C8-Heteroaryl-2′-deoxyguanosine Adducts as Conformational Fluorescent Probes in the NarI Recognition Sequence

Rankin, Katherine M.; Sproviero, Michael; Rankin, Keegan; Sharma, Purshotam; Wetmore, Stacey D.; Manderville, Richard A.

doi:10.1021/jo302164c

Cited by 34 publications

(60 citation statements)

References 68 publications

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“…Structural parameters for the free nucleoside adducts were determined using DFT calculations at the B3LYP/6–31G(d) level. Fully optimized anti and syn minima and transition states on the potential energy surface for the PhG and QG nucleoside adducts are displayed in Supplementary Figures S1 and S2, whereas the corresponding data for FurG ( 49 ) and CNPhG ( 50 ) is published elsewhere. C8-Aryl ring size governs the degree of syn preference ( E anti - E syn = 19.3 for FurG versus 29.5 kJ mol −1 for QG) and the degree of twist ( θ ) between the nucleobase and the C8-aryl substituent ( θ = 343.8º for FurG versus 305.6º for QG, Table 2 ).…”

Section: Resultsmentioning

confidence: 99%

“…C8-aryl = furyl (FurG), phenyl (PhG), 4-cyanophenyl (CNPhG) and quinolyl (QG), Figure 1b ) chosen for this study differ in their ring size (5-membered ring in FurG versus 6-membered ring in PhG and CNPhG versus fused ring in QG), type of substituent (PhG versus CNPhG) and ring type (carbocyclic rings in PhG and CNPhG versus heterocyclic rings in FurG and QG). This series of adducts was designed on the basis of their structural similarities to natural carcinogen DNA-adducts, but having interesting fluorescence properties that we could exploit to define their conformations in DNA ( 49 – 51 ) and establish the relationship between adduct structure and mutagenicity in vitro . Among these adducts, PhG is a known adduct derived from the carcinogen phenylhydrazine ( vide supra ).…”

Section: Introductionmentioning

confidence: 99%

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Structural and biochemical impact of C8-aryl-guanine adducts within the NarI recognition DNA sequence: influence of aryl ring size on targeted and semi-targeted mutagenicity

Sproviero

Verwey

Rankin

et al. 2014

Nucleic Acids Research

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201

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Chemical mutagens with an aromatic ring system may be enzymatically transformed to afford aryl radical species that preferentially react at the C8-site of 2′-deoxyguanosine (dG). The resulting carbon-linked C8-aryl-dG adduct possesses altered biophysical and genetic coding properties compared to the precursor nucleoside. Described herein are structural and in vitro mutagenicity studies of a series of fluorescent C8-aryl-dG analogues that differ in aryl ring size and are representative of authentic DNA adducts. These structural mimics have been inserted into a hotspot sequence for frameshift mutations, namely, the reiterated G3-position of the NarI sequence within 12mer (NarI(12)) and 22mer (NarI(22)) oligonucleotides. In the NarI(12) duplexes, the C8-aryl-dG adducts display a preference for adopting an anti-conformation opposite C, despite the strong syn preference of the free nucleoside. Using the NarI(22) sequence as a template for DNA synthesis in vitro, mutagenicity of the C8-aryl-dG adducts was assayed with representative high-fidelity replicative versus lesion bypass Y-family DNA polymerases, namely, Escherichia coli pol I Klenow fragment exo− (Kf−) and Sulfolobus solfataricus P2 DNA polymerase IV (Dpo4). Our experiments provide a basis for a model involving a two-base slippage and subsequent realignment process to relate the miscoding properties of C-linked C8-aryl-dG adducts with their chemical structures.

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Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Structural and biochemical impact of C8-aryl-guanine adducts within the NarI recognition DNA sequence: influence of aryl ring size on targeted and semi-targeted mutagenicity

Sproviero

Verwey

Rankin

et al. 2014

Nucleic Acids Research

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201

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“…To explore the preferred conformations of OTB-dG adducted DNA, the present work undertakes an extensive molecular modeling study, including molecular dynamics (MD) simulations and post-processing free energy calculations, to determine the conformational preferences of OTB-dG adducted DNA in three protonation states at the G 1 , G 2 or G 3 sites in the Nar I sequence (5′–CTC G 1 G 2 CG 3 CC ATC–3′) opposite complementary cytosine. The center of this sequence (underlined) is the recognition site of the Nar I Type II restriction endonuclease, which is the most vulnerable hotspot for deletion mutations induced by carcinogenic N-linked C8-dG adducts ( 45 ), and the site-specific incorporation of a variety of C8-linked adducts has been studied in this sequence ( 41 , 46 – 50 ). Since OTA exposure has been linked to an increase in the frequency of deletion mutations at carcinogenic target sites ( 20 , 26 ), we chose the Nar I sequence to study the conformational preferences of the OTB-dG lesion.…”

