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• W2115941430 abstract "The C1′-oxidized abasic DNA lesion 2-deoxyribonolactone (dL, 1) has attracted significant attention in recent years owing to its potential mutagenicity, which is associated with the ability of lesion 1 to misincorporate nucleotides during DNA synthesis, its resistance to base-excision-repair (BER) enzymes, and its ability to form cross-links with BER enzymes efficiently.[1] Lesion 1 is produced in model systems by the action of a number of DNA-damaging agents such as copper(I)phenanthroline,[2] other metal complexes,[3] enediyne antibiotics,[4] as well as by UV light,[5] photosensitization,[6] and ionizing radiation.[7] However, the formation of 1 in vivo and its biological effects have been poorly documented. Until recently, lesion 1 in model systems has been identified primarily by detection of its low-molecular decomposition product 5-methylene-2-furanone (5-MF, 3).[2b,8] Only recently has a method for the selective detection of 1 been developed based on its reactivity with biotinylated cysteine.[9]Lesion 1 is relatively unstable; decomposition of 1, which is significantly accelerated by heating or alkaline treatment, results in strand scission and release of 3 (Scheme 1).[10–12] Decomposition of 1 is a two-step process: β elimination of the 3′-phosphate fragment forms butenolide 2, and δ elimination of the 5′-phosphate fragment produces 3 as the final product. The product 3 is unstable at basic pH values and hence cannot be detected upon alkaline decomposition of 1.Scheme 1Decomposition of 1.In our recent paper[8] we demonstrated that 3, a characteristic decomposition product of 1, is released from X-irradiated calf thymus DNA upon postirradiation treatment with DNA-phosphate-binding catalysts such as spermine. We hypothesized that 1 is a precursor to 3 in irradiated DNA and suggested that the yield of 1 in DNA can be quantified by using the yield of released 3.Herein we report the isolation of dL-containing tetramers from X-irradiated d(CGCG) and d(pCGCG) films, with the dL lesions corresponding to all four positions of the d-(C1G2C3G4) tetramer. We demonstrate that these dL-containing tetramers undergo catalytic decomposition with quantitative release of 3. These results provide proof that lesion 1 is the major, perhaps only, precursor to 3 in irradiated highly polymerized DNA.Figure 1 shows the HPLC profiles of d(CGCG), X-irradiated as a “dry” film and then dissolved in water for analysis. In the absence of heat, a group of products that do not contain strand breaks but presumably contain modified nucleotides were observed with a retention time of 16–23 min (Figure 1b). Furthermore, peaks are observed for the free bases C and G and for phosphate fragments produced as a result of immediate strand scission.Figure 1HPLC profiles of the solution of X-irradiated d(CGCG) film (ammonium acetate (40 mM), pH 6.8, spermine (10 mM)). a) 20 min at 90°C with spermine; b) no heat. Peaks for products 4–7 are shown with arrows. HPLC conditions: C18 μ-Bondapack ...Upon heating of the same solution in the presence of spermine (10 MM), a number of peaks corresponding to non-strand-break d(CGCG) lesions disappear. These changes are accompanied by the growth of peaks corresponding to products of strand scission, d(pGCG), d(CGCp), d(CGp), d(pCG), d(pG), and d(Cp), as well as free bases C and G (Figure 1a). This observation indicates that at least some of the non-strand-break products are latent lesions, which undergo catalytic decomposition to give strand scission. Also, the release of 3 was observed (Figure 1a), and is shown below to be a result of the decomposition of dL-containing products.Each of the four products 4–7 (see peaks in Figure 1b), have been identified as a tetramer containing dL located at one of the four numbered positions in d(C1G2C3G4) (see Scheme 2). These products were isolated as individual compounds by semipreparative HPLC and purified through several rounds of HPLC fractionation. MALDI-TOF analysis of the isolated compounds supports the assignments to dL structures 4–7. Similarly, a 5′-phosphorylated tetramer 8, which contains the terminal dL at position 1 of d(pC1G2C3G4) (see Scheme 2), was isolated from the X-irradiated d-(pCGCG) film and identified by using MALDI-TOF and decomposition patterns. Additional evidence is provided by the characteristic decomposition patterns of the dL-containing tetramers 4–8 (see