Your search keyword '"DNA-Formamidopyrimidine Glycosylase pharmacology"' showing total 24 results

1. The enzyme-modified comet assay: Enzyme incubation step in 2 vs 12-gels/slide systems.

Author

Muruzabal D, Langie SAS, Pourrut B, and Azqueta A

Subjects

8-Hydroxy-2'-Deoxyguanosine analysis, Alkylating Agents toxicity, Cell Line, Comet Assay instrumentation, DNA Damage, Dose-Response Relationship, Drug, Electrophoresis, Agar Gel, Gels, Humans, Lymphocytes drug effects, Reproducibility of Results, Time Factors, Comet Assay methods, DNA-Formamidopyrimidine Glycosylase pharmacology, Titrimetry methods

Abstract

The enzyme-modified comet assay is a commonly used method to detect specific DNA lesions. However, still a lot of errors are made by many users, leading to dubious results and even misinterpretations. This technical note describes some critical points in the use of the enzyme-modified comet assay, such as the enzyme concentration, the time of incubation, the format used and the equipment. To illustrate the importance of these conditions/parameters, titration experiments of formamidopyrimidine DNA glycosylase (Fpg) were performed using the 2 gels/slide and the 12 minigels/slide formats (plus the 12-Gel Comet Assay Unit™). Incubation times of 15 and 30 min, and 1 h were used. Results showed that the 12 minigels/slide system requires a lower volume and concentration of Fpg. A longer time of incubation has a bigger impact when using such format. Moreover, the paper describes how to perform and interpret a titration experiment when using the enzyme-modified comet assay., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2019

2. Assessment of DNA damage in Polish children environmentally exposed to pesticides.

Author

Kapka-Skrzypczak L, Czajka M, Sawicki K, Matysiak-Kucharek M, Gabelova A, Sramkova M, Bartyzel-Lechforowicz H, and Kruszewski M

Subjects

Acetylcholinesterase blood, Biological Monitoring methods, Child, Cholinesterase Inhibitors toxicity, Comet Assay, DNA blood, DNA drug effects, DNA Breaks, DNA-Formamidopyrimidine Glycosylase pharmacology, Female, Food Contamination, Guanine analogs & derivatives, Guanine blood, Humans, Male, Micronucleus Tests, Parents, Poland, Rural Population, DNA Damage, Environmental Exposure, Pesticides toxicity

Abstract

Exposure to pesticides leads to complex, long-lasting adverse effects on human health, and poses a substantial risk to those living in areas devoted to agriculture. Children are particularly vulnerable to the pesticide exposure, due to the developmental, dietary and physiological factors. Small body mass and typical exploratory behavior result in increased risk of intoxication. Thus, even exposure to low concentrations of pesticides, if of sufficient duration, may lead to permanent health disorders and limit their harmonious development. In this study 108 children, living in areas of an intense pesticide use and a control group (n = 92) of children from an agrotouristic area were investigated, whether DNA damage increased due to prolonged pesticide exposure. A presence of DNA breaks and oxidative damage to DNA bases, characterized as Fpg-sensitive sites, were detected by comet assay. Micronuclei (MN) formation was evaluated by cytokinesis-block MN assay. The exposure of children to pesticides resulted in increased number of MN in peripheral blood lymphocytes (P = 0.016), increased DNA strand breaks level (P = 0.002) and oxidative damage to DNA (P < 0.001). Negative correlation was demonstrated between the level of DNA strand breaks and acetylcholinesterase (AChE) activity in exposed group. In conclusion, despite just environmental pesticide exposure in the test group of children, significant biological effects were detected., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2019

3. Technical recommendations to perform the alkaline standard and enzyme-modified comet assay in human biomonitoring studies.

Author

Azqueta A, Muruzabal D, Boutet-Robinet E, Milic M, Dusinska M, Brunborg G, Møller P, and Collins AR

Subjects

DNA blood, DNA drug effects, DNA Breaks, DNA-Formamidopyrimidine Glycosylase pharmacology, Electrophoresis, Agar Gel methods, Guanine analogs & derivatives, Guanine blood, Guidelines as Topic, Humans, Hydrogen-Ion Concentration, Laboratory Proficiency Testing, Oxidation-Reduction, Reference Standards, Reproducibility of Results, Sepharose, Staining and Labeling methods, Temperature, Time Factors, Biological Monitoring methods, Comet Assay methods, DNA Damage

Abstract

The comet assay (single cell gel electrophoresis) is widely used as a biomonitoring tool to assess DNA damage - strand breaks, as well as oxidised bases; it can also be adapted to measure DNA repair. It is based on the ability of breaks in the DNA to relax supercoiling, allowing DNA loops to extend from the nuclear core (nucleoid) under an electric field to form a comet-like tail. Most commonly, it is applied to white blood cells. The range of detection is between a few hundred breaks per cell and a few thousand, encompassing levels of damage that can be repaired and tolerated by human cells. Its applications include monitoring various diseases, studying the influence of nutrition on DNA stability, and investigating effects of environmental and occupational mutagens. Here we address the issue of inter-laboratory variation in comet assay results. This variation is largely due to differences in methods. Imposing a standard protocol is not practical, but users should be aware of the crucial parameters that affect performance of the assay. These include the concentration of agarose in which the cells are embedded; the duration of cell lysis, and of enzyme incubation when oxidised bases are being measured; the duration of alkaline unwinding; the duration of electrophoresis and the voltage gradient applied; and the method used to score the comets. Including reference standards in each experiment allows experimental variability to be monitored - and if variation is not extreme, results can be normalised using reference standard values. Reference standards are also essential for inter-laboratory comparison. Finally, we offer recommendations which, we believe, will limit variability and increase the usefulness of this assay in molecular epidemiology., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

4. Fish and salad consumption are inversely associated with levels of oxidatively damaged DNA in a Danish adult cohort.

Author

Møller P, Jensen A, Løhr M, Eriksen L, Grønbæk M, and Loft S

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Animals, Comet Assay, Cross-Sectional Studies, DNA blood, DNA Breaks, DNA Repair, DNA-Formamidopyrimidine Glycosylase pharmacology, Denmark, Edible Grain, Female, Fruit, Guanine analogs & derivatives, Guanine blood, Humans, Leukocytes, Mononuclear chemistry, Male, Middle Aged, Oxidation-Reduction, Oxidative Stress, Vegetables, Young Adult, DNA Damage, Feeding Behavior, Fishes, Salads

