Your search keyword '"Aflatoxin B1 analogs & derivatives"' showing total 112 results

1. Oncogenic and tumor suppressor pathways in subchronic aflatoxicosis in rats: Association with serum and urinary aflatoxin exposure biomarkers.

Author

Apolinário LA, Ramalho LNZ, Moosavi MH, Jager AV, Augusto MJ, Trotta MR, Petta T, Khaneghah AM, Oliveira CAF, and Ramalho FS

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 blood, Aflatoxin B1 metabolism, Aflatoxin B1 urine, Aflatoxin M1 urine, Alanine Transaminase metabolism, Animals, Aspartate Aminotransferases metabolism, Biomarkers blood, Biomarkers urine, Gene Expression drug effects, Guanine analogs & derivatives, Guanine urine, Hepatocytes drug effects, Liver drug effects, Liver pathology, Lysine blood, Male, Precancerous Conditions chemically induced, Precancerous Conditions pathology, Rats, Wistar, Rats, Aflatoxin B1 toxicity, Cyclin D1 metabolism, Cyclin-Dependent Kinase Inhibitor p27 metabolism, Retinoblastoma Protein metabolism, beta Catenin metabolism

Abstract

In this study, the changes in oncogenic and tumor suppressor signaling pathways in liver and their association with serum and urinary biomarkers of aflatoxin exposure were evaluated in Wistar rats fed diets containing aflatoxin B 1 (AFB 1 ) for 90 days. Rats were divided into four groups (n = 15 per group) and assigned to dietary treatments containing 0 (control), 50 (AFB50), 100 (AFB100) and 200 μg AFB 1 kg -1 diet (AFB200). Multiple preneoplastic foci of hepatocytes marked with glutathione-S-transferase-placental form (GST-P) were identified in AFB100 and AFB200 groups. Hepatocellular damage induced by AFB 1 resulted in overexpression of cyclin D1 and β-catenin. The liver expression of retinoblastoma (Rb) and p27 Kip1 decreased in AFB100 and AFB200 groups, confirming the favorable conditions for neoplastic progression to hepatocellular carcinoma. All samples from rats fed AFB 1 -contaminated diets had quantifiable AFB 1 -lysine in serum or urinary AFM 1 and AFB 1 -N 7 -guanine, with mean levels of 20.42-50.34 ng mL -1 , 5.31-37.68 and 39.15-126.37 ng mg -1 creatinine, respectively. Positive correlations were found between AFB 1 -lysine, AFM 1 or AFB 1 -N 7 -guanine and GST-P+, β-catenin+ and cyclin D1+ hepatocytes, while Rb + cells negatively correlated with those AFB 1 exposure biomarkers. The pathways evaluated are critical molecular mechanisms of AFB 1 -induced hepatocarcinogenesis in rats., (Copyright © 2021 Elsevier Ltd. All rights reserved.)

Published

2021

2. Dealing with aflatoxin B1 dihydrodiol acute effects: Impact of aflatoxin B1-aldehyde reductase enzyme activity in poultry species tolerant to AFB1 toxic effects.

Author

Murcia H and Diaz GJ

Subjects

Aflatoxin B1 chemistry, Aflatoxin B1 toxicity, Animals, Female, Kinetics, Male, Aflatoxin B1 analogs & derivatives, Aldehyde Reductase metabolism, Poultry metabolism

Abstract

Aflatoxin B1 aldehyde reductase (AFAR) enzyme activity has been associated to a higher resistance to the aflatoxin B1 (AFB1) toxicity in ethoxyquin-fed rats. However, no studies about AFAR activity and its relationship with tolerance to AFB1 have been conducted in poultry. To determine the role of AFAR in poultry tolerance, the hepatic in vitro enzymatic activity of AFAR was investigated in liver cytosol from four commercial poultry species (chicken, quail, turkey and duck). Specifically, the kinetic parameters Vmax, Km and intrinsic clearance (CLint) were determined for AFB1 dialdehyde reductase (AFB1-monoalcohol production) and AFB1 monoalcohol reductase (AFB1-dialcohol production). In all cases, AFB1 monoalcohol reductase activity saturated at the highest aflatoxin B1 dialdehyde concentration tested (66.4 μM), whereas AFB1 dialdehyde reductase did not. Both activities were highly and significantly correlated and therefore are most likely catalyzed by the same AFAR enzyme. However, it appears that production of the AFB1 monoalcohol is favored over the AFB1 dialcohol. The production of alcohols from aflatoxin dialdehyde showed the highest enzymatic efficiency (highest CLint value) in chickens, a species resistant to AFB1; however, it was also high in the turkey, a species with intermediate sensitivity; further, CLint values were lowest in another tolerant species (quail) and in the most sensitive poultry species (the duck). These results suggest that AFAR activity is related to resistance to the acute toxic effects of AFB1 only in chickens and ducks. Genetic selection of ducks for high AFAR activity could be a means to control aflatoxin sensitivity in this poultry species., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

3. An unusually high production of hepatic aflatoxin B 1 -dihydrodiol, the possible explanation for the high susceptibility of ducks to aflatoxin B 1 .

Author

Diaz GJ and Murcia HW

Subjects

Aflatoxin B1 chemistry, Aflatoxin B1 toxicity, Animal Feed, Animals, Chickens, Ducks, Kinetics, Liver pathology, Microsomes, Liver drug effects, Oxidoreductases chemistry, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Liver drug effects, Oxidoreductases genetics

Abstract

A study was conducted to determine the enzymatic kinetic parameters V max , K M , and intrinsic clearance (CL int ) for the hepatic in vitro production of aflatoxin B 1 -dihydrodiol (AFB 1 -dhd) from aflatoxin B 1 (AFB 1 ) in four commercial poultry species, ranging in sensitivity to AFB 1 from highest (ducks) to lowest (chickens). Significant but small differences were seen for V max , while large significant differences were observed for K M . However, the largest inter-species differences were observed for the CL int parameter, with ducks being extraordinarily efficient in converting AFB 1 into AFB 1 -dhd. Since AFB 1 -dhd is considered the metabolite responsible for the acute toxic effects of AFB 1 , the high hepatic production of AFB 1 -dhd from AFB 1 in ducks is the possible biochemical explanation for the extraordinary high sensitivity of this poultry species to the adverse effects of AFB 1 .

Published

2019

4. Aflatoxin B1: A review on metabolism, toxicity, occurrence in food, occupational exposure, and detoxification methods.

Author

Rushing BR and Selim MI

Subjects

Aflatoxin B1 metabolism, Aflatoxin B1 radiation effects, Aflatoxin B1 toxicity, Animals, Carcinogens chemistry, Carcinogens radiation effects, Carcinogens toxicity, Carcinoma, Hepatocellular etiology, Cytochrome P-450 Enzyme System metabolism, DNA Adducts metabolism, Decontamination, Food Contamination prevention & control, Food Contamination statistics & numerical data, Gamma Rays, Growth Disorders etiology, Humans, Immunologic Factors chemistry, Immunologic Factors metabolism, Immunologic Factors radiation effects, Immunologic Factors toxicity, Liver Neoplasms etiology, Malnutrition etiology, Occupational Exposure statistics & numerical data, Aflatoxin B1 analogs & derivatives, Carcinogenesis metabolism, Carcinogens metabolism, Carcinoma, Hepatocellular metabolism, Liver Neoplasms metabolism

Abstract

Aflatoxins are a class of carcinogenic mycotoxins produced by Aspergillus fungi and are known to contaminate a large portion of the world's food supply. Aflatoxin B1 (AFB1) is the most potent of these compounds and has been well-characterized to lead to the development of hepatocellular carcinoma (HCC) in humans and animals. This review focuses on the metabolism of AFB1, including epoxidation and DNA adduction, as it concerns the initiation of cancer and the underlying mechanisms. The link between AFB1 consumption and HCC is also discussed including synergistic interactions with the hepatitis B virus. Toxic effects of AFB1, including growth suppression, malnutrition, and immunomodulation, are also covered. This review also describes recent reports of AFB1 occurrence in global food supplies and exposures in occupational settings. Furthermore, a summary of recent detoxification methods is included to indicate the present state of the field in developing aflatoxin control methods. This information shows that AFB1 occurs frequently in food supplies at high concentrations, particularly in maize. Regarding detoxification methods, chemical control methods were the fastest methods that still retained high detoxification efficacy. The information presented here highlights the need to implement new and/or existing detoxification methods to reduce the global burden of AFB1 toxicity., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2019

5. Pathways of Metabolite-Related Damage to a Synthetic p53 Gene Exon 7 Oligonucleotide Using Magnetic Enzyme Bioreactor Beads and LC-MS/MS Sequencing.

Author

Malla S, Kadimisetty K, Jiang D, Choudhary D, and Rusling JF

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, Bioreactors, Chromatography, Liquid, Cytochrome P-450 Enzyme System chemistry, Humans, Exons, Magnetic Fields, Mass Spectrometry, Oligonucleotides chemistry, Sequence Analysis, DNA methods, Tumor Suppressor Protein p53 genetics

Abstract

Reactive metabolites of environmental chemicals and drugs can cause site specific damage to the p53 tumor suppressor gene in a major pathway for genotoxicity. We report here a high-throughput, cell-free, 96-well plate magnetic bead-enzyme system interfaced with LC-MS/MS sequencing for bioactivating test chemicals and identifying resulting adduction sites on genes. Bioactivated aflatoxin B1 was reacted with a 32 bp exon 7 fragment of the p53 gene using eight microsomal cytochrome (cyt) P450 enzymes from different organs coated on magnetic beads. All cyt P450s converted aflatoxin B1 to aflatoxin B1-8,9-epoxide that adducts guanine (G) in codon 249, with subsequent depurination to give abasic sites and then strand breaks. This is the first demonstration in a cell-free medium that the aflatoxin B1 metabolite selectively causes abasic site formation and strand breaks at codon 249 of the p53 probe, corresponding to the chemical pathway and mutations of p53 in human liver cells and tumors. Molecular modeling supports the view that binding of aflatoxin B1-8,9-epoxide to G in codon 249 precedes the S N 2 adduction reaction. Among a range of metabolic enzymes characteristic of different organs, human liver microsomes and cyt P450 3A5 supersomes showed the highest bioactivation rate for p53 exon 7 damage. This method of identifying metabolite-related gene damage sites may facilitate predictions of organ specific cancers for test chemicals via correlations with mutation sites.

Published

2018

6. Editor's Highlight: Pregnancy Alters Aflatoxin B1 Metabolism and Increases DNA Damage in Mouse Liver.

Author

Sriwattanapong K, Slocum SL, Chawanthayatham S, Fedeles BI, Egner PA, Groopman JD, Satayavivad J, Croy RG, and Essigmann JM

Subjects

Activation, Metabolic, Aflatoxin B1 metabolism, Aflatoxin B1 toxicity, Animals, Carcinogens metabolism, Cytochrome P-450 CYP1A2 metabolism, Cytochrome P-450 CYP3A metabolism, DNA Adducts metabolism, Female, Gestational Age, Glutathione Transferase metabolism, Guanine metabolism, Guanine toxicity, Hepatocytes metabolism, Isoenzymes metabolism, Liver metabolism, Maternal Exposure, Mice, Inbred C3H, Mice, Inbred C57BL, Mice, Transgenic, Pregnancy, Aflatoxin B1 analogs & derivatives, Carcinogens toxicity, DNA Damage, Guanine analogs & derivatives, Hepatocytes drug effects, Liver drug effects

Abstract

Pregnancy is a complex physiological state, in which the metabolism of endogenous as well as exogenous agents is ostensibly altered. One exogenous agent of concern is the hepatocarcinogen aflatoxin B1 (AFB1), a foodborne fungal toxin, that requires phase I metabolic oxidation for conversion to its toxic and carcinogenic form, the AFB1-8,9-exo-epoxide. The epoxide interacts with cellular targets causing toxicity and cell death; these targets include the covalent modification of DNA leading to mutations that can initiate malignant transformation. The main detoxification pathway of the AFB1-epoxide involves phase II metabolic enzymes including the glutathione-S-transferase (GST) family. Pregnancy can modulate both phase I and II metabolism and alter the biological potency of AFB1. The present work investigated the impact of pregnancy on AFB1 exposure in mice. A single IP dose of 6 mg/kg AFB1 was administered to pregnant C57BL/6 J mice at gestation day 14 and matched non-pregnant controls. Pregnant mice accumulated 2-fold higher AFB1-N7-guanine DNA adducts in the liver when compared with nonpregnant controls 6 h post-exposure. Enhanced DNA adduct formation in pregnant animals paralleled elevated hepatic protein expression of mouse CYP1A2 and mouse homologs of human CYP3A4, phase I enzymes capable of bioactivating AFB1. Although phase II enzymes GSTA1/2 showed decreased protein expression, GSTA3, the primary enzymatic protection against the AFB1-epoxide, was unaffected at the protein level. Taken together, our results reveal that pregnancy may constitute a critical window of susceptibility for maternal health, and provide insight into the biochemical factors that could explain the underlying risks., (© The Author 2017. Published by Oxford University Press on behalf of the Society of Toxicology.)

