Solution Structure of the Minor Conformer of a DNA Duplex Containing a dG Mismatch Opposite a Benzo[<i>a</i>]pyrene Diol Epoxide/dA Adduct:  Glycosidic Rotation from Syn to Anti at the Modified Deoxyadenosine

Schwartz, Jean-Louis; Rice, Jeffrey S.; Luxon, Bruce A.; Sayer, Jane M.; Xie, Guo-Jun; Yeh, Herman J. C.; Liu, X.; Jerina, Donald M.; Gorenstein, David G.

doi:10.1021/bi971306u

Cited by 48 publications

(105 citation statements)

References 18 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…20,21 The 10R(Ϫ)-trans-anti adduct structure shown is essentially the same as that of the NMR solution structure of Zegar et al 22 determined in the same C[A*]A sequence context of codon 61 of the human N-ras gene.…”

Section: Adduct Structuressupporting

confidence: 58%

“…NMR solution structures provided starting models for these simulations. 16,17,21,22 gives rise to multiple and poorly resolved NMR resonances, as well as line broadening, all of which preclude a determination of a high-resolution structure for this stereoisomeric adduct. 21,[23][24][25] However, when the T complementary to the 10S(ϩ)-trans-anti-B[a]P-N 6 -dA is replaced by a mismatched G two different conformations were discerned and characterized.…”

Section: S(ϩ) Trans-anti-b[a]p-nmentioning

confidence: 99%

“…16,17,21,22 gives rise to multiple and poorly resolved NMR resonances, as well as line broadening, all of which preclude a determination of a high-resolution structure for this stereoisomeric adduct. 21,[23][24][25] However, when the T complementary to the 10S(ϩ)-trans-anti-B[a]P-N 6 -dA is replaced by a mismatched G two different conformations were discerned and characterized. Although the major conformer has the glycosidic torsion angle, , at the modified adenine in the syn conformation, and the minor conformer has in the anti conformation, 21,24 in both cases the aromatic B[a]P residue is oriented on the 3Ј-side of the lesion, as it is in the stereochemically related 1S(Ϫ)-trans-…”

Section: S(ϩ) Trans-anti-b[a]p-nmentioning

confidence: 99%

“…5 Because of this absence of an experimental NMR solution structure for the 10S(ϩ)-trans-anti adduct with normal partner dT opposite the lesion, molecular dynamics simulations were employed to elucidate their structures. 19 The NMR solution structure of Schwartz et al 21 in a duplex with an A*:G mismatch was remodeled 19 to the human N-ras codon 61 sequence I, with fully complementary A*:T base pair at the lesion site (Figure 4). The anti conformer for the glycosidic torsion angle was employed as the starting model because the normal partner dT was investigated.…”

Section: S(ϩ) Trans-anti-b[a]p-nmentioning

confidence: 99%

See 3 more Smart Citations

Thermodynamic and structural factors in the removal of bulky DNA adducts by the nucleotide excision repair machinery

et al. 2002

View full text Add to dashboard Cite

The function of the human nucleotide excision repair (NER) apparatus is to remove bulky adducts from damaged DNA. In an effort to gain insights into the molecular mechanisms involved in the recognition and excision of bulky lesions, we investigated a series of site specifically modified oligonucleotides containing single, well-defined polycyclic aromatic hydrocarbon (PAH) diol epoxide-adenine adducts. Covalent adducts derived from the bay region PAH, benzo[a]pyrene, are removed by human NER enzymes in vitro. In contrast, the stereochemically analogous N(6)-dA adducts derived from the topologically different fjord region PAH, benzo[c]phenanthrene, are resistant to repair. The evasion of DNA repair may play a role in the observed higher tumorigenicity of the fjord region PAH diol epoxides. We are elucidating the structural and thermodynamic features of these adducts that may underlie their marked distinction in biologic function, employing high-resolution nuclear magnetic resonance studies, measurements of thermal stabilities of the PAH diol epoxide-modified oligonucleotide duplexes, and molecular dynamics simulations with free energy calculations. Our combined findings suggest that differences in the thermodynamic properties and thermal stabilities are associated with differences in distortions to the DNA induced by the lesions. These structural effects correlate with the differential NER susceptibilities and stem from the intrinsically distinct shapes of the fjord and bay region PAH diol epoxide-N(6)-adenine adducts.