Abstract

This study investigated associations between levels of oxidatively damaged DNA, measured by the formamidopyrimidine DNA glycosylase (Fpg)-modified comet assay and intake of fish, salad, fruits, vegetables, wholegrain items, and potatoes in a cross-sectional study of 382 men and 591 women between 18 and 93 years. Intake of dietary items was obtained from questionnaires, and stratified into less than once per week, weekly or daily consumption. Intake of fish as main course was inversely associated with levels of Fpg-sensitive sites in peripheral blood mononuclear cells (PBMCs) in especially women (P < 0.001 multivariate linear regression). Intake of fish was also inversely associated with lower levels of Fpg-sensitive sites in men (P < 0.05, univariate analysis), although it was not statistically significant in analysis adjusted for lifestyle and other dietary factors. Intake of salad was inversely associated with levels of Fpg-sensitive sites in men (P < 0.001, multivariate linear regression). Statistically significant associations were also observed for intake of vegetables and potatoes in men, although these were weak and not robust in all statistical models. The sum the six individual dietary items was inversely associated with levels of Fpg-sensitive sites in the strata of men (P < 0.001, multivariate linear regression). Finally, levels of DNA repair incision activity were not associated with individual food categories or the total dietary food score. In summary, consumption of health-promoting foods is associated with lower levels of Fpg-sensitive sites in human PBMCs and strongest effects in the present population were ingestions of fish and salad., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2019

5. Isolation of leukocytes from frozen buffy coat for comet assay analysis of DNA damage.

Author

Bøhn SK, Vebraite V, Shaposhnikov S, and Collins AR

Subjects

Adult, Centrifugation, Density Gradient, DNA blood, DNA drug effects, DNA Breaks, DNA-Formamidopyrimidine Glycosylase pharmacology, Female, Guanine analogs & derivatives, Guanine blood, Humans, Hydrogen Peroxide pharmacology, Leukocytes drug effects, Leukocytes, Mononuclear chemistry, Middle Aged, Blood Buffy Coat cytology, Blood Preservation, Cell Separation methods, Comet Assay methods, Cryopreservation, DNA Damage, Leukocytes chemistry

Abstract

Frozen buffy coat fractions are often stored in human biomonitoring trials but their use for biomarker purposes has been limited. The purpose of the current study was to study whether frozen buffy coats can be used to monitor DNA damage levels. EDTA blood samples were provided from 9 healthy, non-smoking female volunteers, aged 26-48. Pre-existing DNA damage (strand breaks and oxidised purines) was measured with the comet assay in thawed resuspended buffy coat samples and washed leukocytes from these buffy coats, as well as resistance to DNA damage induced exogenously by H 2 O 2 in the latter, and compared with damage measured in peripheral blood mononuclear cells isolated from fresh blood using percoll gradient centrifugation. Basal DNA damage levels (strand breaks) were significantly higher in the leukocytes isolated from frozen buffy coats in the untreated samples compared with peripheral blood mononuclear cells. However, the levels of strand breaks were still low (<4% tail DNA), indicating that little damage is caused by freezing or processing. Base oxidation was significantly higher in isolated buffy coat leukocytes than in peripheral blood mononuclear cells from fresh blood, but showed a good correlation (r = 0.67) between the two cell types. The correlation for strand breaks was stronger (r = 0.85). H 2 O 2 induced DNA breaks in the cells both from fresh blood and buffy coats. The results indicate that buffy coat samples stored from cohort studies might be usefully analysed for DNA damage in retrospective epidemiological investigations. However, caution should be exercised when comparing the absolute levels of DNA damage in buffy coat leukocytes and peripheral blood mononuclear cells., (Copyright © 2019. Published by Elsevier B.V.)

Published

2019

6. DNA damage in blood cells exposed to low-level lasers.

Author

Sergio LP, Silva AP, Amorim PF, Campos VM, Magalhães LA, de Paoli F, and de Souza da Fonseca A

Subjects

Animals, Comet Assay, DNA-Formamidopyrimidine Glycosylase pharmacology, Endodeoxyribonucleases pharmacology, Rats, Wistar, Blood Cells radiation effects, DNA Damage radiation effects, Lasers

Abstract

Background and Objective: In regenerative medicine, there are increasing applications of low-level lasers in therapeutic protocols for treatment of diseases in soft and in bone tissues. However, there are doubts about effects on DNA, and an adequate dosimetry could improve the safety of clinical applications of these lasers. This work aimed to evaluate DNA damage in peripheral blood cells of Wistar rats induced by low-level red and infrared lasers at different fluences, powers, and emission modes according to therapeutic protocols., Material and Methods: Peripheral blood samples were exposed to lasers and DNA damage was accessed by comet assay. In other experiments, DNA damage was accessed in blood cells by modified comet assay using formamidopyrimidine DNA glycosylase (Fpg) and endonuclease III enzymes., Results: Data show that exposure to low-level red and infrared lasers induce DNA damage depending on fluence, power and emission mode, which are targeted by Fpg and endonuclease III., Conclusion: Oxidative DNA damage should be considered for therapeutic efficacy and patient safety in clinical applications based on low-level red and infrared lasers., (© 2015 Wiley Periodicals, Inc.)

Published

2015

7. Evaluation of basal DNA damage and oxidative stress in Wistar rat leukocytes after exposure to microwave radiation.

Author

Garaj-Vrhovac V, Gajski G, Trosić I, and Pavicić I

Subjects

Animals, Comet Assay methods, DNA blood, DNA-Formamidopyrimidine Glycosylase pharmacology, Leukocytes, Mononuclear metabolism, Male, Rats, Rats, Wistar, DNA radiation effects, DNA Damage, Leukocytes, Mononuclear radiation effects, Microwaves adverse effects, Oxidative Stress

Abstract

The aim of this study was to assess whether microwave-induced DNA damage is basal or it is also generated through reactive oxygen species (ROS) formation. After having irradiated Wistar rats with 915MHz microwave radiation, we assessed different DNA alterations in peripheral leukocytes using standard and formamidopyrimidine DNA-glycosylase (Fpg)-modified comet assay. The first is a sensitive tool for detecting primary DNA damage, and the second is much more specific for detecting oxidative damage. The animals were irradiated for 1h a day for 2 weeks at a field power density of 2.4W/m(2), and the whole-body average specific absorption rate (SAR) of 0.6W/kg. Both the standard and the Fpg-modified comet assay detected increased DNA damage in blood leukocytes of the exposed rats. The significant increase in Fpg-detected DNA damage in the exposed rats suggests that oxidative stress is likely to be responsible. DNA damage detected by the standard comet assay indicates that some other mechanisms may also be involved. In addition, both methods served proved sensitive enough to measure basal and oxidative DNA damage after long-term exposure to 915MHz microwave radiation in vivo.