Published

2017

7. DNA polymerase ζ limits chromosomal damage and promotes cell survival following aflatoxin exposure.

Author

Lin YC, Owen N, Minko IG, Lange SS, Tomida J, Li L, Stone MP, Wood RD, McCullough AK, and Lloyd RS

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 genetics, Aflatoxin B1 toxicity, Aflatoxins toxicity, Animals, Carcinoma, Hepatocellular chemically induced, Carcinoma, Hepatocellular pathology, Cell Survival drug effects, Chromosome Aberrations drug effects, Cytidine analogs & derivatives, Cytidine genetics, Cytidine toxicity, DNA Adducts drug effects, DNA Adducts genetics, DNA Damage drug effects, DNA Repair genetics, DNA-Directed DNA Polymerase chemistry, Fibroblasts drug effects, Fibroblasts metabolism, Humans, Liver Neoplasms chemically induced, Liver Neoplasms pathology, Mice, Mutagenesis drug effects, Mutagenesis genetics, Mutation, Carcinoma, Hepatocellular genetics, DNA-Binding Proteins genetics, DNA-Directed DNA Polymerase genetics, Liver Neoplasms genetics

Abstract

Routine dietary consumption of foods that contain aflatoxins is the second leading cause of environmental carcinogenesis worldwide. Aflatoxin-driven mutagenesis is initiated through metabolic activation of aflatoxin B 1 (AFB 1 ) to its epoxide form that reacts with N7 guanine in DNA. The resulting AFB 1 -N7-dG adduct undergoes either spontaneous depurination or imidazole-ring opening yielding formamidopyrimidine AFB 1 (AFB 1 -Fapy-dG). Because this latter adduct is known to persist in human tissues and contributes to the high frequency G-to-T mutation signature associated with many hepatocellular carcinomas, we sought to establish the identity of the polymerase(s) involved in processing this lesion. Although our previous biochemical analyses demonstrated the ability of polymerase ζ (pol ζ) to incorporate an A opposite AFB 1 -Fapy-dG and extend from this mismatch, biological evidence supporting a unique role for this polymerase in cellular tolerance following aflatoxin exposure has not been established. Following challenge with AFB 1 , survival of mouse cells deficient in pol ζ (Rev3L -/- ) was significantly reduced relative to Rev3L +/- cells or Rev3L -/- cells complemented through expression of the wild-type human REV3L. Furthermore, cell-cycle progression of Rev3L -/- mouse embryo fibroblasts was arrested in late S/G2 following AFB 1 exposure. These Rev3L -/- cells showed an increase in replication-dependent formation of γ-H2AX foci, micronuclei, and chromosomal aberrations (chromatid breaks and radials) relative to Rev3L +/- cells. These data suggest that pol ζ is essential for processing AFB 1 -induced DNA adducts and that, in its absence, cells do not have an efficient backup polymerase or a repair/tolerance mechanism facilitating survival., Competing Interests: The authors declare no conflict of interest.

Published

2016

8. Bioactivation and Regioselectivity of Pig Cytochrome P450 3A29 towards Aflatoxin B₁.

Author

Wu J, Chen R, Zhang C, Li K, Xu W, Wang L, Chen Q, Mu P, Jiang J, Wen J, and Deng Y

Subjects

Activation, Metabolic, Aflatoxin B1 metabolism, Allosteric Regulation, Animals, Binding Sites, Cloning, Molecular, Cytochrome P-450 CYP3A genetics, Isoenzymes, Molecular Docking Simulation, Mutagenesis, Site-Directed, Mutation, Protein Binding, Protein Conformation, Recombinant Proteins metabolism, Structure-Activity Relationship, Substrate Specificity, Sus scrofa, Aflatoxin B1 analogs & derivatives, Cytochrome P-450 CYP3A metabolism, Liver enzymology

Abstract

Due to unavoidable contaminations in feedstuff, pigs are easily exposed to aflatoxin B₁ (AFB₁) and suffer from poisoning, thus the poisoned products potentially affect human health. Heretofore, the metabolic process of AFB₁ in pigs remains to be clarified, especially the principal cytochrome P450 oxidases responsible for its activation. In this study, we cloned CYP3A29 from pig liver and expressed it in Escherichia coli, and its activity has been confirmed with the typical P450 CO-reduced spectral characteristic and nifedipine-oxidizing activity. The reconstituted membrane incubation proved that the recombinant CYP3A29 was able to oxidize AFB₁ to form AFB₁-exo-8,9-epoxide in vitro. The structural basis for the regioselective epoxidation of AFB₁ by CYP3A29 was further addressed. The T309A mutation significantly decreased the production of AFBO, whereas F304A exhibited an enhanced activation towards AFB₁. In agreement with the mutagenesis study, the molecular docking simulation suggested that Thr309 played a significant role in stabilization of AFB₁ binding in the active center through a hydrogen bond. In addition, the bulk phenyl group of Phe304 potentially imposed steric hindrance on the binding of AFB₁. Our study demonstrates the bioactivation of pig CYP3A29 towards AFB₁ in vitro, and provides the insight for understanding regioselectivity of CYP3A29 to AFB₁., Competing Interests: The authors declare no conflict of interest.

Published

2016

9. Assessment of aflatoxin exposure using serum and urinary biomarkers in São Paulo, Brazil: A pilot study.

Author

Jager AV, Tonin FG, Baptista GZ, Souto PC, and Oliveira CA

Subjects

Adult, Aflatoxin B1 blood, Aflatoxin B1 urine, Arachis chemistry, Biomarkers blood, Biomarkers urine, Brazil, Dairy Products analysis, Diet, Environmental Monitoring, Guanine urine, Humans, Middle Aged, Pilot Projects, Zea mays chemistry, Aflatoxin B1 analogs & derivatives, Aflatoxin M1 urine, Food Contamination analysis, Guanine analogs & derivatives, Lysine blood

Abstract

The aim of this study was to evaluate the human exposure of individuals from Pirassununga, Brazil, to dietary aflatoxins B1 (AFB1) and M1 (AFM1) by determination of serum AFB1-lysine and urinary aflatoxin biomarkers (AFM1 and AFB1-N(7)-guanine). The participants were recruited among employees from a Campus of the University of São Paulo, which provided food samples from their homes, as well as serum and urine samples four times every three months, from June 2011 until March 2012. The probable daily intake (PDI) of aflatoxin was estimated by using the results from analysis of food products collected by the time of samples collection, and data from a 24-hour dietary recall questionnaire. Analyses of AFB1 and AFM1 in food samples were conducted by high-performance liquid chromatography with fluorescence detection. Biomarkers in serum and urine were determined by tandem mass spectrometry. AFB1 and AFM1 were detected in 38 samples of cereals (28%, N=136) and 31 milk products (36%, N=86), respectively. AFB1-lysine and AFB1-N(7)-guanine and were not detected in serum or urine samples, respectively. However, AFM1 was found in 74 urine samples (65%), at mean levels in the 4 sampling times ranging from 0.37±0.23 to 1.70±2.88pg/mg creatinine. The mean PDI varied among different sampling times, ranging from 0.09±0.09 to 1.35±5.98ng/kg body weight/day. A modest though significant correlation (r=0.45; p=0.03; N=23) was found for the first time in Brazil between the AFM1 concentration in urine and the PDI for total aflatoxins (AFB1+AFM1) in sampling 1 (June 2011). Urinary AFM1 was confirmed as very sensitive for monitoring the human exposure to dietary aflatoxin. Further studies using serum and urinary biomarkers are needed to estimate the aflatoxin exposure of populations in higher risk areas in Brazil., (Copyright © 2015 Elsevier GmbH. All rights reserved.)

Published

2016

10. DNA Sequence Modulates Geometrical Isomerism of the trans-8,9- Dihydro-8-(2,6-diamino-4-oxo-3,4-dihydropyrimid-5-yl-formamido)- 9-hydroxy Aflatoxin B1 Adduct.

Author

Li L, Brown KL, Ma R, and Stone MP

Subjects

Base Sequence, Cytidine chemistry, Magnetic Resonance Spectroscopy, Stereoisomerism, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, Cytidine analogs & derivatives, DNA chemistry

Abstract

Aflatoxin B(1) (AFB(1)), a mycotoxin produced by Aspergillus flavus, is oxidized by cytochrome P450 enzymes to aflatoxin B(1)-8,9-epoxide, which alkylates DNA at N7-dG. Under basic conditions, this N7-dG adduct rearranges to yield the trans-8,9-dihydro-8-(2,6-diamino-4-oxo-3,4-dihydropyrimid-5-yl-formamido)-9-hydroxy aflatoxin B(1) (AFB(1)−FAPY) adduct. The AFB(1)−FAPY adduct exhibits geometrical isomerism involving the formamide moiety. NMR analyses of duplex oligodeoxynucleotides containing the 5′-XA-3′, 5′-XC-3′, 5′-XT-3′, and 5′-XY-3′ sequences (X = AFB(1)−FAPY; Y = 7-deaza-dG)demonstrate that the equilibrium between E and Z isomers is controlled by major groove hydrogen bonding interactions.Structural analysis of the adduct in the 5′-XA-3′ sequence indicates the preference of the E isomer of the formamide group,attributed to formation of a hydrogen bond between the formyl oxygen and the N(6) exocyclic amino group of the 3′-neighboradenine. While the 5′-XA-3′ sequence exhibits the E isomer, the 5′-XC-3′ sequence exhibits a 7:3 E:Z ratio at equilibrium at 283K. The E isomer is favored by a hydrogen bond between the formyl oxygen and the N(4)-dC exocyclic amino group of the 3′-neighbor cytosine. The 5′-XT-3′ and 5′-XY-3′ sequences cannot form such a hydrogen bond between the formyl oxygen and the 3′-neighbor T or Y, respectively, and in these sequence contexts the Z isomer is favored. Additional equilibria between α and β anomers and the potential to exhibit atropisomers about the C5−N(5) bond do not depend upon sequence. In each of the four DNA sequences, the AFB(1)−FAPY adduct maintains the β deoxyribose configuration. Each of these four sequences feature the atropisomer of the AFB(1) moiety that is intercalated above the 5′-face of the damaged guanine. This enforces the Ra axialc onformation for the C5−N(5) bond.

Published

2015

11. Analyses by UPLC Q-TOF MS of products of aflatoxin B(1) after ozone treatment.

Author

Luo X, Wang R, Wang L, Li Y, Zheng R, Sun X, Wang Y, Chen Z, and Tao G

Subjects

Aflatoxin B1 chemistry, Aflatoxin B1 toxicity, Chromatography, High Pressure Liquid methods, Food Contamination prevention & control, Food Handling, Food Safety, Hazard Analysis and Critical Control Points methods, Humans, Molecular Structure, Spectrometry, Mass, Electrospray Ionization methods, Structure-Activity Relationship, Aflatoxin B1 analogs & derivatives, Food Contamination analysis, Ozone

Abstract

Analysing the products of ozone-treated aflatoxin B1 (AFB1) is essential in order to study the practical use of ozone treatment. In this paper, the products of AFB1 were investigated using ultra-performance liquid chromatography-quadrupole time-of-flight mass spectrometry (UPLC Q-TOF MS). The products were well separated using UPLC, and the accurate masses of all the products were determined using Q-TOF MS. Finally, the possible pathways of fragmentation ion generation from the products of AFB1 and the structures of four products were proposed. From the view of the proposed structures of products, the C8-C9 double bond in the terminal furan ring was destroyed. According to the structure-activity relationship, the toxicity of products was significantly reduced compared with that of AFB1. The result indicated that ozone was an effective agent for degrading AFB1, and UPLC Q-TOF MS was a useful analytical tool for proposing and identifying a series of unknown products.