show abstract

Section: Adduct Structuressupporting

confidence: 58%

Section: S(ϩ) Trans-anti-b[a]p-nmentioning

confidence: 99%

Section: S(ϩ) Trans-anti-b[a]p-nmentioning

confidence: 99%

Section: S(ϩ) Trans-anti-b[a]p-nmentioning

confidence: 99%

See 2 more Smart Citations

Thermodynamic and structural factors in the removal of bulky DNA adducts by the nucleotide excision repair machinery

et al. 2002

View full text Add to dashboard Cite

show abstract

“…It has been shown that the stability of a (ϩ)-anti-trans-BPDE-adducted adenine mismatched with dG is significantly higher than the stability of the adducted adenine paired with the correct dT (41,43). This suggests that the differences in stability between the incorrect and correct base pairs containing the different diastereomers may play a role in BPDEinduced mutagenesis.…”

Section: Discussionmentioning

confidence: 99%

Highly Mutagenic Bypass Synthesis by T7 RNA Polymerase of Site-specific Benzo[a]pyrene Diol Epoxide-adducted Template DNA

Remington

Bennett

Harris

et al. 1998

Journal of Biological Chemistry

View full text Add to dashboard Cite

We have previously developed an in vitro system that allows quantitative evaluation of the fidelity of transcription during synthesis on a natural template in the presence of all four nucleotides. Here, we have employed this system using a TAA ochre codon reversion assay to examine the fidelity of transcription by T7 RNA polymerase past an adenine residue adducted at the N 6 -position with (؊)-anti-trans-or (؉)-anti-trans-benzo-[a]pyrene diol epoxide (BPDE). T7 RNAP was capable of transcribing past either BPDE isomer to generate fulllength run-off transcripts. The extent of bypass was found to be 32% for the (؊)-anti-trans-isomer and 18% for the (؉)-anti-trans-isomer. Transcription past both adducts was highly mutagenic. The reversion frequency of bypass synthesis of the (؊)-anti-trans-isomer was elevated 11,000-fold and that of the (؉)-anti-trans-isomer 6000-fold, relative to the reversion frequency of transcription on unadducted template. Adenine was misinserted preferentially, followed by guanine, opposite the adenine adducted with either BPDE isomer. Although base substitution errors were by far the most frequent mutation on the adducted template, three-and six-base deletions were also observed. These results suggest that transcriptional errors, particularly with regard to damage bypass, may contribute to the mutational burden of the cell.It is well documented that genomic instability can result from errors made during DNA replication, repair, or recombination. However, less is known concerning the effects of inaccurate transcription and/or translation on the integrity of the genetic information. Transcriptional and translational errors may lead to production of mutant proteins. If the defective protein is involved in DNA replication or repair, then even its transient presence may result in permanent changes in the cell's DNA. In fact, a recent paper by Slupska et al. (1) suggests that translational miscoding may result in a mutator phenotype in Escherichia coli due to production of mutant DNA polymerases with dysfunctional proofreading activity.A likely source of transcriptional errors is damage to the DNA template and/or ribonucleotide pools. Some DNA lesions, such as UV light-induced cyclobutane dimers, block the progression of RNA polymerase (2). Such lesions have been shown to be preferentially repaired, relative to other parts of the genome, when present in the template strand of an actively transcribed gene (3-4). However, lesions that are bypassed by the polymerase may result in erroneous transcripts that, if translated, will give rise to mutant proteins. The biological consequences of transcriptional mutagenesis may be particularly significant in nondividing cells in which some mutant proteins may accumulate over time. Evidence presented by van Leeuwen et al. (5) points to transcription errors as a possible source of a mutant form of ␤-amyloid precursor protein found in neurons of Alzheimer's and Down's syndrome patients. Deposition of this mutant protein in neuritic plaque is probably involved in...

show abstract

Recognition and Removal of Bulky DNA Lesions by the Nucleotide Excision Repair System

Cai

Kropachev

Kolbanovskiy

et al. 2010

The Chemical Biology of DNA Damage

View full text Add to dashboard Cite

Solution Structure of the Minor Conformer of a DNA Duplex Containing a dG Mismatch Opposite a Benzo[a]pyrene Diol Epoxide/dA Adduct: Glycosidic Rotation from Syn to Anti at the Modified Deoxyadenosine

Cited by 48 publications

References 18 publications

Thermodynamic and structural factors in the removal of bulky DNA adducts by the nucleotide excision repair machinery

Thermodynamic and structural factors in the removal of bulky DNA adducts by the nucleotide excision repair machinery

Highly Mutagenic Bypass Synthesis by T7 RNA Polymerase of Site-specific Benzo[a]pyrene Diol Epoxide-adducted Template DNA

Recognition and Removal of Bulky DNA Lesions by the Nucleotide Excision Repair System

Contact Info

Product

Resources

About