Published

2009

8. Humic acid induced genotoxicity in human peripheral blood lymphocytes using comet and sister chromatid exchange assay.

Author

Hseu YC, Chen SC, Chen YL, Chen JY, Lee ML, Lu FJ, Wu FY, Lai JS, and Yang HL

Subjects

Catalase pharmacology, Cells, Cultured, Chelating Agents pharmacology, Chromans pharmacology, Comet Assay, DNA-Formamidopyrimidine Glycosylase pharmacology, Deoxyribonuclease (Pyrimidine Dimer) pharmacology, Egtazic Acid pharmacology, Escherichia coli Proteins pharmacology, Humans, Lymphocytes drug effects, NG-Nitroarginine Methyl Ester pharmacology, Phenanthrolines pharmacology, Sister Chromatid Exchange, Superoxide Dismutase pharmacology, omega-N-Methylarginine pharmacology, DNA Damage drug effects, Humic Substances toxicity, Water Pollutants toxicity

Abstract

Humic acid (HA) in well water used by the inhabitants for drinking is one of the possible etiological factors for blackfoot disease (BFD). Moreover, within BFD endemic areas cancers occur at significantly higher rates than in areas free of BFD. In this study, the genotoxic potential of HA is assessed using human peripheral blood lymphocytes. The cells were exposed to HA (0-200 microg/mL for 2 h), and the induction of DNA primary damage in cellular DNA was evaluated by single-cell gel electrophoresis (comet assay). HA-induced DNA damage was decreased by superoxide (O(2)(-)), hydrogen peroxide (H(2)O(2)), and reactive oxygen species (ROS) scavengers (superoxide dismutase, catalase, and Trolox), and nitric oxide (NO) synthase inhibitors (N(G)-nitro-l-arginine methyl ester and N(G)-methyl-l-arginine). Moreover, formamidopyrimidine-DNA glycosylase (Fpg) and endonuclease III (Endo III), known to catalyze the excision of oxidized bases, increase the amount of DNA migration in HA-treated cells. Pretreatment of the cells with both the Ca(2+)-chelator BAPTA and EGTA completely inhibited HA-induced DNA damage, indicating that HA-induced changes in Ca(2+)-homeostasis are the predominant pathways for the HA induction of genotoxicity. Furthermore, sister chromatid exchange was found in the HA-treated lymphocytes. Our findings suggest that HA can induce oxidative DNA damage and genotoxicity in human lymphocytes.

Published

2008

9. Photosensitized DNA damage induced by NADH: site specificity and mechanism.

Author

Ito K, Hiraku Y, and Kawanishi S

Subjects

8-Hydroxy-2'-Deoxyguanosine, Animals, Cattle, DNA Damage, DNA Fragmentation, DNA-Formamidopyrimidine Glycosylase pharmacology, Deoxyguanosine analogs & derivatives, Deoxyguanosine pharmacology, Genes, p53, Humans, Hydrogen Peroxide pharmacology, Riboflavin pharmacology, Tumor Suppressor Protein p53 metabolism, Ultraviolet Rays, Light, NAD chemistry, Photosensitizing Agents pharmacology

Abstract

Increasing evidence reveals the carcinogenicity of UVA radiation. We demonstrated that UVA-irradiated NADH induced damage to (32)P-labeled DNA fragments obtained from the p53 gene in the presence of Cu(II). Formamidopyrimidine glycosylase (Fpg)-sensitive lesions were formed at guanine residues, whereas piperidine-labile lesions occurred frequently at thymine residues. Formation of 8-oxo-7,8-dihydro-2'-deoxyguanosine (8-oxodG), upon UVA exposure in the presence of Cu(II), increased depending on NADH concentration. Catalase and bathocuproine, a Cu(I)-specific chelator, inhibited the DNA damage, suggesting the involvement of reactive species derived from H(2)O(2) and Cu(I). UVA-irradiated riboflavin induced DNA cleavage through electron transfer at 5' guanine of the 5'-GG-3' sequence with both Fpg and piperidine treatments; Fpg induced less cleavage at the guanine residues than piperidine. These results imply that NADH may participate as an endogenous photosensitizer in UVA carcinogenesis via H(2)O(2) generation, producing metal-mediated mutagenic lesions such as 8-oxodG.

Published

2007

10. Repeated inhalations of diesel exhaust particles and oxidatively damaged DNA in young oxoguanine DNA glycosylase (OGG1) deficient mice.

Author

Risom L, Dybdahl M, Møller P, Wallin H, Haug T, Vogel U, Klungland A, and Loft S

Subjects

8-Hydroxy-2'-Deoxyguanosine, Administration, Inhalation, Age Factors, Animals, Body Weight drug effects, Bronchoalveolar Lavage Fluid cytology, DNA Glycosylases biosynthesis, DNA Glycosylases genetics, DNA Glycosylases physiology, DNA Repair drug effects, DNA-Binding Proteins biosynthesis, DNA-Binding Proteins genetics, DNA-Formamidopyrimidine Glycosylase pharmacology, Deoxyguanosine analogs & derivatives, Deoxyguanosine analysis, Endonucleases biosynthesis, Endonucleases genetics, Escherichia coli Proteins pharmacology, Female, Heme Oxygenase-1 biosynthesis, Heme Oxygenase-1 genetics, Interleukin-6 biosynthesis, Interleukin-6 genetics, Liver chemistry, Liver drug effects, Lung chemistry, Lung drug effects, Lung radiation effects, Macrophages, Alveolar drug effects, Membrane Proteins biosynthesis, Membrane Proteins genetics, Mice, Mice, Inbred C57BL, Mice, Knockout, Neutrophils drug effects, Oxidative Stress, Pyrrolidines pharmacology, Quinolizines pharmacology, RNA, Messenger biosynthesis, DNA Damage, DNA Glycosylases deficiency, Vehicle Emissions toxicity

Abstract

DNA repair may prevent increased levels of oxidatively damaged DNA from prolonged oxidative stress induced by, e.g. exposure to diesel exhaust particles (DEP). We studied oxidative damage to DNA in broncho-alveolar lavage cells, lungs, and liver after 4 x 1.5 h inhalations of DEP (20 mg/m3) in Ogg1-/- and wild type (WT) mice with similar extent of inflammation. DEP exposure increased lung levels of 8-oxo-7,8-dihydro-2'-deoxyguanosine (8-oxodG) in Ogg1-/- mice, whereas no effect on 8-oxodG or oxidized purines in terms of formamidopyrimidine DNA glycosylase (FPG) sites was observed in WT mice. In both unexposed and exposed Ogg1-/- mice the level of FPG sites in the lungs was 3-fold higher than in WT mice. The high basal level of FPG sites in Ogg1-/- mice probably saturated the assay and prevented detection of DEP-generated damage. In conclusion, Ogg1-/- mice have elevated pulmonary levels of FPG sites and accumulate genomic 8-oxodG after repeated inhalations of DEP.