Published

2014

12. Functional characterization of alpha-class glutathione s-transferases from the Turkey (meleagris gallopavo).

Author

Kim JE, Bunderson BR, Croasdell A, and Coulombe RA Jr

Subjects

Aflatoxin B1 pharmacokinetics, Aflatoxin B1 toxicity, Amino Acid Sequence, Animals, Cloning, Molecular, Cytosol enzymology, Electrophoresis, Polyacrylamide Gel, Escherichia coli genetics, Glutathione Transferase chemistry, Glutathione Transferase genetics, Humans, Isoenzymes chemistry, Isoenzymes genetics, Liver drug effects, Male, Mice, Molecular Sequence Data, Protein Structure, Secondary, Protein Subunits, Rats, Sequence Alignment, Species Specificity, Substrate Specificity, Aflatoxin B1 analogs & derivatives, Glutathione Transferase physiology, Isoenzymes physiology, Liver enzymology, Turkeys

Abstract

Six Alpha-class glutathione S-transferase (GST) subunits were cloned from domestic turkey livers, which are one of the most susceptible animals known to the carcinogenic mycotoxin aflatoxin B₁. In most animals, GST dysfunction is a risk factor for susceptibility toward AFB₁, and we have shown that turkeys lack GSTs with affinity toward the carcinogenic intermediate exo-aflatoxin B(1)-8-9-epoxide (AFBO). Conversely, mice are resistant to AFB₁ carcinogenesis, due to high constitutive expression of mGSTA3 that has high affinity toward AFBO. When expressed in Escherichia coli, all six tGSTA subunits possessed conjugating activities toward substrates 1-chloro-2,4-dinitrobenzene (CDNB), 1,2-dichloro-4-nitrobenzene (DCNB), ethacrynic acid (ECA), and cumene hydroperoxide (CHP) with tGSTA1.2 appearing most active. Interestingly, tGSTA1.1, which lacks one of the four Alpha-class signature motifs, possessed enzymatic activities toward all substrates. All had comparable activities toward AFBO conjugation, an activity absent in turkey liver cytosols. E. coli-expressed mGSTA3 conjugated AFBO with more than 3-fold greater activity than that of tGSTAs and had higher activity toward GST prototype substrates. Mouse hepatic cytosols had approximately 900-fold higher catalytic activity toward AFBO compared with those from turkey. There was no apparent amino acid profile in tGSTAs that might correspond to specificity toward AFBO, although tGSTA1.2, which had slightly higher AFBO-trapping ability, shared Tyr¹⁰⁸ with mGSTA3, a residue postulated to be critical for AFBO trapping activity in mammalian systems. The observation that recombinant tGSTAs detoxify AFBO, whereas their hepatic forms do not, implies that the hepatic forms of these enzymes are silenced by one or more regulatory mechanisms.

Published

2011

13. Role of aflatoxin B1 as a risk for primary liver cancer in north Indian population.

Author

Asim M, Sarma MP, Thayumanavan L, and Kar P

Subjects

Adult, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 urine, Alcohol Drinking, Carcinoma, Hepatocellular etiology, Case-Control Studies, Chronic Disease, Female, Food Analysis, Food Microbiology, Guanine analogs & derivatives, Hepatitis B complications, Hepatitis C complications, Humans, India, Liver Diseases epidemiology, Liver Neoplasms etiology, Male, Middle Aged, Risk Factors, Aflatoxin B1 analysis, Carcinoma, Hepatocellular epidemiology, Liver Neoplasms epidemiology

Abstract

Objectives: The present study was designed to determine whether aflatoxin B1 (AFB1) exposure has any role to play in hepatocellular carcinoma (HCC) patients from northern India., Design and Methods: A total of 266 HCC patients and 251 patients of chronic liver disease without-HCC were enrolled into the study. All samples were screened for serological markers for hepatitis B and C infections and levels of AFB1 in food and urine samples., Results: A threefold (OR=3.43) and five-fold (OR=5.47) increased risk of HCC was observed amongst HBV infection and AFB1-levels in food and urine samples, respectively. However, a non-significant risk was observed with respect to HCV infection (OR=1.27) and alcohol consumption (OR=1.18). A threefold (OR=3.15) increased risk of HCC was observed amongst cases of non-viral etiology with respect to urinary AFB1., Conclusion: The data provides an exposure and disease risk information for establishing intervention studies to diminish the impact of aflatoxin exposure in Indian population., (Copyright © 2011. Published by Elsevier Inc.)

Published

2011

14. Sulforaphane-mediated reduction of aflatoxin B₁-N⁷-guanine in rat liver DNA: impacts of strain and sex.

Author

Fiala JL, Egner PA, Wiriyachan N, Ruchirawat M, Kensler KH, Wogan GN, Groopman JD, Croy RG, and Essigmann JM

Subjects

Aflatoxin B1 metabolism, Animals, Dose-Response Relationship, Drug, Female, Guanine metabolism, Isothiocyanates, Liver metabolism, Male, Rats, Rats, Inbred F344, Rats, Sprague-Dawley, Species Specificity, Sulfoxides, Aflatoxin B1 analogs & derivatives, Anticarcinogenic Agents pharmacology, DNA drug effects, Guanine analogs & derivatives, Liver drug effects, Thiocyanates pharmacology

Abstract

Aflatoxin B₁ (AFB₁) is a DNA-binding toxin that contributes to the burden of liver cancer in tropical areas. AFB₁-DNA adducts are powerful biomarkers that discern individual and population risk from exposure to this carcinogen. The discovery of concordance between the metabolic pathways of the male Fischer rat and humans allowed data from rats to guide the development of chemoprevention strategies employed in clinical trials in high-risk regions. In this study, the variables of strain and sex are studied in the rat model, as a step toward understanding how ethnic differences and sex influence DNA adduct formation and the induction of enzymes by chemoprotective agents. Sulforaphane (SF), which induces phase II enzymes including glutathione S-transferases (GSTs), was evaluated for its ability to induce GST activity and reduce the AFB₁-DNA adducts in livers of both sexes of two rat strains that differ in susceptibility to AFB₁ hepatocarcinogenesis. A dose-dependent relationship was found for SF for both induction of GST and reduction in of AFB₁-N⁷-guanine in both Fischer (sensitive to AFB₁) and Sprague-Dawley rats (relatively resistant). Sprague-Dawley rats exhibited the greatest increase in GST levels and the largest reduction in AFB₁-N⁷-guanine in liver DNA. Males and females of each strain were also compared to determine if the ability of SF to induce GST and reduce AFB₁-N⁷-guanine correlated with gender differences in sensitivity to AFB₁ carcinogenesis. No gender-specific responses to SF were observed. These results support the view that SF induction of liver GST activity may play a role in its chemoprotective activity.

Published

2011

15. Aflatoxin B1 albumin adducts in plasma and aflatoxin M1 in urine are associated with plasma concentrations of vitamins A and E.

Author

Obuseh FA, Jolly PE, Jiang Y, Shuaib FM, Waterbor J, Ellis WO, Piyathilake CJ, Desmond RA, Afriyie-Gyawu E, and Phillips TD

Subjects

Adult, Aflatoxin B1 blood, Albumins, Antibodies, Viral blood, Cross-Sectional Studies, Female, Ghana, Hepacivirus isolation & purification, Hepatitis B Surface Antigens blood, Hepatitis C blood, Hepatitis C urine, Humans, Liver Function Tests, Male, Multivariate Analysis, Regression Analysis, Socioeconomic Factors, Young Adult, Aflatoxin B1 analogs & derivatives, Aflatoxin M1 urine, Aflatoxins blood, Vitamin A blood, Vitamin E blood

Abstract

Background: Although aflatoxin exposure has been associated with micronutrient deficiency in animals, there are few investigations on the effects of aflatoxin exposure on micronutrient metabolism in humans., Objective: To examine the relationship between aflatoxin B1 (AFB1) albumin adducts (AF-ALB) in plasma and the aflatoxin M1 (AFM1) metabolite in urine and plasma concentrations of retinol (vitamin A) and alpha-tocopherol (vitamin E) in Ghanaians., Methods: A cross-sectional study of 147 adult participants was conducted. Blood and urine samples were tested for aflatoxin and vitamins A and E levels., Results: Multivariable analysis showed that participants with high AF-ALB (>or=0.80 pmol/mg albumin) had increased odds of having vitamin A deficiency compared to those with lower AF-ALB [Odds Ratio (OR)=2.61; CI=1.03-6.58; p=0.04]. Participants with high AF-ALB also showed increased odds of having vitamin E deficiency but this was not statistically significant (OR=2.4; CI=0.96-6.05; p=0.06). Conversely, those with higher AFM1 values had a statistically nonsignificant reduced odds of having vitamin A deficiency (OR=0.31; CI=0.09-1.02; p=0.05) and a statistically significant reduced odds of having vitamin E deficiency (OR=0.31; CI=0.10-0.97; p=0.04). Participants with high AF-ALB or high AFM1 (>or=437.95 pg/dL creatinine) were almost 6 times more likely to be hepatitis B virus surface antigen (HBsAg)-positive (OR=5.88; CI=1.71-20.14; p=0.005) and (OR=5.84; CI=1.15-29.54; p=0.03) respectively., Conclusions: These data indicate that aflatoxin may modify plasma micronutrient status. Thus, preventing aflatoxin exposure may reduce vitamin A and E deficiencies.

Published

2010

16. The role of selected cytochrome P450 enzymes on the bioactivation of aflatoxin B1 by duck liver microsomes.

Author

Diaz GJ, Murcia HW, Cepeda SM, and Boermans HJ

Subjects

Aflatoxin B1 analogs & derivatives, Animals, Blotting, Western, Chromatography, High Pressure Liquid, Female, Fluorescence, Male, Aflatoxin B1 metabolism, Cytochrome P-450 Enzyme System metabolism, Ducks metabolism, Microsomes, Liver metabolism

Abstract

A study was conducted to determine the cytochrome (CYP) P450 enzymes responsible for the bioactivation of aflatoxin B1 (AFB1) into its epoxide form (AFBO) in duck liver microsomes. Six male and six female 6-week-old Pekin ducks were used. The biochemical toxicology strategies applied included the use of selective inhibitors, prototype substrate activity for specific human P450s, correlation between aflatoxin bioactivation and enzymatic activity of prototype substrates, and the expression of specific CYP450 enzymes using antibodies against human CYP450s. Enzymatic activity was detected for the duck orthologues CYP1A1/2, CYP2A6 and CYP3A4 but not for the CYP2D6 orthologue. Immunoreactive proteins for CYP1A1, CYP2A6 and CYP3A4 were also detected. Inhibition studies suggested that the duck turkey CYP2A6 orthologue and, to a lesser extent, the CYP1A1 orthologue are involved in the bioactivation of AFB1. Correlation studies, however, suggest that CYP3A4, CYP2A6 and CYP1A1/2 are all involved in AFBO formation. The finding that four CYP enzymes may be involved in AFB1 bioactivation in ducks could explain the high sensitivity of this species to AFB1. Further studies are needed to fully elucidate the phase I hepatic metabolism of AFB1 in ducks, the only poultry species that develops hepatic cancer from AFB1 exposure.

Published

2010

17. Sulforaphane induces glutathione S-transferase isozymes which detoxify aflatoxin B(1)-8,9-epoxide in AML 12 cells.

Author

Gao SS, Chen XY, Zhu RZ, Choi BM, and Kim BR

Subjects

Aflatoxin B1 metabolism, Animals, Cells, Cultured, Chemoprevention, Dinitrochlorobenzene chemistry, Inactivation, Metabolic, Isoenzymes metabolism, Isothiocyanates, Mice, Sulfoxides, Transfection, Aflatoxin B1 analogs & derivatives, Anticarcinogenic Agents pharmacology, Glutathione Transferase metabolism, Thiocyanates pharmacology

Abstract

The aflatoxin B(1)-8,9-epoxide (AFBO) is hepatocarcinogenic intermediate of aflatoxin B(1) (AFB(1)) and is detoxified by glutathione S-transferases (GSTs). In this study, we investigated whether sulforaphane (SFN) could increase the rate of conjugation between AFBO and glutathione (GSH) as well as which of the GST isozymes were involved in the conjugation reaction. The conjugation potential was inhibited dose dependently with curcumin, an inhibitor of GSTs. SFN induced the expression of GST A3, GST A4, GST M1, GST P1, and GST T1 in alpha mouse line (AML) 12 cells. The cells treated with SFN (10 microM) for 12 h showed a 35-fold increase in conjugation potential of AFBO with GSH compared with the vehicle-treated cell. The conjugation potential was blocked partially by transfection of cells with siRNAs against each of the GST isozymes. The activity of GST A3 had the strongest effect on the conjugation potential. SFN treatment also increased total GST activity detected with 1-chloro-2,4-dinitrobenzene (CDNB) up to 4.3-fold. The induction fold was much lower than that detected with AFBO. These results suggest that the chemopreventive effect of SFN on the decomposition of AFBO is related to the upregulation of several GST isozymes genes. The increase of GST activity by SFN was extremely specific toward the conjugation reaction of AFBO compared with CDNB. Therefore, this system for detecting GST activity seems to be an excellent method for screening chemopreventive compounds toward AFB(1) toxicity.

