods

et al. 2012

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“…In addition, disposition of Hoechst 33258 in the DNA minor groove was demonstrated for type I and II complexes with poly(dGdC)·poly(dG-dC) 28 . Recently we found that the presence of a bulky benzo[a]pyrene residue in the DNA minor groove caused a dramatic decrease in prokaryotic MTases SssI and HhaI methylating capacity because of distortion of DNA contacts with the enzyme catalytic loop 29,30 . Superimposition of the DNA methyltransferase HhaI (M.HhaI-DNA) complex structure onto the Dnmt3a-CD structure showed high similarity of M.HhaI and Dnmt3a-CD catalytic loop conformations 7 .…”

Section: Resultsmentioning

confidence: 99%

Dimeric bisbenzimidazoles inhibit the DNA methylation catalyzed by the murine Dnmt3a catalytic domain

Cherepanova

Ivanov

Maltseva

et al. 2010

Journal of Enzyme Inhibition and Medicinal Chemistry

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Effects of benzene and its metabolites on global DNA methylation in human normal hepatic l02 cells

Zhang

et al. 2011

Environmental Toxicology

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Benzene is an important industrial chemical that is also widely present in cigarette smoke, automobile exhaust, and gasoline. It is reported that benzene can cause hematopoietic disorders and has been recognized as a human carcinogen. However, the mechanisms by which it increases the risk of carcinogenesis are only partially understood. Aberrant DNA methylation is a major epigenetic mechanism associated with the toxicity of carcinogens. To understand the carcinogenic capacity of benzene, experiments were designed to investigate whether exposure to benzene and its metabolites would change the global DNA methylation status in human normal hepatic L02 cells and then to evaluate whether the changes would be induced by variation of DNA methyltransferase (DNMT) activity in HaeIII DNMT-mediated methylation assay in vitro. Our results showed that hydroquinone and 1,4-benzoquinone could induce global DNA hypomethylation with statistically significant difference from control (p \ 0.05), but no significant global DNA methylation changes were observed in L02 cells with benzene, phenol, and 1,2,4-trihydroxybenzene exposure. Benzene metabolites could not influence HaeIII DNMT activity except that 1,4-benzoquinone shows significantly inhibiting effect on enzymatic methylation reaction at concentrations of 5 lM (p \ 0.05). These results suggest that benzene metabolites, hydroquinone, and 1,4-benzoquinone can disrupt global DNA methylation, and the potential epigenetic mechanism by which that global DNA hypomethylation induced by 1,4-benzoquinone may work through the inhibiting effects of DNMT activity at 10 lM (p \ 0.05). #

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Impact of Benzo[a]pyrene-2‘-deoxyguanosine Lesions On Methylation Of DNA by SssI and HhaI DNA Methyltransferases

Cited by 27 publications

References 83 publications

Probing murine methyltransfease Dnmt3a interactions with benzo[a]pyrene‐modified DNA by fluorescence methods

Probing murine methyltransfease Dnmt3a interactions with benzo[a]pyrene‐modified DNA by fluorescence methods

Dimeric bisbenzimidazoles inhibit the DNA methylation catalyzed by the murine Dnmt3a catalytic domain

Effects of benzene and its metabolites on global DNA methylation in human normal hepatic l02 cells

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