Published

2007

11. DNA damage and repair capacity by comet assay in lymphocytes of white-collar active smokers and passive smokers (non- and ex-smokers) at workplace.

Author

Fracasso ME, Doria D, Franceschetti P, Perbellini L, and Romeo L

Subjects

Adult, Biomarkers urine, Comet Assay, Cotinine urine, DNA Repair, DNA-Formamidopyrimidine Glycosylase pharmacology, Female, Glutathione metabolism, Humans, Hydrogen Peroxide toxicity, Lymphocytes drug effects, Male, Nicotine urine, Smoking metabolism, Workplace, Air Pollutants, Occupational adverse effects, DNA Damage, Occupational Exposure adverse effects, Smoking adverse effects, Tobacco Smoke Pollution adverse effects

Abstract

The comet assay has been widely used to quantify DNA damage in isolated lymphocytes from subjects exposed to several environmental or occupational substances, especially for estimation of oxidative damage in the DNA, which is well-known to be induced by tobacco smoke. Passive smoking or environmental tobacco smoke (ETS) has been included among those substances that cause cancer with sufficient evidence in humans. In this study, we analyzed, by the alkaline version of comet assay, the lymphocyte DNA damage of white-collar active smokers and non- and ex-smokers exposed to ETS at the workplace. We investigated basal DNA damage, DNA oxidation by formamidopyrimidine glycosylase (Fpg), the repair capacity H2O2-induced DNA damage by kinetics studies and lymphocyte GSH levels, the major intracellular defense against exogenous oxidative stress imposed by cigarette smoking. Our results indicated high basal DNA damage with clear significant correlations with urinary nicotine and cotinine, number of cigarettes/day, and an inverse significant correlation with GSH cellular content in active smokers. Significant Fpg-sensitive sites were found in smokers (> 85%), considerably high but not significant in passive non- and ex-smokers (> 51% and 37%, respectively). The DNA repair capacity had seriously decreased in non-smokers > smokers > ex-smokers, while the same damage was repaired in a short time in never smokers.

Published

2006

12. Cationic peptides containing tyrosine protect against radiation-induced oxidative DNA damage.

Author

Ly A, Bullick S, Won JH, and Milligan JR

Subjects

Binding Sites, DNA Damage radiation effects, DNA Repair radiation effects, DNA-Formamidopyrimidine Glycosylase pharmacology, Dose-Response Relationship, Drug, Gamma Rays, Ligands, Phenylalanine chemistry, Phenylalanine pharmacology, Reactive Oxygen Species metabolism, Reactive Oxygen Species radiation effects, Thiocyanates pharmacology, Time Factors, Tryptophan chemistry, Tryptophan pharmacology, Tyrosine chemistry, Antimicrobial Cationic Peptides pharmacology, DNA Damage drug effects, DNA Repair drug effects, Radiation-Protective Agents pharmacology, Tyrosine pharmacology

Abstract

Purpose: To examine the effect of the amino acid tyrosine on oxidatively or direct-type damaged DNA damage when it is present in a DNA binding ligand., Materials and Methods: We made use of tetralysine ligands to ensure binding to DNA and to condense the DNA, and simulated direct-type damage by using gamma irradiation in the presence of thiocyanate ions. These ligands contained an additional C terminal amino acid. Phenylalanine was used as a control for tyrosine. These ligands were used in conjuction with a plasmid substrate to quantify strand break yields. Base damage yields were estimated by measuring the strand break yield after incubation of the plasmid with the bacterial base excision repair enzyme formamidopyrimidine-DNA N-glycosylase (FPG)., Results: When the condensing ligand contains an additional tyrosine or tryptophan residue, the plasmid is protected against the effects of a single electron oxidation, as assayed by sensitivity to a base excision repair enzyme. This protection is significantly greater in condensed plasmid where the amino acid residues are in close proximity to the DNA, and can be observed even when only a small fraction of the ligand contains tyrosine., Conclusions: Bound tyrosine residues located in close proximity to DNA are capable of reversing oxidative DNA damage far more efficiently than when present unbound in the bulk solution. This suggests that tyrosine residues in DNA binding proteins may participate in the repair of DNA that has been oxidatively damaged by ionizing radiation.

Published

2006

13. Genotoxic effects of myosmine in a human esophageal adenocarcinoma cell line.

Author

Vogt S, Fuchs K, and Richter E

Subjects

Adenocarcinoma, Cell Line, Tumor, Comet Assay, DNA-Formamidopyrimidine Glycosylase pharmacology, Esophageal Neoplasms, Humans, Alkaloids toxicity, DNA Damage

Abstract

The incidence of esophageal adenocarcinoma is rapidly rising in Western populations. Gastroesophageal reflux disease (GERD) is thought to be one of the most important risk factors. However, the mechanisms by which GERD enhances tumor formation at the gastroesophageal junction are not well understood. Myosmine is a tobacco alkaloid which has also a wide spread occurrence in human diet. It is readily activated by nitrosation and peroxidation giving rise to the same hydroxypyridylbutanone-releasing DNA adducts as the esophageal carcinogen N'-nitrosonornicotine. Therefore, the genotoxicity of myosmine was tested in a human esophageal adenocarcinoma cell line (OE33). DNA damage was assessed by single-cell gel electrophoresis (Comet assay). DNA strand breaks, alkali labile sites and incomplete excision repair were expressed using the Olive tail moment (OTM). The Fapy glycosylase (Fpg) enzyme was incorporated into the assay to reveal additional oxidative DNA damage. DNA migration was determined after incubation of the cells for 1-24h. Under neutral conditions high myosmine concentrations of 25-50mM were necessary to elicit a weak genotoxic effect. At pH 6 genotoxicity was clearly enhanced giving a significant increase of OTM values at 5mM myosmine. Lower pH values could not be tested because of massive cytotoxicity even in the absence of myosmine. Co-incubation of 25 mM myosmine with 1mM H(2)O(2) for 1h significantly enhanced the genotoxicity of H(2)O(2) but not the oxidative lesions additionally detected with the Fpg enzyme. In the presence of the peroxynitrite donor 3-morpholinosydnonimine (SIN-1) a dose-dependent significant genotoxic effect was obtained with 1-10mM myosmine after 4h incubation. NS-398, a selective inhibitor of cyclooxygenase 2, did not affect the SIN-1 stimulated genotoxicity of myosmine. Finally, the 23 h repair of N-methyl-N'-nitro-N-nitrosoguanidine-induced DNA lesions was significantly inhibited in the presence of 10mM myosmine. In conclusion, myosmine exerts significant genotoxic effects in esophageal cells under conditions which may prevail in GERD such as increased oxidative and nitrosative stress resulting from chronic inflammation.