Published

2010

18. Docking studies on DNA-ligand interactions: building and application of a protocol to identify the binding mode.

Author

Ricci CG and Netz PA

Subjects

Acridines chemistry, Acridines metabolism, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, Aflatoxin B1 metabolism, Binding Sites, Computer Simulation, Crystallography, X-Ray, DNA chemistry, Ellipticines chemistry, Ellipticines metabolism, Ligands, Models, Molecular, Netropsin chemistry, Netropsin metabolism, Nucleic Acid Conformation, DNA metabolism

Abstract

Despite DNA being an important target for several drugs, most of the docking programs are validated only for proteins and their ligands. In this paper, we used AutoDock 4.0 to perform self-dockings and cross dockings between two DNA ligands (a minor groove binder and an intercalator) and four distinct receptors: 1) crystallographic DNA without intercalation gap; 2) crystallographic DNA with intercalation gap; 3) canonical B-DNA; and 4) modified B-DNA with intercalation gap. Besides being efficient in self-dockings, AutoDock is capable of correctly identifying two of the main DNA binding modes with the condition that the target possesses an artificial intercalation gap. Therefore, we suggest a default protocol to identify DNA binding modes which uses a modified canonical DNA (with gap) as receptor. This protocol was applied to dock two different Troger bases to DNA and the predicted binding modes agree with those suggested, yet not established, by experimental data. We also applied the protocol to dock aflatoxin B(1) exo-8,9-epoxide, and the results are in complete agreement with experimental data from the literature. We propose that this approach can be used to investigate other ligands whose binding mode to DNA remains unknown, yielding a suitable starting point for further theoretical studies such as molecular dynamics simulations.

Published

2009

19. Inherent stereospecificity in the reaction of aflatoxin B(1) 8,9-epoxide with deoxyguanosine and efficiency of DNA catalysis.

Author

Brown KL, Bren U, Stone MP, and Guengerich FP

Subjects

Aflatoxin B1 chemistry, Catalysis, Chromatography, High Pressure Liquid, Stereoisomerism, Tandem Mass Spectrometry, Thermodynamics, Aflatoxin B1 analogs & derivatives, DNA chemistry, Deoxyguanosine chemistry

Abstract

Kinetic analysis of guanine alkylation by aflatoxin B(1) exo-8,9-epoxide, the reactive form of the hepatocarcinogen aflatoxin B(1), shows the reaction to be >2000 times more efficient in DNA than in aqueous solution, that is, with free 2'-deoxyguanosine. Thermodynamic analysis reveals AFB(1) exo-8,9-epoxide intercalation as the predominant source of the observed DNA catalytic effect. However, the known exo > endo epoxide stereospecificity of the DNA alkylation is observed even with free deoxyguanosine (ratio >20:1 determined by LC-MS and NMR measurements), as predicted by theoretical calculations [ Bren , U. , et al. ( 2007 ) Chem. Res. Toxciol. 20 , 1134 - 1140 ].

Published

2009

20. Protective effect of Ocimum sanctum on 3-methylcholanthrene, 7,12-dimethylbenz(a)anthracene and aflatoxin B1 induced skin tumorigenesis in mice.

Author

Rastogi S, Shukla Y, Paul BN, Chowdhuri DK, Khanna SK, and Das M

Subjects

9,10-Dimethyl-1,2-benzanthracene administration & dosage, 9,10-Dimethyl-1,2-benzanthracene toxicity, Administration, Topical, Aflatoxin B1 administration & dosage, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 toxicity, Animals, Anticarcinogenic Agents isolation & purification, Anticarcinogenic Agents therapeutic use, Carcinogens administration & dosage, Cocarcinogenesis, Female, Glutathione metabolism, Glutathione S-Transferase pi metabolism, HSP70 Heat-Shock Proteins metabolism, Interleukin-1beta blood, Interleukin-1beta drug effects, Lipid Peroxidation drug effects, Methylcholanthrene administration & dosage, Methylcholanthrene toxicity, Mice, Ornithine Decarboxylase metabolism, Plant Extracts isolation & purification, Plant Extracts therapeutic use, Plant Leaves chemistry, Skin metabolism, Skin pathology, Skin Neoplasms blood, Skin Neoplasms chemically induced, Tetradecanoylphorbol Acetate administration & dosage, Tetradecanoylphorbol Acetate toxicity, Tumor Necrosis Factor-alpha blood, gamma-Glutamyltransferase metabolism, Anticarcinogenic Agents pharmacology, Carcinogens toxicity, Ocimum chemistry, Plant Extracts pharmacology, Skin drug effects, Skin Neoplasms prevention & control

Abstract

A study on the protective effect of alcoholic extract of the leaves of Ocimum sanctum on 3-methylcholanthrene (MCA), 7,12-dimethylbenzanthracene (DMBA) and aflatoxin B1 (AFB1) induced skin tumorigenesis in a mouse model has been investigated. The study involved pretreatment of mice with the leaf extract prior to either MCA application or tetradecanoyl phorbol acetate (TPA) treatment in a two-stage tumor protocol viz a viz, DMBA/TPA and AFB1/TPA. The results of the present study indicate that the pretreatment with alcoholic extract of the leaves of O. sanctum decreased the number of tumors in MCA, DMBA/TPA and AFB1/TPA treated mice. The skin tumor induced animals pretreated with alcoholic extract led to a decrease in the expression of cutaneous gamma-glutamyl transpeptidase (GGT) and glutathione-S-transferase-P (GST-P) protein. The histopathological examination of skin tumors treated with leaf extract showed increased infiltration of polymorphonuclear, mononuclear and lymphocytic cells, decreased ornithine decarboxylase activity with concomitant enhancement of interleukin-1beta (IL-1beta) and tumor necrosis factor-alpha (TNF-alpha) in the serum, implying the in vivo antiproliferative and immunomodulatory activity of leaf extract. The decrease in cutaneous phase I enzymes and elevation of phase II enzymes in response to topical application of leaf extract prior to MCA, AFB1, DMBA/TPA and AFB1/TPA treatment indicate the possibility of impairment in reactive metabolite(s) formation and thereby reducing skin carcinogenicity. Furthermore, pretreatment of leaf extract in the carcinogen induced animals resulted in elevation of glutathione levels and decrease in lipid peroxidation along with heat shock protein expression, indicating a scavenging or antioxidant potential of the extract during chemical carcinogenesis. Thus it can be concluded that leaf extract of O. sanctum provides protection against chemical carcinogenesis in one or more of the following mechanisms: (i) by acting as an antioxidant; (ii) by modulating phase I and II enzymes; (iii) by exhibiting antiproliferative activity.

Published

2007

21. Hydroxyl-specific fluorescence labeling of ABP-deoxyguanosine, PhIP-deoxyguanosine, and AFB1-formamidopyrimidine with BODIPY-FL.

Author

Jang HG, Park M, Wishnok JS, Tannenbaum SR, and Wogan GN

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, Aminobiphenyl Compounds chemistry, Animals, Biomarkers analysis, Carcinogens chemistry, Carcinogens isolation & purification, DNA Adducts chemistry, Imidazoles, Indicators and Reagents, Mutagens chemistry, Mutagens isolation & purification, Pyrimidines isolation & purification, Sensitivity and Specificity, Aflatoxin B1 isolation & purification, Boron Compounds chemistry, DNA Adducts isolation & purification, Deoxyguanosine analogs & derivatives, Environmental Exposure analysis, Fluorescent Dyes chemistry

Abstract

Detection and analysis of DNA adducts resulting from endogenous or exogenous exposures to carcinogens are essential not only for quantifying biologically effective doses but also for establishing relationships between exposure and cancer risk. We have developed and validated a procedure of high sensitivity and specificity based on fluorescence labeling of DNA adducts combined with high-performance liquid chromatography-laser-induced fluorescence detection. The fluorescent dye 4,4-difluoro-5,7-dimethyl-4-bora-3a,4a-diaza-s-indacene-3-propionic acid (BODIPY FL) was used to label the deoxynucleoside adducts N-(2'-deoxyguanosine-8-yl)-4-aminobiphenyl and N-(2'-deoxyguanosine-8-yl)-2-amino-1-methyl-6-phenylimidazo[4,5-b]pyridine and the base adduct aflatoxin B(1)-formamidopyrimidine by acylation. The labeling reaction was carried out on adducts at 1pmol to 30nmol concentrations at 25 degrees C for 4h in dichloromethane with 200- to 5000-fold excess of BODIPY FL. BODIPY FL and its activating agents 1,3-dicyclohexylcarbodiimide and 4-dimethylaminopyridine were used at a molar ratio of 1:2:2. Under these conditions, all of the above adducts were quantitatively converted to bis-labeled products, as confirmed by mass spectrometry. Sites of derivatization of adduct deoxynucleosides were established primarily by nuclear magnetic resonance and by collision-induced dissociation mass spectrometric analysis, which indicated that the bis-BODIPY groups were located predominantely on the 3'- and 5'-hydroxyl groups of the deoxyribose ring.

Published

2006

22. Quantification of aflatoxin-B1-N7-Guanine in human urine by high-performance liquid chromatography and isotope dilution tandem mass spectrometry.

Author

Egner PA, Groopman JD, Wang JS, Kensler TW, and Friesen MD

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 urine, Guanine analogs & derivatives, Guanine urine, Humans, Reproducibility of Results, Sensitivity and Specificity, Chromatography, High Pressure Liquid methods, Mass Spectrometry methods

Abstract

We report validation of the first isotope dilution mass spectrometry method for determination of aflatoxin B(1)-N(7)-guanine (AFB(1)-N(7)-Gua), a major human aflatoxin-DNA adduct that is excreted in the urine. Measurement of urinary AFB(1)-N(7)-Gua, a biomarker of the biologically effective dose following dietary aflatoxin B(1) (AFB(1)) exposure, has helped identify AFB(1) as a risk factor in the development of hepatocellular carcinoma, a common cancer worldwide. Triple-quadrupole mass spectrometry, coupled with the use of a stable isotope-labeled internal standard (AFB(1)-N(7)-(15)N(5)-Gua) and better solid phase extraction and immunoaffinity column chromatography, have enabled us to greatly improve accuracy, precision, specificity, and sensitivity over previously published determinations. The limit of quantitation for AFB(1)-N(7)-Gua was 0.8 pg/20 mL urine (0.07 pg/mg creatinine). The method was validated for accuracy and precision over the range of 0.8-25 pg/20 mL urine, with between-day and within-day reproducibility for analysis of six aliquots of a human urine sample containing 6.0 pg/20 mL measured at <6% coefficient of variation. AFB(1)-N(7)-Gua concentrations were measured in 20 human urine samples collected in a region with known aflatoxin exposure. The mean concentration of AFB(1)-N(7)-Gua, measured in 16/20 urine samples with levels above the method's limit of quantitation, was 2.9 pg/20 mL urine (0.28 pg/mg creatinine) with a range of <0.8-7.2 pg/20 mL urine (0.04-65 pg/mg creatinine). With improved accuracy and precision, this sensitive biomarker for recent human exposure to AFB(1) will be especially useful for measuring the efficacy of planned interventions to reduce aflatoxin-related liver cancer in AFB(1)-exposed populations.

Published

2006

23. Probiotic supplementation reduces a biomarker for increased risk of liver cancer in young men from Southern China.

Author

El-Nezami HS, Polychronaki NN, Ma J, Zhu H, Ling W, Salminen EK, Juvonen RO, Salminen SJ, Poussa T, and Mykkänen HM

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 pharmacokinetics, Aflatoxin B1 toxicity, Aflatoxin B1 urine, Carcinoma, Hepatocellular chemically induced, Carcinoma, Hepatocellular prevention & control, China, DNA Adducts urine, Double-Blind Method, Guanine analogs & derivatives, Guanine urine, Humans, Lacticaseibacillus rhamnosus, Liver Neoplasms chemically induced, Liver Neoplasms urine, Placebos, Propionibacterium, Risk Factors, Biomarkers, Tumor urine, Liver Neoplasms prevention & control, Probiotics administration & dosage

Abstract

Background: In vitro and in vivo studies suggest that selected strains of probiotic bacteria can form tight complexes with aflatoxin B(1) and other carcinogens., Objective: The aim of the present study was to determine whether administration of probiotic bacteria could block the intestinal absorption of aflatoxin B(1) and thereby lead to reduced urinary excretion of aflatoxin B(1)-N(7)-guanine (AFB-N(7)-guanine), a marker for a biologically effective dose of aflatoxin exposure. Elevated urinary excretion of this aflatoxin-DNA adduct is associated with an increased risk of liver cancer., Design: Ninety healthy young men from Guangzhou, China, were randomly assigned to 2 groups; one group received a mixture of Lactobacillus rhamnosus LC705 and Propionibacterium freudenreichii subsp. shermanii strains 2 times/d for 5 wk, and the other group received a placebo preparation. The subjects provided 4 urine samples: at baseline, at 3 and 5 wk after starting the supplementation, and at the end of the 5-wk postintervention period., Results: The percentage of samples with negative AFB-N(7)-guanine values tended to be higher in the probiotic group than in the placebo group during the 5-wk intervention period (odds ratio: 2.63, P = 0.052), and a statistically significant decrease in the concentration of urinary AFB-N(7)-guanine was observed in the probiotic group. The reduction was 36% at week 3 and 55% at week 5. The geometric means for the probiotic and placebo groups were 0.24 and 0.49 ng AFB-N(7)-guanine/mL, respectively, during the intervention period (P = 0.005)., Conclusion: A probiotic supplement reduces the biologically effective dose of aflatoxin exposure and may thereby offer an effective dietary approach to decrease the risk of liver cancer.