Figures 2 and ​and33).Figure 2Thermal decomposition of 5, 6, and 8. Reaction mixtures contained 50 mM sodium acetate buffer, pH 5.2, 10 mM spermine (added before or after heating). A–C: RP HPLC; a) 20 min at 90°C with spermine; b) as a) but heated without spermine; ...Figure 3Thermal decomposition of 4 (A) and 7 (B). A) sodium acetate buffer (50 mM), pH 5.2, spermine (10 mM); a) 20 min at 90 °C with spermine; b) as a) but heated without spermine; c) no heat; HPLC conditions: as in Figure 2A–C. B) ammonium acetate ...Scheme 2Structures and decomposition patterns of dL-containing oligonucleotides isolated from X-irradiated d(CGCG) and d(pCGCGp) films.The patterns of the thermal decomposition of 4–8 are shown in Scheme 2. Thermal decomposition of 5, 6, and 8 under conditions analogous to those used for the release of 3 from X-irradiated highly polymerized DNA[8] is illustrated in Figure 2. It can be seen from Figure 2C that 8 and its product d(pGCG) have overlapping retention times in the reversed-phase (RP) HPLC chromatogram; therefore, ion-exchange chromatography was applied to resolve the peaks for 8 and d(pGCG) (Figure 2D).All dLs shown in Figure 2 (5, 6, and 8) are heat-resistant at pH 5.2 in the absence of a catalyst (see panels b of Figure 2A–C). Furthermore, 5, 6, and 8 readily decompose with release of 3 upon heating under the same conditions but with spermine (10 mM) added. Thus these dLs show decomposition patterns analogous to irradiated calf thymus DNA.[8] All dLs in Figure 2 undergo quantitative decomposition; 3 and its corresponding phosphate fragments are formed in nearly stoichiometric ratios (with the exception of d(Cp) for 5). These results show that the yield of 3, released upon catalytic treatment of dL-containing oligonucleotides, correlates well with the yield of its dL precursor.The 5′-terminal dL 4 undergoes about 80% conversion upon heating for 20 min at 90°C with spermine (10 MM) at pH 5.2 (Figure 3Aa), while its 3′-terminal analogue 7 is stable under these conditions (results not shown). Significant decomposition of 7 required more prolonged heating at pH 6.8 (30 min or more, Figure 3B,a. The optical absorption of the butenolides 9 and 10 (see Scheme 2) supposedly formed upon decomposition of 4 and 7 respectively, is apparently too weak at 254 nm to be detected under the conditions of this study.The total yield of dL was estimated for the X-irradiated films of d(pCGCGp) (Figure 4). All four types of dL formed from d(pCGCGp) release 3 upon thermal catalytic decomposition; the yield of 3 therefore, is assumed to correlate with the total yield of dL. This assumption is justified by the quantitative release of 3 upon decomposition of phosphorylated dL-containing tetramers and by the stability of 3 under the experimental conditions employed (at slightly acidic pH values).[8] The inset in Figure 4 shows the dose dependence for the formation of 3; the radiation yield of 3, 0.0103 ± 0.0004 μmolJ−1, was obtained from the slope of the linear fit to the experimental data. This yield is 3.4-fold lower than the yield of 3 obtained for the X-irradiated films of calf thymus DNA[8] subjected to analogous post-irradiation treatment. This degree of variation is not surprising given the large differences in the primary and tertiary structures of d-(pCGCGp) when compared with genomic DNA.Figure 4Release of 3 from the solution of the X-irradiated d-(pCGCGp) film. The reaction mixture containing ammonium acetate buffer (40 mM), pH 6.8, and spermine (10 mM) was heated 25 min at 90°C. The inset shows the dose dependence of the release of ...In conclusion, we have demonstrated that catalytic decomposition of dL isolated from X-irradiated d(CGCG) and d(pCGCG) films quantitatively produces 3. This finding supports our earlier hypothesis that 1 is the major, perhaps only, precursor of 3 released from X-irradiated highly polymerized DNA.[8] Our data suggest that quantification of the yield of 3 released upon catalytic decomposition of dL can be applied as a method for selective quantitative detection of lesion 1 in DNA." @default.
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• W2115941430 title "2-Deoxyribonolactone Lesions in X-ray-Irradiated DNA: Quantitative Determination by Catalytic 5-Methylene-2-furanone Release" @default.
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• W2115941430 doi "https://doi.org/10.1002/anie.200501956" @default.
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