Published

2006

14. Guanine-specific DNA damage photosensitized by the dihydroxo(tetraphenylporphyrinato)antimony(V) complex.

Author

Hirakawa K, Kawanishi S, Matsumoto J, Shiragami T, and Yasuda M

Subjects

8-Hydroxy-2'-Deoxyguanosine, DNA-Formamidopyrimidine Glycosylase pharmacology, Deoxyguanosine analogs & derivatives, Deoxyguanosine metabolism, Electron Transport drug effects, Escherichia coli Proteins pharmacology, Guanine analogs & derivatives, Light, Membrane Lipids metabolism, Oxidation-Reduction, Phospholipids metabolism, Piperidines pharmacology, Proteins metabolism, Singlet Oxygen metabolism, DNA metabolism, DNA Damage drug effects, DNA, Single-Stranded metabolism, Guanine metabolism, Metalloporphyrins pharmacology, Photosensitizing Agents pharmacology

Abstract

The dihydroxo(tetraphenylporphyrinato)antimony(V) complex (SbTPP) demonstrates bactericidal activity under visible-light irradiation. This phototoxic effect could be caused by photodamage to biomolecules, but the mechanism has not been well understood. In this study, to clarify the mechanism of phototoxicity by SbTPP, DNA damage photosensitized by SbTPP was examined using [(32)P]-5'-end-labeled DNA fragments. SbTPP induced markedly severe photodamage to single-stranded rather than to double-stranded DNA. Photo-irradiated SbTPP frequently caused DNA cleavage at the guanine residue of single-stranded DNA after Escherichia coli formamidopyrimidine-DNA glycosylase or piperidine treatment. HPLC measurement confirmed the formation of 8-oxo-7,8-dihydro-2'-deoxyguanosine (8-oxodG), an oxidation product of 2'-deoxyguanosine, and showed that the content of 8-oxodG in single-stranded DNA is larger than that in double-stranded DNA. The effects of scavengers of reactive oxygen species on DNA damage suggested the involvement of singlet oxygen. These results have shown that the mechanism via singlet oxygen formation mainly contributes to the phototoxicity of SbTPP. On the other hand, SbTPP induced DNA damage specifically at the underlined G of 5'-GG, 5'-GGG, and 5'-GGGG in double-stranded DNA. The sequence-specificity of DNA damage is quite similar to that induced by the type I photosensitizers, suggesting that photo-induced electron transfer slightly participates in the phototoxicity of SbTPP. In conclusion, SbTPP induces DNA photodamage via singlet oxygen formation and photo-induced electron transfer. A similar mechanism can damage other biomacromolecules, such as protein and the phospholipid membrane. The damage to biomacromolecules via these mechanisms may participate in the phototoxicity of SbTPP.

Published

2006

15. Uranyl acetate induces hprt mutations and uranium-DNA adducts in Chinese hamster ovary EM9 cells.

Author

Stearns DM, Yazzie M, Bradley AS, Coryell VH, Shelley JT, Ashby A, Asplund CS, and Lantz RC

Subjects

Animals, CHO Cells, Cell Survival drug effects, Comet Assay, Cricetinae, Cricetulus, DNA Adducts genetics, DNA Damage drug effects, DNA-Formamidopyrimidine Glycosylase pharmacology, Dose-Response Relationship, Drug, Female, Hydrogen Peroxide pharmacology, Mutation genetics, Ribonuclease, Pancreatic pharmacology, Thioguanine pharmacology, Uranium, DNA Adducts drug effects, Hypoxanthine Phosphoribosyltransferase genetics, Mutagenesis drug effects, Mutation drug effects, Organometallic Compounds pharmacology

Abstract

Questions about possible adverse health effects from exposures to uranium have arisen as a result of uranium mining, residual mine tailings and use of depleted uranium in the military. The purpose of the current study was to measure the toxicity of depleted uranium as uranyl acetate (UA) in mammalian cells. The activity of UA in the parental CHO AA8 line was compared with that in the XRCC1-deficient CHO EM9 line. Cytotoxicity was measured by clonogenic survival. A dose of 200 microM UA over 24 h produced 3.1-fold greater cell death in the CHO EM9 than the CHO AA8 line, and a dose of 300 microM was 1.7-fold more cytotoxic. Mutagenicity at the hypoxanthine (guanine) phosphoribosyltransferase (hprt) locus was measured by selection with 6-thioguanine. A dose of 200 microM UA produced approximately 5-fold higher averaged induced mutant frequency in the CHO EM9 line relative to the CHO AA8 line. The generation of DNA strand breaks was measured by the alkaline comet assay at 40 min and 24 h exposures. DNA strand breaks were detected in both lines; however a dose response may have been masked by U-DNA adducts or crosslinks. Uranium-DNA adducts were measured by inductively coupled plasma optical emission spectroscopy (ICP-OES) at 24 and 48 h exposures. A maximum adduct level of 8 U atoms/10(3) DNA-P for the 300 microM dose was found in the EM9 line after 48 h. This is the first report of the formation of uranium-DNA adducts and mutations in mammalian cells after direct exposure to a depleted uranium compound. Data suggest that uranium could be chemically genotoxic and mutagenic through the formation of strand breaks and covalent U-DNA adducts. Thus the health risks for uranium exposure could go beyond those for radiation exposure.

Published

2005

16. Ochratoxin A: induction of (oxidative) DNA damage, cytotoxicity and apoptosis in mammalian cell lines and primary cells.