Published

2006

24. Fecal and urinary excretion of aflatoxin B1 metabolites (AFQ1, AFM1 and AFB-N7-guanine) in young Chinese males.

Author

Mykkänen H, Zhu H, Salminen E, Juvonen RO, Ling W, Ma J, Polychronaki N, Kemiläinen H, Mykkänen O, Salminen S, and El-Nezami H

Subjects

Aflatoxin M1 urine, Aflatoxins urine, China, Feces chemistry, Guanine urine, Hepatitis B complications, Hepatitis B urine, Humans, Male, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Aflatoxin B1 urine, Guanine analogs & derivatives

Abstract

Our study was designed to assess the fecal and urinary excretion of 3 aflatoxin B1 (AFB1) metabolites, aflatoxins M1 (AFM1) and Q1 (AFQ1) and aflatoxin B1-N7-guanine (AFB-N7-guanine) that are produced by the predominant forms of cytochrome P450 enzymes responsible for the biotransformation of AFB1. Fecal and urinary AFM1, AFQ1 and urinary AFB-N7-guanine were assessed in 83 young Chinese males selected from a larger population (n = 300) based on detectable urinary AFM1. The concentration of fecal AFQ1 (median 137 ng/g fresh weight, IQR 9.1 to 450) was approximately 60 times higher than that of AFM1 (2.3 ng/g, IQR 0.0 to 7.3). In urine, the median AFQ1 was 10.4 ng/ml (IQR 3.4 to 23.3), and the median AFM1 and AFB-N7-guanine 0.04 ng/ml (IQR 0.01 to 0.33) and 0.38 ng/ml (IQR 0.0 to 2.15), respectively. A subgroup (n = 14) with hepatitis B virus (HBV) infection had significantly higher fecal concentrations of AFQ1 (p = 0.043) and AFM1 (p = 0.001) than those who were hepatitis B-virus antigen (HBsAg) negative, and the respective differences in urinary AFQ1 and AFM1 concentrations approached statistical significance (p = 0.054, p = 0.138). Our study demonstrates that AFQ1 is excreted in urine and feces at higher levels than AFM1, and feces are an important route of excretion of these AFB1 metabolites. AFQ1 should be further assessed for its predictive value as a marker for exposure and risk of dietary aflatoxins., (Copyright 2005 Wiley-Liss, Inc.)

Published

2005

25. Susceptibility to aflatoxin B1-induced carcinogenesis correlates with tissue-specific differences in DNA repair activity in mouse and in rat.

Author

Bedard LL, Alessi M, Davey S, and Massey TE

Subjects

Aflatoxin B1 metabolism, Animals, Carcinogens toxicity, DNA drug effects, DNA metabolism, Female, Genetic Predisposition to Disease, Guanine metabolism, Liver drug effects, Liver metabolism, Liver physiology, Liver Neoplasms metabolism, Lung drug effects, Lung metabolism, Lung physiology, Lung Neoplasms metabolism, Male, Mice, Pyrimidines metabolism, Rats, Rats, Sprague-Dawley, Species Specificity, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 toxicity, Cocarcinogenesis, DNA Repair physiology, Guanine analogs & derivatives, Liver Neoplasms chemically induced, Liver Neoplasms genetics, Lung Neoplasms chemically induced, Lung Neoplasms genetics

Abstract

To investigate the mechanisms responsible for species- and tissue-specific differences in susceptibility to aflatoxin B(1) (AFB(1))-induced carcinogenesis, DNA repair activities of nuclear extracts from whole mouse lung and liver and rat liver were compared, and the ability of in vivo treatment of mice with AFB(1) to alter repair of AFB(1)-DNA damage was determined. Plasmid DNA containing AFB(1)-N(7)-guanine or AFB(1)-formamidopyrimidine adducts were used as substrates for the in vitro determination of DNA repair synthesis activity, detected as incorporation of radiolabeled nucleotides. Liver extracts from CD-1 mice repaired AFB(1)-N(7)-guanine and AFB(1)-formamidopyrimidine adducts 5- and 30-fold more effectively than did mouse lung, and approximately 6- and 4-fold more effectively than did liver extracts from Sprague-Dawley rats. The susceptibility of mouse lung and rat liver to AFB(1)-induced carcinogenesis correlated with lower DNA repair activity of these tissues relative to mouse liver. Lung extracts prepared from mice treated with a single tumorigenic dose of 50 mg/kg AFB(1) i.p. and euthanized 2 hours post-dosing showed minimal incision and repair synthesis activities relative to extracts from vehicle-treated mice. Conversely, repair activity towards AFB(1)-N(7)-guanine damage was approximately 3.5-fold higher in liver of AFB(1)-treated mice relative to control. This is the first study to show that in vivo treatment with AFB(1) can lead to a tissue-specific induction in DNA repair. The results suggest that lower DNA repair activity, sensitivity of mouse lung to inhibition by AFB(1), and selective induction of repair in liver contribute to the susceptibility of mice to AFB(1)-induced lung tumorigenesis relative to hepatocarcinogenesis.

Published

2005

26. Interactions of aflatoxin B1 with SRP components can disrupt protein targeting.

Author

Singh J, Singh S, Dani HM, Sharma R, and Steinberg P

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 pharmacology, Animals, Dogs, Endoplasmic Reticulum metabolism, Genetic Engineering, Humans, Pancreas chemistry, Peptides genetics, Peptides isolation & purification, Peptides metabolism, Protein Transport drug effects, Ribosomes metabolism, Signal Recognition Particle drug effects, Signal Recognition Particle genetics, Spectrometry, Fluorescence methods, Aflatoxin B1 metabolism, Proteins metabolism, Signal Recognition Particle metabolism

Abstract

Spectrofluorimetric studies have revealed that aflatoxin B1 (AFB1) interacts with signal recognition particle (SRP), which acts as an escort for polyribosomes with signal peptides to be transported and bound to the cytoplasmic face of the endoplasmic reticulum (ER). We further report that the binding of AFB1 to SRP is selective as it only binds to two (SRP9 and 14) out of its three constituent polypeptides studied. Binding of AFB1 to proteins is known to alter their conformations. Interactions of AFB1 with SRP polypeptides may generate structural and functional alterations in this particle and hinder secretory protein synthesis.

Published

2005

27. Increased levels of aflatoxin-albumin adducts are associated with CYP3A5 polymorphisms in The Gambia, West Africa.

Author

Wojnowski L, Turner PC, Pedersen B, Hustert E, Brockmöller J, Mendy M, Whittle HC, Kirk G, and Wild CP

Subjects

Adolescent, Adult, Aflatoxin B1 blood, Aflatoxins toxicity, Aged, Albumins, Base Sequence, Carcinoma, Hepatocellular etiology, Child, Cytochrome P-450 CYP3A, DNA genetics, Female, Gambia, Gene Expression, Gene Frequency, Genetic Variation, Haplotypes, Humans, Liver Neoplasms etiology, Male, Middle Aged, Mutagens metabolism, Risk Factors, Aflatoxin B1 analogs & derivatives, Aflatoxins blood, Cytochrome P-450 Enzyme System genetics, Polymorphism, Genetic

Abstract

Objectives: Major risk factors for hepatocellular carcinoma (HCC) are hepatitis viruses and exposure to aflatoxins, including aflatoxin B1 (AFB1). The mutagenic effect of AFB1 results from hepatic bioactivation to AFB1-exo-8,9-epoxide. This is in part catalysed by CYP3A5, an enzyme expressed polymorphically. We investigated the role of CYP3A5 polymorphisms in the formation of AFB1-exo-8,9-epoxide in The Gambia, a population exposed to high aflatoxin levels., Methods: Common CYP3A5 polymorphisms were identified in an African-American population. Subsequently, 288 Gambian subjects were genotyped and CYP3A5 activity predicted using haplotypes of the three variant loci (CYP3A5*3, *6 and *7) associated with decreases in protein expression. CYP3A5 expression was then compared to aflatoxin-albumin (AF-alb) adduct, a biomarker of AFB1 bioactivation; data were also analysed in relation to expression of other aflatoxin-metabolizing enzymes., Results: CYP3A5 haplotypes reflecting high CYP3A5 protein expression were associated with increased AF-alb. Compared to individuals with predicted low expression those predicted to express CYP3A5 from one allele displayed 16.1% higher AF-alb (95% CI: -2.5, 38.2, P = 0.093) and homozygous expressers displayed 23.2% higher AF-alb levels (95% CI: -0.01, 52.0, P = 0.051). The effect of the CYP3A5 polymorphism was strongest in individuals with low CYP3A4 activity with a 70.1% increase in AF-alb (95% CI: 11.8, 158.7, P < 0.05) in high compared to low expressers. A similar effect was observed for individuals with null alleles of GSTM1, which conjugates the AFB1-exo-8,9-epoxide to reduced glutathione., Conclusions: The CYP3A5 polymorphism is associated with increased levels of the mutagenic AFB1-exo-8,9-epoxide, particularly in individuals with low CYP3A4, and this may modulate individual risk of HCC.

Published

2004

28. Expression of the aflatoxin B1-8,9-epoxide-metabolizing murine glutathione S-transferase A3 subunit is regulated by the Nrf2 transcription factor through an antioxidant response element.

Author

Jowsey IR, Jiang Q, Itoh K, Yamamoto M, and Hayes JD

Subjects

Animals, Base Sequence, Chromosome Mapping, DNA analysis, Exons, Glutathione Transferase genetics, Isothiocyanates, Mice, Molecular Sequence Data, NF-E2-Related Factor 2, Protein Subunits genetics, Protein Subunits metabolism, Regulatory Sequences, Nucleic Acid genetics, Response Elements, Sequence Homology, Nucleic Acid, Sulfoxides, Tumor Cells, Cultured, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Antioxidants pharmacology, DNA-Binding Proteins physiology, Gene Expression Regulation, Enzymologic drug effects, Glutathione Transferase metabolism, Thiocyanates pharmacology, Trans-Activators physiology

Abstract

High expression of the aflatoxin B1 (AFB1)-8,9-epoxide-conjugating glutathione S-transferase A3 (mGSTA3) subunit in mouse liver confers intrinsic resistance to AFB1 hepatocarcinogenesis. It is not known how the gene encoding this protein is regulated. The murine mGSTA3 gene has been identified using bioinformatics. It localizes to mouse chromosome 1 (A3-4), spans approximately 24.6 kilobases (kb) of DNA, and comprises seven exons. High levels of mGSTA3 mRNA are present in organs associated with detoxification. Expression of mGSTA3 in Hepa1c1c7 mouse hepatoma cells was found to be inducible by sulforaphane, an organic isothiocyanate that can transcriptionally activate genes through the antioxidant response element (ARE). Sulforaphane also induced transcription of a luciferase reporter containing a 1.5 kb fragment of the mGSTA3 5'-upstream region. A putative ARE, with sequence 5'-TGACATTGC-3', was identified within this fragment, approximately 150 base pairs upstream of exon 1. Mutation of this sequence abrogated both basal and sulforaphane-inducible reporter activity. Overexpression of the basic-region leucine zipper Nrf2 transcription factor augmented activity of the mGSTA3-luciferase reporter through this ARE. Electrophoretic mobility shift assays demonstrated that Nrf2 binds the mGSTA3 ARE. Measurement of mGSTA3 mRNA levels in tissues isolated from both wild-type and nrf2-null mice revealed that loss of the Nrf2 transcription factor is associated with a reduction in basal expression of mGSTA3. Collectively, these data demonstrate a role for Nrf2 and the ARE in regulating transcription of mGSTA3.

Published

2003

29. Preferential carcinogen-DNA adduct formation at codons 12 and 14 in the human K-ras gene and their possible mechanisms.