Section: Introductionmentioning

confidence: 99%

Structural and energetic characterization of the major DNA adduct formed from the food mutagen ochratoxin A in the NarI hotspot sequence: influence of adduct ionization on the conformational preferences and implications for the NER propensity

Sharma

Manderville

Wetmore

2014

Nucleic Acids Research

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The nephrotoxic food mutagen ochratoxin A (OTA) produces DNA adducts in rat kidneys, the major lesion being the C8-linked-2′-deoxyguanosine adduct (OTB-dG). Although research on other adducts stresses the importance of understanding the structure of the associated adducted DNA, site-specific incorporation of OTB-dG into DNA has yet to be attempted. The present work uses a robust computational approach to determine the conformational preferences of OTB-dG in three ionization states at three guanine positions in the NarI recognition sequence opposite cytosine. Representative adducted DNA helices were derived from over 2160 ns of simulation and ranked via free energies. For the first time, a close energetic separation between three distinct conformations is highlighted, which indicates OTA-adducted DNA likely adopts a mixture of conformations regardless of the sequence context. Nevertheless, the preferred conformation depends on the flanking bases and ionization state due to deviations in discrete local interactions at the lesion site. The structural characteristics of the lesion thus discerned have profound implications regarding its repair propensity and mutagenic outcomes, and support recent experiments suggesting the induction of double-strand breaks and deletion mutations upon OTA exposure. This combined structural and energetic characterization of the OTB-dG lesion in DNA will encourage future biochemical experiments on this potentially genotoxic lesion.

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“…For the free Fur dG nucleoside, the syn-conformation is more stable than the anti-structure by ~ 19 kJ mol −1 , based on DFT calculations. 21 Consequently, Fur dG stabilized an antiparallel GQ formed by the 15-mer thrombin-binding aptamer (TBA) when substituted for a syn-G (increase in T m by ~ 9 °C compared to native TBA in K + buffer), but destabilized the GQ when substituted for an anti-G (decrease in T m by ~ −11 °C). 19 The positions chosen for modification within HTelo22 included G3, G4, G8 and G10.…”

Section: Resultsmentioning

confidence: 99%

Positional Impact of Fluorescently Modified G-Tetrads within Polymorphic Human Telomeric G-Quadruplex Structures

et al. 2015

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Emissive C8-aryl-2'-deoxyguanosines placed within G-tetrads of G-quadruplex structures are useful probes for distinguishing G-quadruplexes from duplex structures using fluorescence spectroscopy. Here, we report the positional impact of C8-furyl-dG ((Fur)dG) on G-quadruplex folding in the human telomere 22-mer oligonucleotide (HTelo22, (d[AG3(T2AG3)3])). The (Fur)dG probe was inserted into four different positions within the three unique G-tetrads of HTelo22, and G-quadruplex folding was monitored by UV-vis thermal denaturation, circular dichroism, and fluorescence spectroscopy. Our studies demonstrate the impacts of C8-aryl-dG adduct formation on G-quadruplex polymorphism in K(+) solution and in the presence of the additives and cosolutes, CH3CN, polyethylene glycol (PEG-600), and N-methyl mesoporphyrin IX (NMM). Our experiments predict that C8-aryl-dG derivatives can serve as useful tools for various in vitro studies aimed at understanding both the implications of DNA adduct formation within G-quadruplex structures and the unique implications imposed by various folding topologies on biological function/recognition.

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C⁸-Heteroaryl-2′-deoxyguanosine Adducts as Conformational Fluorescent Probes in the NarI Recognition Sequence

Cited by 34 publications

References 68 publications

Structural and biochemical impact of C8-aryl-guanine adducts within the NarI recognition DNA sequence: influence of aryl ring size on targeted and semi-targeted mutagenicity

Structural and biochemical impact of C8-aryl-guanine adducts within the NarI recognition DNA sequence: influence of aryl ring size on targeted and semi-targeted mutagenicity

Structural and energetic characterization of the major DNA adduct formed from the food mutagen ochratoxin A in the NarI hotspot sequence: influence of adduct ionization on the conformational preferences and implications for the NER propensity

Positional Impact of Fluorescently Modified G-Tetrads within Polymorphic Human Telomeric G-Quadruplex Structures

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