Author

Kamp HG, Eisenbrand G, Schlatter J, Würth K, and Janzowski C

Subjects

Animals, Carcinogens toxicity, Cell Line, Cell Proliferation drug effects, Chlorocebus aethiops, Comet Assay, Cricetinae, Cricetulus, DNA-Formamidopyrimidine Glycosylase pharmacology, Endonucleases pharmacology, Fibroblasts drug effects, Glutathione metabolism, Kidney cytology, Kidney metabolism, Lung cytology, Lung drug effects, Male, Oxidative Stress drug effects, Rats, Rats, Wistar, Apoptosis drug effects, DNA drug effects, DNA Damage, Kidney drug effects, Ochratoxins toxicity

Abstract

Ochratoxin A (OTA) is a nephrotoxic/-carcinogenic mycotoxin, produced by several Aspergillus- and Penicillium-strains. Humans are exposed to OTA via food contamination, a causal relationship of OTA to human endemic Balkan nephropathy is still under debate. Since DNA-adducts of OTA or its metabolites could not be identified unambiguously, its carcinogenic effectiveness might be related to secondary effects, such as oxidative cell damage or cell proliferation. In this study, OTA mediated induction of (oxidative) DNA damage, cytotoxicity (necrosis, growth inhibition, apoptosis) and modulation of glutathione were investigated in cell lines (V79, CV-1) and primary rat kidney cells. After 24 h incubation, viability of V79 cells was strongly decreased by OTA concentrations >2.5 micromol/L, whereas CV-1 cells were clearly less sensitive. Strong growth inhibition occurred in both cell lines (IC(50) approximately 2 micromol/L). Apoptosis, detected with an immunochemical test and with flow cytometry, was induced by >1 micromol/L OTA. Oxidative DNA damage, detected by comet assay after additional treatment with repair enzymes, was induced in all cell systems already at five-fold lower concentrations. Glutathione in CV-1 cells was depleted after 1 h incubation (>100 micromol/L). In contrast, an increase was measured after 24 h incubation (>0.5 micromol/L). In conclusion, OTA induces oxidative DNA damage at low, not yet cytotoxic concentrations. Oxidative DNA damage might initiate cell transformation eventually in connection with proliferative response following cytotoxic cell death. Both events might represent pivotal factors in the chain of cellular events leading into nephro-carcinogenicity of OTA.

Published

2005

17. Genotoxicity of acrylamide in human lymphocytes.

Author

Blasiak J, Gloc E, Wozniak K, and Czechowska A

Subjects

Adult, Apoptosis drug effects, Apoptosis physiology, Ascorbic Acid pharmacology, Caspase 3, Caspases metabolism, Cell Survival drug effects, Cell Survival physiology, Comet Assay, Cyclic N-Oxides, DNA Glycosylases pharmacology, DNA Repair genetics, DNA-Formamidopyrimidine Glycosylase pharmacology, Electrophoresis, Gel, Pulsed-Field, Humans, Lymphocytes cytology, Lymphocytes metabolism, Male, Nitrogen Oxides pharmacology, Spin Trapping, Thymine DNA Glycosylase pharmacology, Vitamin E pharmacology, Acrylamide toxicity, DNA Damage, DNA Repair drug effects, Lymphocytes drug effects, Mutagens toxicity

Abstract

Acrylamide is used in the industry and can be a by-product in a high-temperature food processing. It is reported to interact with DNA, but the mechanism of this interaction is not fully understood. In the present study, we investigated the DNA-damaging potential of acrylamide (ACM) in normal human lymphocytes using the alkaline-, neutral- and 12.1 versions of the comet assay and pulsed-field gel electrophoresis. We also investigated effect of acrylamide on caspase-3 activity as well as its influence on the repair process of hydrogen peroxide-induced DNA damage. Acrylamide at 0.5-50 microM induced mainly alkali-labile sites. This damage was repaired during a 60-min repair incubation. Post-treatment of the damaged DNA with repair enzymes: thymine glycol DNA N-glycosylase (Nth) and formamidopyrimidine-DNA glycosylase (Fpg), recognizing oxidized DNA bases, as well as 3-methyladenine-DNA glycosylase II (Alk A), recognizing alkylated bases, caused an increase in the extent of DNA damage, indicating the induction of oxidative and alkylative DNA base modifications by acrylamide. Pre-treatment of the lymphocytes with N-tert-butyl-alpha-phenylnitrone (PBN), a spin trap, as well as vitamins C and E decreased the DNA-damaging effect of acrylamide, which suggest that free radicals/reactive oxygen species may be involved in this effect. Acrylamide impaired the repair of DNA damaged by hydrogen peroxide and increased the activity of caspase-3, which may indicate its potential to induce apoptosis. Our results suggest that acrylamide may exert a wide spectrum of diverse effects on DNA of normal cells, including mostly DNA base modifications and apoptosis. Acrylamide may also impair DNA repair. Free radicals may underline these effects and some dietary antioxidants can be considered as protective agents against genotoxic action of acrylamide. As normal lymphocytes contain cyp2e1 and P450, engaged in the bioactivation of ACM to glicidamide it is uncertain whether acrylamide causes all of measured effect per se or this is the result of the action of its metabolites.

Published

2004

18. Analysis of 8-hydroxyguanine (8-OH-Gua) released from DNA by the formamidopyrimidine DNA glycosylase (Fpg) protein: a reliable method to estimate cellular oxidative stress.

Author

Orimo H, Mei N, Boiteux S, Tokura Y, and Kasai H

Subjects

Cell Line, Cells drug effects, Chromatography, High Pressure Liquid, DNA metabolism, Electrochemistry, Humans, Keratinocytes metabolism, Lung Neoplasms metabolism, Cells metabolism, Cells radiation effects, DNA drug effects, DNA Damage, DNA-Formamidopyrimidine Glycosylase pharmacology, Guanine analogs & derivatives, Guanine metabolism, Oxidative Stress

Abstract

To improve the analyses of a form of oxidative DNA damage, 8-hydroxyguanine (8-OH-Gua), we treated isolated DNA with formamidopyrimidine DNA glycosylase (Fpg) and analyzed the released 8-OH-Gua by using a high-performance liquid chromatography system equipped with an electrochemical detector (HPLC-ECD). The human lung carcinoma cells (A549) and human keratinocyte (HaCaT) were irradiated with gamma-rays. After the isolated DNA was treated with the Fpg protein, we analyzed the released 8-OH-Gua by using an HPLC-ECD. With this method, the background level of 8-OH-Gua in DNA from human lung carcinoma cells was determined to be 3.4 residues per 10(7) guanine (Gua). A similar background level of 8-OH-Gua (3.1 residues per 10(7) Gua) was also detected in human keratinocyte DNA with this method. These background 8-OH-Gua levels in cellular DNA are comparable to that obtained previously by an analysis of 8-OH-dGMP after nuclease P1 digestion of cellular DNA (4.3 residues per 10(7) dCMP). A dose-dependent increase of 8-OH-Gua (0.17/10(7) Gua/Gy) was observed after cells were irradiated with gamma-rays. Twenty hours after gamma-irradiation with 60 Gy, 75% of the 8-OH-Gua produced in keratinocyte DNA was repaired. With our new analysis method, it is possible to detect the small changes in the 8-OH-Gua levels in cellular DNA induced by various environmental factors.