Author

Hu W, Feng Z, and Tang MS

Subjects

7,8-Dihydro-7,8-dihydroxybenzo(a)pyrene 9,10-oxide toxicity, Aflatoxin B1 toxicity, Bronchi drug effects, Bronchi metabolism, Cells, Cultured, CpG Islands, Cytosine chemistry, DNA genetics, DNA Damage drug effects, DNA Methylation, Endodeoxyribonucleases metabolism, Epithelial Cells drug effects, Escherichia coli Proteins metabolism, Exons, Fluorenes toxicity, Humans, Mutation genetics, Aflatoxin B1 analogs & derivatives, Carcinogens toxicity, Codon genetics, Cytosine metabolism, DNA Adducts metabolism, Genes, ras

Abstract

In the ras gene superfamily, codon 12 (-TGGTG-) of the K-ras gene is the most frequently mutated codon in human cancers. Recently, we have found that bulky chemical carcinogens preferentially form DNA adducts at codons 12 and 14 (-CGTAG-) in the K-ras gene in normal human bronchial epithelial (NHBE) cells. Furthermore, DNA adducts formed at codon 12 of the K-ras gene are poorly repaired compared with those at other codons including codon 14. These results suggest that targeted carcinogen-DNA adduct formation is a major reason for the observed high mutation frequency at codon 12 of the K-ras gene in human cancers. This preferential carcinogen-DNA adduct formation at codons 12 and 14 could result from effects of (1) primary sequences of these codons and their surrounding codons in the K-ras gene, (2) the chromatin structure, and/or (3) epigenetic factors such as C5 cytosine methylation or other DNA modifications at these codons and their surrounding codons. To distinguish these possibilities, we have introduced modifications with benzo[a]pyrene diol epoxide, N-hydroxy-2-aminofluorene, and aflatoxin B1 8,9-epoxide in (1) naked intact genomic DNA isolated from NHBE cells, (2) fragmented genomic DNA digested by restriction enzymes, and (3) in vitro synthesized DNA fragments containing the K-ras gene exon 1 sequence with or without methylation of the cytosines at CpG sites and the cytosines pairing with the guanines of codons 12 and 14. The distribution of carcinogen-DNA adducts in the K-ras gene was mapped at the nucleotide sequence level using the UvrABC nuclease incision method with or without the ligation-mediated polymerase chain reaction technique. We have found that carcinogens preferentially form adducts at codons 12 and 14 in the K-ras gene exon 1 in intact as well as in fragmented genomic DNA. In contrast, this preferential DNA adduct formation at codons 12 and 14 was not observed in PCR-amplified DNA fragments containing the K-ras gene exon 1 sequence. Methylation of the cytosine at the CpG site of codon 14, or the cytosine pairing with guanine of codon 14, greatly enhanced carcinogen-DNA adduct formation at codon 14 but did not affect carcinogen-DNA adduct formation at codon 12. Methylation of the cytosine pairing with the guanine of codon 12 also did not enhance carcinogen-DNA adduct formation at codon 12. Furthermore, we found that the cytosine at the CpG site of codon 14 is highly methylated in NHBE cells. These results suggest that cytosine methylation at the CpG site is the major reason for the preferential DNA damage at codon 14 and that epigenetic modification(s) other than cytosine methylation may contribute to the preferential DNA damage at codon 12 of the K-ras gene.

Published

2003

30. Wobble dC.dA pairing 5' to the cationic guanine N7 8,9-dihydro-8-(N7-guanyl)-9-hydroxyaflatoxin B1 adduct: implications for nontargeted AFB1 mutagenesis.

Author

Giri I and Stone MP

Subjects

Base Composition, Base Sequence, Cations, Deoxyadenine Nucleotides chemistry, Deoxycytosine Nucleotides chemistry, Hydrogen-Ion Concentration, Intercalating Agents chemistry, Models, Molecular, Nuclear Magnetic Resonance, Biomolecular, Nucleic Acid Conformation, Nucleic Acid Heteroduplexes chemistry, Oligodeoxyribonucleotides chemistry, Protons, Structure-Activity Relationship, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, Base Pair Mismatch, DNA Adducts chemistry, Guanine analogs & derivatives, Guanine chemistry

Abstract

The structure of 5'-d(ACATC(AFB)GATCT)-3'.5'-d(AGATCAATGT)-3', containing the C(5).A(16) mismatch at the base pair 5' to the modified (AFB)G(6), was determined by NMR. The characteristic 5'-intercalation of the AFB(1) moiety was maintained. The mismatched C(5).A(16) pair existed in the wobble conformation, with the C(5) imino nitrogen hydrogen bonded to the A(16) exocyclic amino group. The wobble pair existed as a mixture of protonated and nonprotonated species. The pK(a) for protonation at the A(16) imino nitrogen was similar to that of the C(5).A(16) wobble pair in the corresponding duplex not adducted with AFB(1). Overall, the presence of AFB(1) did not interfere with wobble pair formation at the mismatched site. Molecular dynamics calculations restrained by distances derived from NOE data and torsion angles derived from (1)H (3)J couplings were carried out for both the protonated and nonprotonated wobble pairs at C(5).A(16). Both sets of calculations predicted the A(16) amino group was within 3 A of the C(5) imino nitrogen. The calculations suggested that protonation of the C(5).A(16) wobble pair should shift C(5) toward the major groove and shift A(16) toward the minor groove. The NMR data showed evidence for the presence of a minor conformation characterized by unusual NOEs between T(4) and (AFB)G(6). T(4) is two nucleotides in the 5'-direction from the modified base. These NOEs suggested that in the minor conformation nucleotide T(4) was in closer proximity to (AFB)G(6) than would be expected for duplex DNA. Modeling studies examined the possibility that T(4) transiently paired with the mismatched A(16), allowing it to come within NOE distance of (AFB)G(6). This model structure was consistent with the unusual NOEs associated with the minor conformation. The structural studies are discussed in relationship to nontargeted C --> T transitions observed 5' to the modified (AFB)G in site-specific mutagenesis experiments [Bailey, E. A., Iyer, R. S., Stone, M. P., Harris, T. M., and Essigmann, J. M. (1996) Proc. Natl. Acad. Sci. U.S.A. 93, 1535-1539].

Published

2003

31. Thermal stabilization of the DNA duplex by adducts of aflatoxin B1.

Author

Giri I and Stone MP

Subjects

Base Sequence, Cations chemistry, Magnetic Resonance Spectroscopy, Models, Molecular, Nucleic Acid Conformation, Thermodynamics, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, DNA chemistry, DNA Adducts chemistry

Abstract

The trans-8,9-dihydro-8-(N7-guanyl)-9-hydroxyaflatoxin B(1) cationic guanine N7 adduct of aflatoxin B(1) thermally stabilizes the DNA duplex, as reflected in increased T(m) values upon adduction. The magnitude of the increased T(m) value is characteristically 2-3 degrees C. The major rotamer of the neutral guanine N7 adduct trans-8,9-dihydro-8-(2,6-diamino-4-oxo-3,4-dihydropyrimid-5-yl-formamido)-9-hydroxy aflatoxin B(1) (the FAPY major adduct) exhibits a 15 degrees C increase in T(m) in 5'-d(CTAT(FAPY)GATTCA)-3'-5'-d(TGAATCATAG)-3'. Site-specific mutagenesis experiments reveal the FAPY major adduct induces G-->T mutations in Escherichia coli at a frequency six times higher than that of the cationic adduct (Smela, M. E.; Hamm, M. L.; Henderson, P. T.; Harris, C. M.; Harris, T. M.; Essigmann, J. M. Proc Natl Acad Sci USA, 99, 6655-6660). Thus, the FAPY major lesion may account substantially for the genotoxicity of AFB(1). Structural studies for cationic and FAPY adducts of aflatoxin B(1) suggest both adducts intercalate above the 5'-face of the modified deoxyguanosine and that in each instance the aflatoxin moiety spans the DNA helix. Intercalation of the aflatoxin moiety, accompanied by favorable stacking with the neighboring base pairs, is thought to account for the increased thermal stability of the aflatoxin cationic guanine N7 and the FAPY major adducts. However, the structural basis for the large increase in thermal stability of the FAPY major adduct in comparison to the cationic guanine N7 adduct of aflatoxin B(1) is not well understood. In light of the site-specific mutagenesis studies, it is of considerable interest. For both adducts, the intercalation structures are similar, although improved stacking with neighboring base pairs is observed for the FAPY major adduct. In addition, the presence of the formamido group in the aflatoxin B(1) FAPY major adduct may enhance duplex stability, perhaps via intrastrand sequence-specific hydrogen bonding interactions within the duplex., (Copyright 2002 Wiley Periodicals, Inc. Biopolymers (Nucleic Acid Sci) 65: 190-201, 2002)

Published

2002

32. Comparison of nixtamalization and extrusion processes for a reduction in aflatoxin content.

Author

Elias-Orozco R, Castellanos-Nava A, Gaytán-Martínez M, Figueroa-Cárdenas JD, and Loarca-Piña G

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 analysis, Calcium Compounds, Carcinogens analysis, Environmental Exposure, Food, Fortified analysis, Humans, Hydrogen Peroxide, Mexico, Oxides, Aflatoxins analysis, Cooking methods, Zea mays chemistry

Abstract

Traditional nixtamalization and an extrusion method for making the dough (masa) for corn tortillas that requires using lime and hydrogen peroxide were evaluated for the detoxification of aflatoxins. The traditional nixtamalization process reduced levels of aflatoxin B(1) (AFB(1)) by 94%, aflatoxin M(1) (AFM(1)) by 90% and aflatoxin B(1)-8,9-dihydrodiol (AFB(1)-dihydrodiol) by 93%. The extrusion process reduced levels of AFB(1) by 46%, AFM(1) by 20% and AFB(1)-dihydrodiol by 53%. Extrusion treatments with 0, 0.3 and 0.5% lime reduced AFB(1) levels by 46, 74 and 85%, respectively. The inactivation of AFB(1), AFM(1) and AFB(1)-dihydrodiol in the extrusion process using lime together with hydrogen peroxide showed higher elimination of AFB(1) than treatments with lime or hydrogen peroxide alone. The extrusion process with 0.3% lime and 1.5% hydrogen peroxide was the most effective process to detoxify aflatoxins in corn tortillas, but a high level of those reagents negatively affected the taste and aroma of the corn tortilla as compared with tortillas elaborated by the traditional nixtamalization process.

Published

2002

33. Glutathione-S-transferase activity toward aflatoxin epoxide in livers of mastomys and other rodents.

Author

Esaki H and Kumagai S

Subjects

Animals, Cricetinae, Cytosol enzymology, DNA metabolism, Mesocricetus, Mice, Mice, Inbred ICR, Microsomes, Liver enzymology, Rats, Rats, Inbred F344, Species Specificity, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Carcinogens metabolism, Glutathione Transferase metabolism, Liver enzymology, Muridae metabolism

Abstract

In order to study the liver glutathione-S-transferase (GST) activity toward aflatoxin B1 (AFB1) epoxide in mastomys in comparison with other rodents, we performed in vitro studies of the cytosolic GST activity toward AFB1-epoxide using mastomys, rat, mouse and hamster liver. Also AFB1 metabolism by liver microsomes including formation of AFB1-DNA adducts was studied. Cytosolic GST activity toward AFB1-epoxide was highest in mastomys liver, and higher in the hamster and mouse livers than in the rat liver, correlating well with the differences of the sensitivity of these species to the toxicity of AFB1. However, no relationship was noted between the sensitivity of a given species to the toxicity of AFB1 and the microsomal activity of binding of AFB1 to DNA or metabolizing AFB1 to AFM1, AFQ1 and AFP1. These results demonstrate the importance of the GST mediated AFB1-epoxide conjugation with glutathione in determining the differing sensitivities of these species to AFB1 toxicity. The extremely high activity of GST in mastomys indicates that this species would be a good model animal for studying GST toward AFB1-epoxide.

Published

2002

34. Structure of the aflatoxin B(1) dialdehyde adduct formed from reaction with methylamine.

Author

Guengerich FP, Voehler M, Williams KM, Deng Z, and Harris TM

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemical synthesis, Aldehydes chemical synthesis, Aldehydes chemistry, Buffers, Chromatography, High Pressure Liquid, Cyclization, Hydrogen-Ion Concentration, Mass Spectrometry, Nuclear Magnetic Resonance, Biomolecular methods, Spectrometry, Fluorescence, Spectrophotometry, Ultraviolet, Aflatoxin B1 chemistry, Methylamines chemistry

Abstract

Amine conjugates of activated aflatoxin (AF) B(1) are formed in various systems, e.g., buffer amines and with protein lysine groups. Structures have been published in the literature, but the evidence is indirect in that (i) halogenated AFB(1) was usually used as the precursor and (ii) the assignment of the structure of the five-membered ring formed by cyclization is based on NMR chemical shifts. To better define these adducts and distinguish among several possibilities, we synthesized AFB(1) dialdehyde and reacted this with the surrogate methylamine at neutral pH, to simplify the system. The isolated product had the expected molecular ion (mass spectrometry) and showed pH-dependent UV spectra similar to those published for a lysine conjugate. Nuclear Overhauser enhanced spectroscopy (two-dimensional NMR, 800 MHz) of the sample (2H(2)O) showed proximity of the N-CH(3) protons only with a singlet at delta 4.10, assigned to the methylene of the added five-membered ring, but not to a delta 6.53 singlet assigned as the vinylic proton of that ring. All protons in the coumarin-furanone portion of the system were correlated to each other but not to those in the added five-membered ring. These experiments establish the structure as 2,3-dihydro-2-oxo-4-(1,2,3,4-tetrahydro-7-hydroxy-9-methoxy-3,4-dioxocyclopenta[c][1]benzopyran-6-yl)-1H-pyrrole-1-methane. The similarity of the reaction to that occurring in the reaction of AFB(1) dialdehyde with lysine and the agreement of the UV spectra suggest that this structure is applicable for the lysine analogue. The NMR results support the possible structure B of Sabbioni et al. [Sabbioni, G., Skipper, P. L., Buchi, G., and Tannenbaum, S. R. (1987) Carcinogenesis 8, 819-824] and the proposed structure 8 of Sabbioni [Sabbioni, G. (1990) Chem.-Biol. Interact. 75, 1-15] but not alternative proposals. Kinetic and mechanistic considerations of the reaction of lysine with AFB(1) dialdehyde are presented in the previous article in this issue [Guengerich, F. P., Arneson, K. O., Williams, K. M., Deng, Z., and Harris, T. M. (2002) Chem. Res. Toxicol. 15, 780-793].

Published

2002

35. Biochemical factors underlying the age-related sensitivity of turkeys to aflatoxin B(1).

Author

Klein PJ, Van Vleet TR, Hall JO, and Coulombe RA Jr

Subjects

Aflatoxin B1 analogs & derivatives, Age Factors, Aldehyde Reductase metabolism, Animals, Aryl Hydrocarbon Hydroxylases metabolism, Biotransformation, Blotting, Western, Chromatography, High Pressure Liquid methods, Cytosol enzymology, Epoxy Compounds chemistry, Epoxy Compounds metabolism, Glutathione Transferase metabolism, Isoenzymes metabolism, Kinetics, Male, Mice, Microsomes, Liver drug effects, Microsomes, Liver enzymology, Rats, Rats, Sprague-Dawley, Aflatoxin B1 pharmacokinetics, Aflatoxin B1 toxicity, Turkeys metabolism

Abstract

Poultry are some of the most sensitive species to the toxic effects of aflatoxin B(1) (AFB(1)), and younger poultry are more sensitive to this mycotoxin. To elucidate the mechanisms for this age-related susceptibility, various enzyme activities relevant to AFB(1) were measured in liver microsomes prepared from male turkeys 9, 41 and 65 days of age. Hepatic microsomal o-dealkylation of methoxy- and pentoxyresorufin significantly increased, while that of ethoxyresorufin decreased with age. Microsomal AFB(1) activation to the reactive AFB(1)-8,9-epoxide (AFBO) was most efficient in the youngest birds, with apparent K(m) and V(max) values of 168 and 19, 110 and 6, and 116 microM and 10 nmol/mg/min for 9, 41 and 65-day-old birds, respectively. The activity of hepatic cytosolic glutathione S-transferases (GSTs) was deficient in the youngest age group, but were higher in the older groups. There was also an age-related increase in the expression of GST isoforms Yc, Yc(2), as well as AFB(1)-aldehyde reductase (AFAR). However, livers from all ages lacked specific GST-mediated conjugation of AFBO, indicating that turkeys are deficient in this key AFB(1)-detoxification pathway. Our data indicate that efficient activation may underlie the extreme sensitivity of young turkeys to the toxic effects of AFB(1).

Published

2002

36. Reaction of aflatoxin B(1) oxidation products with lysine.

Author

Guengerich FP, Arneson KO, Williams KM, Deng Z, and Harris TM

Subjects

Aflatoxin B1 chemistry, Aldehydes chemistry, Aldehydes metabolism, Animals, Binding Sites, Binding, Competitive, Buffers, Cattle, Chromatography, High Pressure Liquid, Glutathione analogs & derivatives, Glutathione chemistry, Hydrogen-Ion Concentration, Kinetics, Lysine chemistry, Oxidation-Reduction, Serum Albumin metabolism, Serum Albumin, Bovine chemistry, Spectrometry, Mass, Electrospray Ionization, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Spectrophotometry, Ultraviolet, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Lysine analogs & derivatives, Lysine metabolism, Serum Albumin, Bovine metabolism

Abstract

Aflatoxin (AF) B(1) exo-8,9-epoxide hydrolysis yields AFB(1) dihydrodiol, which undergoes base-catalyzed rearrangement to, and is in equilibrium with, AFB(1) dialdehyde. We investigated the reaction of AFB(1) dialdehyde with albumin to generate a Lys adduct, previously characterized by others [Sabbioni, G., Skipper, P. L., Büchi, G., and Tannenbaum, S. R. (1987) Carcinogenesis8, 819-824; Sabbioni, G. (1990) Chem.-Biol. Interact. 75, 1-15]. Pronase digestion of bovine albumin serum treated with AFB(1) dialdehyde and HPLC yielded the adduct, identified by its characteristic UV and mass spectra. The structure of the Lys-AFB(1) dialdehyde adduct is concluded to be (S)-alpha-amino-2,3-dihydro-2-oxo-4-(1,2,3,4-tetrahydro-7-hydroxy-9-methoxy-3,4-dioxocyclopenta[c][1]benzopyran-6-yl)-1H-pyrrole-1-hexanoic acid, structure B of the former paper and 8 of the latter, based on work with the methylamine adduct described in the following paper in this issue [Guengerich, F. P., Voehler, M., Williams, K. M., Deng, Z., and Harris, T. M. (2002) Chem. Res. Toxicol. 15, 793-798]. The time course of product formation at varying concentrations of AFB(1) dialdehyde could be described by complexation with albumin with a K(d) of 1.5 mM and a first-order reaction rate with the N6-amino group of Lys of 0.033 min(-)(1). The reaction of AFB(1) dialdehyde with N(2)-acetylLys was monitored by UV spectroscopy and yielded a final spectrum similar to that of the described Lys adduct. Kinetic analysis of the changes at pH 7.2 was best described with a scheme involving equilibrium of the dialdehyde with dihydrodiol and a rate-limiting reaction of AFB(1) dialdehyde with the N6 atom of N(2)-acetylLys, with an apparent second-order rate constant of 2.6 x 10(3) M(-)(1) min(-)(1), followed by putative carbinolamine formation and rearrangement, collectively described by a first-order rate constant of 7.6 min(-)(1). Competition experiments with the hydrolysis of AFB(1) exo-8,9-epoxide indicate that N2-acetylLys also reacts with the epoxide at pH 7.2 (k = 350 M(-)(1) min(-)(1)) and 9.5 (k = 1.8 x 10(3) M(-)(1) min(-)(1)). This reaction might contribute to the formation of protein Lys adducts, depending upon the local concentration of free or protein Lys. Mass spectral analysis of trypsin digests of bovine serum albumin modified with AFB(1) dialdehyde indicated selective modification of Lys455 and Lys548. Collectively, these results provide more insight into the mechanism of formation of AFB(1) dialdehyde-protein adducts and indicate that the formation of Lys adducts is a moderately efficient process. The binding of AFB(1) dialdehyde to albumin or the protonation of the N6-amino group retards the reaction with Lys residues.

Published

2002

37. The aflatoxin B(1) formamidopyrimidine adduct plays a major role in causing the types of mutations observed in human hepatocellular carcinoma.

Author

Smela ME, Hamm ML, Henderson PT, Harris CM, Harris TM, and Essigmann JM

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 chemistry, Bacteriophage M13 genetics, DNA, Viral drug effects, Guanine analogs & derivatives, Guanine pharmacology, Humans, Molecular Structure, Mutagenesis, Mutagens chemistry, Pyrimidines chemistry, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Aflatoxin B1 genetics, Aflatoxin B1 pharmacology, Carcinoma, Hepatocellular genetics, DNA Adducts genetics, DNA, Neoplasm, Liver Neoplasms genetics, Mutagens pharmacology, Pyrimidines pharmacology

Abstract

A G to T mutation has been observed at the third position of codon 249 of the p53 tumor-suppressor gene in over 50% of the hepatocellular carcinoma cases associated with high exposure to aflatoxin B(1) (AFB(1)). Hypotheses have been put forth that AFB(1), in concert with hepatitis B virus (HBV), may play a role in the formation of, and/or the selection for, this mutation. The primary DNA adduct of AFB(1) is 8,9-dihydro-8-(N(7)-guanyl)-9-hydroxyaflatoxin B(1) (AFB(1)-N7-Gua), which is converted naturally to two secondary lesions, an apurinic site and an AFB(1)-formamidopyrimidine (AFB(1)-FAPY) adduct. AFB(1)-FAPY is detected at near maximal levels in rat DNA days to weeks after AFB(1) exposure, underscoring its high persistence in vivo. The present study reveals two striking properties of this DNA adduct: (i) AFB(1)-FAPY was found to cause a G to T mutation frequency in Escherichia coli approximately 6 times higher than that of AFB(1)-N7-Gua, and (ii) one proposed rotamer of AFB(1)-FAPY is a block to replication, even when the efficient bypass polymerase MucAB is used by the cell. Taken together, these characteristics make the FAPY adduct the prime candidate for both the genotoxicity of aflatoxin, because mammalian cells also have similar bypass mechanisms for combating DNA damage, and the mutagenicity that ultimately may lead to liver cancer.

Published

2002

38. Structural refinement of the 8,9-dihydro-8-(N7-guanyl)-9-hydroxy-aflatoxin B(1) adduct in a 5'-Cp(AFB)G-3' sequence.

Author

Giri I, Jenkins MD, Schnetz-Boutaud NC, and Stone MP

Subjects

Aflatoxin B1 analogs & derivatives, Molecular Conformation, Oligodeoxyribonucleotides chemical synthesis, Stereoisomerism, Structure-Activity Relationship, Aflatoxin B1 chemistry, Models, Molecular, Oligodeoxyribonucleotides chemistry

Abstract

The structure of the cationic 8,9-dihydro-8-(N7-guanyl)-9-hydroxy-aflatoxin B(1) adduct embedded in a 5'-CpG-3' sequence context and paired with deoxycytosine in the oligodeoxynucleotide d(ACATC(AFB)GATCT) x d(AGATCGATGT) was refined using molecular dynamics calculations restrained by NOE data and dihedral angle restraints obtained from NMR data. The aflatoxin moiety intercalated above the 5' face of the modified guanine. It stacked between C(5) x G(16) and (AFB)G(6) x C(15). The AFB(1) H5, OCH(3), and methylene protons faced into the minor groove, with the methylene protons oriented between the C(15) and G(16) nucleobases. The aflatoxin B(1) H6a, H8, H9, and H9a protons faced the major groove, with H6a and H9a pointing toward the 5' direction from the lesion site. The refined structure was compared to the structure of the aflatoxin B(1) adduct embedded in a 5'-ATGCAT-3' sequence in the oligodeoxynucleotide d(TAT(AFB)GCATA)(2) [Jones, W. R., Johnston, D. S., and Stone, M. P. (1998) Chem. Res. Toxicol.11, 873-881]. The structure of the intercalated aflatoxin B(1) lesion in the ATC(AFB)GAT sequence is similar to its structure in the d(AT(AFB)GCAT) sequence. This is consistent with a mechanism in which the precovalent intercalation of aflatoxin-8,9-exo-epoxide on the 5' face of guanine places the epoxide in close proximity and in the proper orientation to the N7 position of guanine, thus facilitating an S(N)2 reaction. The data provides additional insight into the nature of the disruption of the B-DNA duplex induced by aflatoxin B(1) intercalation. Overall, the results suggest that sequence contributes a minor role in modulating the structure of the cationic guanine N7 AFB(1) lesion in duplex DNA. On the other hand, structural differences are observed when the correctly paired structure is compared to the structure of the cationic AFB(1) adduct mispaired with dA [Giri, I., Johnston, D. S., and Stone, M. P. (2002) Biochemistry 41, 5462-5472].