Published

2004

19. Cell-specific oxidative DNA damage induced by estrogen in rat testicular cells in vitro.

Author

Wellejus A, Bornholdt J, Vogel UB, Risom L, Wiger R, and Loft S

Subjects

Animals, Cells, Cultured, Comet Assay, DNA Glycosylases genetics, DNA-Formamidopyrimidine Glycosylase pharmacology, Male, RNA, Messenger genetics, RNA, Ribosomal, 18S genetics, Rats, Rats, Wistar, Reverse Transcriptase Polymerase Chain Reaction, Testis cytology, Testis metabolism, DNA Damage, Ethinyl Estradiol toxicity, Oxidative Stress drug effects, Ploidies, Testis drug effects

Abstract

17 alpha-Ethinylestradiol (EE) can induce oxidative DNA damage in terms of 8-oxo-7,8-dihydro-2'-deoxyguanosine (8-oxodG) in rat testicular cells by an apparent estrogen receptor-mediated mechanism. We investigated differential susceptibility to EE in cell sub-populations from rat testes and the role of rat 8-oxo-guanine DNA glycosylase (rOGG1). Isolated rat testicular cells were incubated with EE concentrations ranging from 0.1 to 1000 nM. Single strand DNA breaks and oxidised purines as fapyguanine glycosylase (FPG) sensitive sites were assessed by the comet assay. In the total cell population and in round haploid cells, oxidised purines showed a bell-shaped concentration-response relationship with a maximally increased levels at 10 nM EE, whereas, no significant effects were seen in diploid, S-phase or tetraploid cells. The mRNA level of rOGG1 in testes cells was unaffected by EE, whereas, baseline levels were higher than in liver tissue and similar to colon tissue.

Published

2004

20. Sensitivity of the FPG protein towards alkylation damage in the comet assay.

Author

Speit G, Schütz P, Bonzheim I, Trenz K, and Hoffmann H

Subjects

Alkylation, Animals, Cells, Cultured, Cricetinae, Humans, Hydrogen-Ion Concentration, Oxidation-Reduction, Sensitivity and Specificity, Comet Assay methods, DNA Damage, DNA-Formamidopyrimidine Glycosylase pharmacology

Abstract

The comet assay (single cell gel electrophoresis) is widely used for the evaluation of DNA-damaging effects in genotoxicity testing and population monitoring. In its standard version at pH >13, DNA double strand breaks (DSB), DNA single strand breaks (SSB) and alkali-labile sites (ALS) lead to increased DNA migration. At reduced pH (12.5-12.1) the expression of ALS as SSB can be eliminated and the effect of SSB only can be identified. Specific endonucleases have been used to characterize specific classes of DNA damage. The formamido pyrimidine glycosylase (FPG) protein has been used to assess oxidative DNA base damage because it detects 8-OH guanine and other oxidatively damaged purines. Here, we show that the FPG protein also detects alkylation damage with high sensitivity in the comet assay. Human whole blood, isolated lymphocytes and V79 cells were treated with alkylating agents and post-incubated with FPG. FPG strongly enhanced MMS- and EMS-induced DNA damage but had no significant effect on ENU-induced DNA damage, indicating that the amount of N-7 guanine alkylation is responsible for the observed effect. Reducing the pH during alkali unwinding and electrophoresis to 12.5 to avoid the contribution of ALS to the comet assay effects, strongly decreased the sensitivity of the comet assay with and without FPG treatment and prevented DNA migration. We conclude that enhanced DNA effects in the comet assay by FPG after exposure to genotoxins with unknown mode of action should not directly be regarded as evidence for the presence of oxidative damage. Furthermore, reducing the pH leads to a considerable loss in sensitivity and should not be used in biomonitoring and other applications which require a sensitive protocol.

Published

2004

21. Vanadyl sulfate can differentially damage DNA in human lymphocytes and HeLa cells.

Author

Wozniak K and Blasiak J

Subjects

Ascorbic Acid pharmacology, Cell Survival drug effects, Comet Assay, DNA Damage, DNA Repair drug effects, DNA-Formamidopyrimidine Glycosylase pharmacology, Deoxyribonuclease (Pyrimidine Dimer) pharmacology, Dose-Response Relationship, Drug, Drug Combinations, Drug Synergism, Escherichia coli Proteins pharmacology, HeLa Cells pathology, Humans, Hydrogen-Ion Concentration, Lymphocytes pathology, Spin Trapping, DNA drug effects, HeLa Cells drug effects, Hypoglycemic Agents toxicity, Lymphocytes drug effects, Mutagens toxicity, Vanadium Compounds toxicity

Abstract

Using the comet assay, we showed that vanadyl sulfate induced DNA damage in human normal lymphocytes and in HeLa cells. Vanadyl at 0.5 and 1 mM produced DNA single- and double-strand breaks (SSBs and DSBs) in lymphocytes, whereas in HeLa cells we observed only SSBs. Post-treatment of vanadyl-damaged DNA from lymphocytes with formamidopyrimidine-DNA glycosylase (Fpg), an enzyme recognizing oxidized purines, gave rise to a significant increase in the extent of DNA damage. A similar effect was observed in HeLa cells, but, using endonuclease III, we also detected oxidized pyrimidines in DNA of these cells. There were no differences in the extent of DNA damage in the lymphocytes and HeLa cells in the pH >13 and pH 12.1 conditions of the comet assay, which indicates that strand breaks, and not alkali-labile sites, contributed to the measured DNA damage. Study of DNA repair, determined in the comet assay as an ability of cells to decrease of DNA damage, revealed that HeLa cells retained the ability to repair vanadyl-damaged DNA induced at a ten-fold higher concentration than that in lymphocytes. Incubation of the cells with nitrone spin traps DMPO, POBN and PBN decreased the extent of DNA damage, which might follow from the production of free radicals by vanadyl sulfate. The presence of vitamins A, C or E caused an increase of DNA damage in HeLa cells whereas in lymphocytes such an increase was observed only for vitamin C. Our data indicate that vanadyl sulfate can be genotoxic for normal and cancer cells. It seems to have a higher genotoxic potential for cancer cells than for normal lymphocytes. Vitamins A, C and E can increase this potential.

Published

2004

22. Detection of oxidative DNA damage in isolated marine bivalve hemocytes using the comet assay and formamidopyrimidine glycosylase (Fpg).

Author

Gielazyn ML, Ringwood AH, Piegorsch WW, and Stancyk SE

Subjects

Animals, Bivalvia drug effects, Comet Assay, Hemocytes metabolism, Hydrogen Peroxide toxicity, In Vitro Techniques, Ostreidae drug effects, DNA Damage, DNA-Formamidopyrimidine Glycosylase pharmacology, Hemocytes drug effects, Mollusca drug effects, Oxidative Stress drug effects

Abstract

Organisms in polluted areas can be exposed to complex mixtures of chemicals; however, exposure to genotoxic contaminants can be particularly devastating. DNA damage can lead to necrosis, apoptosis, or heritable mutations, and therefore has the potential to impact populations as well as individuals. Single cell gel electrophoresis (the comet assay) is a simple and sensitive technique used to examine DNA damage in single cells. The lesion-specific DNA repair enzyme formamidopyrimidine glycoslyase (Fpg) can be used in conjunction with the comet assay to detect 8-oxoguanine and other damaged bases, which are products of oxidative damage. Fpg was used to detect oxidative DNA damage in experiments where isolated oyster (Crassostrea virginica) and clam (Mercenaria mercenaria) hemocytes were exposed to hydrogen peroxide. Standard enzyme buffers used with Fpg and the comet assay produced unacceptably high amounts of DNA damage in the marine bivalve hemocytes used in this study necessitating a modification of existing methods. A sodium chloride based reaction buffer was successfully used. Oxidative DNA damage can be detected in isolated oyster and clam hemocytes using Fpg and the comet assay when the sodium chloride reaction buffer and protocols outlined here are employed. The use of DNA repair enzymes, such as Fpg, in conjunction with the comet assay expands the usefulness and sensitivity of this assay, and provides important insights into the mechanisms of DNA damage.

Published

2003

23. Effects of ozone on DNA single-strand breaks and 8-oxoguanine formation in A549 cells.

Author

Cheng TJ, Kao HP, Chan CC, and Chang WP

Subjects

Antioxidants pharmacology, Ascorbic Acid pharmacology, Comet Assay, DNA Repair, DNA-Formamidopyrimidine Glycosylase pharmacology, Dose-Response Relationship, Drug, Humans, Oxidative Stress, Tumor Cells, Cultured, Vitamin E pharmacology, DNA Damage, Guanine analogs & derivatives, Guanine analysis, Lung Neoplasms pathology, Oxidants, Photochemical toxicity, Ozone toxicity

Abstract

Animal studies have demonstrated that ozone exposure can induce lung tumors. Recent epidemiological studies have also shown that increased ozone exposure is associated with a greater risk of lung cancer. This study used single-cell gel electrophoresis (the Comet assay) and flow cytometry to investigate DNA damage in A549 cells exposed to ozone levels below the current ambient standard. Cells were exposed to ozone at levels of 0, 60, 80, and 120 ppb, and then DNA single-strand breaks and 8-oxoguanine levels were measured. Additionally, the formamidopyrimidine glycosylase (Fpg) repair enzyme was added to the Comet assay to enhance detection of oxidative damage. Vitamins C and E were also added to determine their inhibitory effects on ozone-induced 8-oxoguanine. Measurements of tail length, tail intensity, and tail moment of the Comet assay were shown to correlate with each other. However, tail moment appeared to be more sensitive than the other two indicators in detecting DNA single-strand breaks. Tail moments of cells exposed to 80 and 120 ppb of ozone were significantly higher than those exposed to 0 ppb (P<0.05). These three indicators of DNA single-strand breaks with Fpg were shown to be increased and more sensitive than those without Fpg. After Fpg was introduced, the tail moments at ozone levels of 60, 80, and 120 ppb were significantly higher than those at 0 ppb (P<0.05). Furthermore, 8-oxoguanine levels, determined by fluorescence intensity, at 80 and 120 ppb of ozone exposure were significantly higher than the level at 0 ppb. Pretreatment with vitamins C and E reduced the 8-oxoguanine levels caused by ozone. We conclude that ozone levels below current ambient standards may induce DNA breaks and oxidative DNA damage. Moreover, the Fpg repair enzyme in the Comet assay can increase the sensitivity of oxidative damage detection in vitro.

Published

2003

24. Measurement of DNA oxidation in human cells by chromatographic and enzymic methods.

Subjects

Cell Line, Chromatography, High Pressure Liquid methods, DNA drug effects, DNA Damage, DNA Repair, DNA-Formamidopyrimidine Glycosylase pharmacology, Dose-Response Relationship, Drug, Free Radicals, Gas Chromatography-Mass Spectrometry methods, Guanine pharmacology, HeLa Cells, Humans, Hydrolysis, Light, Photosensitizing Agents pharmacology, Pyrrolidines pharmacology, Quinolizines pharmacology, Chromatography methods, DNA metabolism, Guanine analogs & derivatives, Oxygen metabolism

Abstract

The European Standards Committee on Oxidative DNA Damage (ESCODD) was set up to resolve problems in the measurement of DNA oxidation that have resulted in varying estimates of the extent of this damage in humans. HeLa cells, sent to members for analysis, were either untreated, or treated with light in the presence of a photosensitizer to induce different amounts of 8-oxo-7,8-dihydroguanine (8-oxoGua) in DNA. Laboratories employing HPLC with electrochemical detection were able to measure the induced damage with similar efficiency; dose response gradients for seven of the eight sets of results were almost identical. GC-MS and HPLC-MS/MS, employed in three laboratories, did not convincingly detect the dose response. An alternative approach to measuring base oxidation employs the enzyme formamidopyrimidine DNA N-glycosylase (FPG) to convert 8-oxoGua to strand breaks, which are then measured by alkaline unwinding, alkaline elution, or the comet assay. Ten laboratories used this approach; five were able to detect the dose response in cells treated with photosensitizer plus light (at lower doses than for chromatographic methods, because the enzymic methods are more sensitive and less prone to spurious oxidation). Median values for 8-oxoGua (or FPG-sensitive sites) in untreated cells were 4.01 per 10(6) guanines for chromatographic methods, and 0.53 per 10(6) guanines for techniques based on FPG.

Published

2003