Published

2002

39. Chlorophyllin intervention reduces aflatoxin-DNA adducts in individuals at high risk for liver cancer.

Author

Egner PA, Wang JB, Zhu YR, Zhang BC, Wu Y, Zhang QN, Qian GS, Kuang SY, Gange SJ, Jacobson LP, Helzlsouer KJ, Bailey GS, Groopman JD, and Kensler TW

Subjects

Adult, Aflatoxin B1 urine, Aflatoxins urine, Aged, Animals, Biomarkers urine, Carcinoma, Hepatocellular etiology, China, DNA Adducts urine, Female, Food Contamination, Guanine urine, Humans, Liver Neoplasms etiology, Male, Middle Aged, Risk Factors, Aflatoxin B1 analogs & derivatives, Aflatoxins toxicity, Carcinoma, Hepatocellular prevention & control, Chlorophyllides pharmacology, DNA Adducts drug effects, Guanine analogs & derivatives, Liver Neoplasms prevention & control

Abstract

Residents of Qidong, People's Republic of China, are at high risk for development of hepatocellular carcinoma, in part from consumption of foods contaminated with aflatoxins. Chlorophyllin, a mixture of semisynthetic, water-soluble derivatives of chlorophyll that is used as a food colorant and over-the-counter medicine, has been shown to be an effective inhibitor of aflatoxin hepatocarcinogenesis in animal models by blocking carcinogen bioavailability. In a randomized, double-blind, placebo-controlled chemoprevention trial, we tested whether chlorophyllin could alter the disposition of aflatoxin. One hundred and eighty healthy adults from Qidong were randomly assigned to ingest 100 mg of chlorophyllin or a placebo three times a day for 4 months. The primary endpoint was modulation of levels of aflatoxin-N(7)-guanine adducts in urine samples collected 3 months into the intervention measured by using sequential immunoaffinity chromatography and liquid chromatography-electrospray mass spectrometry. This aflatoxin-DNA adduct excretion product serves as a biomarker of the biologically effective dose of aflatoxin, and elevated levels are associated with increased risk of liver cancer. Adherence to the study protocol was outstanding, and no adverse events were reported. Aflatoxin-N(7)-guanine could be detected in 105 of 169 available samples. Chlorophyllin consumption at each meal led to an overall 55% reduction (P = 0.036) in median urinary levels of this aflatoxin biomarker compared with those taking placebo. Thus, prophylactic interventions with chlorophyllin or supplementation of diets with foods rich in chlorophylls may represent practical means to prevent the development of hepatocellular carcinoma or other environmentally induced cancers.

Published

2001

40. Development of aflatoxin B(1)-lysine adduct monoclonal antibody for human exposure studies.

Author

Wang JS, Abubaker S, He X, Sun G, Strickland PT, and Groopman JD

Subjects

Antibodies, Monoclonal, Antigens, Binding, Competitive, Environmental Exposure, Humans, Lysine immunology, Reproducibility of Results, Sensitivity and Specificity, Serum Albumin, Bovine immunology, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 blood, Aflatoxin B1 immunology, Carcinogens, Environmental analysis, Radioimmunoassay methods

Abstract

Mouse monoclonal antibodies were developed against a synthetic aflatoxin B(1) (AFB)-lysine-cationized bovine serum albumin conjugate. The isotype of one of these antibodies, IIA4B3, has been classified as immunoglobulin G1(lambda). The affinity and specificity of IIA4B3 were further characterized by a competitive radioimmunoassay. The affinities of IIA4B3 for AFB and its associated adducts and metabolites are ranked as follows: AFB-lysine > 8,9-dihydro-8-(2,6-diamino-4-oxo-3,4-dihydropyrimid-5-yl formamido)-9-hydroxy-AFB > AFB = 8,9-dihydro-8-(N(7)-guanyl)-9-hydroxy-AFB > aflatoxin M(1) > aflatoxin Q(1). IIA4B3 had about a 10-fold higher affinity for binding to AFB-lysine adduct than to AFB when (3)H-AFB-lysine was used as the tracer. The concentration for 50% inhibition for AFB-lysine was 0.610 pmol; that for AFB was 6.85 pmol. IIA4B3 had affinities at least sevenfold and twofold higher than those of 2B11, a previously developed antibody against parent AFB, for the major aflatoxin-DNA adducts 8,9-dihydro-8-(N(7)-guanyl)-9-hydroxy-AFB and 8,9-dihydro-8-(2,6-diamino-4-oxo-3,4-dihydropyrimid-5-yl formamido)-9-hydroxy-AFB, respectively. An analytical method based on a competitive radioimmunoassay with IIA4B3 and (3)H-AFB-lysine was validated with a limit of detection of 10 fmol of AFB-lysine adduct. The method has been applied to the measurement of AFB-albumin adduct levels in human serum samples collected from the residents of areas at high risk for liver cancer.

Published

2001

41. Quantification and validation of enzyme immunoassay for urinary aflatoxin B1-N7-guanine adduct for biological monitoring of aflatoxins.

Author

Nayak S, Sashidhar RB, and Bhat RV

Subjects

Aflatoxins administration & dosage, Animals, DNA Adducts urine, Enzyme-Linked Immunosorbent Assay methods, Female, Humans, Male, Rabbits, Rats, Rats, Inbred F344, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 urine, Environmental Monitoring methods, Food Contamination, Guanine analogs & derivatives, Guanine urine

Abstract

The aflatoxin B1-N7-guanine (AFB1-N7-guanine) adduct has been established as one of the relevant biomarkers of dietary aflatoxin (AFB1) exposure. Measurement of this adduct is potentially a useful dosimeter in molecular epidemiological studies. This paper reports the application and evaluation of a sensitive indirect competitive enzyme-linked immunosorbent assay (ELISA) for the detection and quantification of urinary AFB1-N7-guanine adduct in high risk populations exposed to dietary aflatoxin. Earlier, we had reported a simple and rapid indirect ELISA method for AFB1-N7-guanine adduct in the urine and liver tissues using polyclonal antibodies specific to AFB1-N7-guanine adduct. The method was evaluated using a rodent model (Fischer 344), exposed to 1 mg kg-1 body mass of AFB1 and human urine samples obtained from a maize eating population, environmentally exposed to AFB1 through their diet. The levels of AFB1-N7-guanine adduct in rat and human urine ranged from 6.42 to 20.16 micrograms mg-1 creatinine and from 9.30 to 13.43 ng mg-1 creatinine, respectively. The level of AFB1 in the diet as estimated by ELISA ranged from 1000 to 3600 ng d-1. The interesting observation in these studies is that the females (in both rodents and human subjects) are more efficient than males at excreting the adduct. Total adduct (DNA bound adduct and guanine adduct excreted in urine) was found to be similar in male and female rats. However, 63% of the total adduct was accounted for in urine of female rats, whereas male rats excreted 47% of the total adduct in their urine. The present method may find wide application as a biochemical tool in molecular epidemiological studies with respect to human exposure to dietary aflatoxins.

Published

2001

42. Cytotoxicity of aflatoxin B1 and its chemically synthesised epoxide derivative on the A549 human epithelioid lung cell line.

Author

Palanee T, Dutton MF, and Chuturgoon AA

Subjects

Aflatoxin B1 chemical synthesis, Epithelioid Cells drug effects, Formazans, Humans, Tetrazolium Salts, Tumor Cells, Cultured, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 toxicity, Carcinogens toxicity, Lung drug effects

Abstract

Aflatoxin B1 (AFB1 ) is a carcinogenic mycotoxin found in feeds and in airborne grain dusts. Aflatoxin B1 requires biotransformation to the AFB1-8,9 epoxide (AFBO) by a bioactivation system and subsequent covalent binding to DNA or proteins, to exert its carcinogenic potential. The lung contains cytochrome P450, prostaglandin-H-synthase, lipoxygenase, epoxide hydrolase and other bioactivation enzymes, and is thus a potential target for the effects of AFB1 via the routes of inhalation and ingestion. The A549 human epithelioid lung cell line and the methylthiazol tetrazolium (MTT) bioassay were used to investigate the cytotoxicity of AFB1 and its chemically synthesised epoxide (AFBO) in vitro. Statistical analysis of the MTT results indicated that there were overall significant differences between the control and both the AFB1-treated (p < 0.0001) and AFBO-treated cells (p = 0.002). However, there was no significant difference between AFB1 and AFBO-treated cells, when the entire range of concentrations were assessed against each other (p = 0.2877). When analysed at each concentration, only at 0.01 mM was there a significant difference between the effects of AFB1 and AFBO (p = 0.0358). The results of this investigation show that AFB1 and AFBO are both cytotoxic in the A549 cell line.

Published

2001

43. Interindividual differences in response to chemoprotection against aflatoxin-induced hepatocarcinogenesis: implications for human biotransformation enzyme polymorphisms.

Author

Eaton DL, Bammler TK, and Kelly EJ

Subjects

Aflatoxin B1 adverse effects, Aflatoxin B1 chemistry, Aflatoxin B1 pharmacokinetics, Aflatoxins adverse effects, Aflatoxins chemistry, Aflatoxins pharmacokinetics, Animals, Carcinogens adverse effects, Carcinogens chemistry, Carcinogens pharmacokinetics, Humans, Inactivation, Metabolic, Polymorphism, Genetic, Species Specificity, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Aflatoxins metabolism, Carcinogens metabolism, Cytochrome P-450 Enzyme System metabolism, Epoxide Hydrolases metabolism, Glutathione Transferase metabolism, Liver Neoplasms metabolism

Abstract

It is now evident that most, if not all, of the remarkable species differences in susceptibility to AFB hepatocarcinogenesis is due in large part, if not exclusively, to differences in biotransformation. Certainly the relative rate of oxidative formation of the proximate carcinogen, AFB-8,9-exo-epoxide, is an important determinant of species and interindividual differences in susceptibility to AFB. However, mice produce relatively large amounts of exo-AFBO, yet are highly resistant to AFB-hepatocarcinogenesis because they express a particular form of GST with remarkably high catalytic activity toward the exo-epoxide of AFB. Rats, which are highly susceptible to AFB hepatocarcinogenesis,can be made resistant through dietary induction of an orthologous form of GST that is normally expressed in only very small amounts. Based on these findings in laboratory animal models, there is great interest in identifying chemicals and/or specific dietary constituents that could offer protection against AFB-hepatocarcinogenesis to humans. Current experimental strategies have focused on the antiparasitic drug, oltipraz, which induces protection in rats and has also shown some promise in humans. The mechanism of protection in rats appears to be via induction of an alpha class GST with high catalytic activity toward AFBO (rGSTA5-5). vet human alpha class GST proteins that are constitutively expressed in the liver (hGSTA1 and hGSTA2) have little, if any activity toward AFBO. Rather, it appears that mu class GSTs may be responsible for the very low, but potentially significant, detoxification activity toward AFBO. Oltipraz and certain dietary constituents may induce mu class GSTs in human liver, and this could afford some protection against the genotoxic effects of AFBO. However, it also appears that oltipraz, and perhaps certain dietary constituents, act as competitive inhibitors of human CYP1A2. As CYP1A2 appears to mediate most of the activation of AFB to exo-AFBO in human liver at low dietary concentrations of AFB encountered in the human diet, much of the putative protective effects of oltipraz could be mediated via inhibition of CYP1A2 rather than induction of GSTs. There is now evidence that human microsomal epoxide hydrolase (mEH) could play a role in protecting human DNA from the genotoxic effects of AFB, although the importance of this detoxification pathway, relative to mu class GSTs, remains to be elucidated. Oltipraz is an effective inducer of mEH in rats (Lamb Franklin, 2000), and thus induction of this pathway in humans could also potentially contribute to the protective effects of this drug toward AFB genotoxicity. Because the dihydrodiol of AFB may contribute indirectly to the carcinogenic effects of AFB via protein adduction and subsequent hepatotoxicity, the recently characterized human aflatoxin aldehyde reductase (AFAR) may also offer some protection against AFB-induced carcinogenicity in humans. Current and future dietary and/or chemointervention strategies aimed at reducing the carcinogenic effects of AFB in humans should consider all of the possible mechanistic approaches for modifying AFB-induced genotoxicity.

Published

2001

44. Replication of a site-specific trans-8,9-dihydro-8-(N7-guanyl)-9-hydroxyaflatoxin B(1) adduct by the exonuclease deficient klenow fragment of DNA polymerase I.

Author

Johnston DS and Stone MP

Subjects

Aflatoxin B1 chemical synthesis, Aflatoxin B1 isolation & purification, DNA biosynthesis, DNA chemistry, DNA genetics, DNA Adducts chemical synthesis, DNA Adducts isolation & purification, Exonucleases deficiency, Exonucleases metabolism, Guanine chemical synthesis, Guanine isolation & purification, Oligonucleotides chemical synthesis, Templates, Genetic, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 genetics, DNA Adducts genetics, DNA Polymerase I metabolism, DNA Replication, Guanine analogs & derivatives, Oligonucleotides genetics

Abstract

A 19-mer oligodeoxynucleotide containing a site-specific trans-8, 9-dihydro-8-(N7-guanyl)-9-hydroxyaflatoxin B(1) adduct was prepared and purified. This was used as a template for replication with DNA polymerase I exo(-) (Klenow exo(-)) in vitro. The chemical stability of the modified template strand containing the cationic aflatoxin B(1) adduct was monitored by mass spectrometry. Under the conditions used in these assays, the cationic aflatoxin B(1) adduct remained intact; quantitative conversion to the corresponding formamidopyrimidine adduct was not observed. The results revealed that the cationic guanine AFB(1) N7 adduct blocked translesional DNA synthesis at the adducted site and one nucleotide 3' to the adducted site. Correct incorporation of cytosine opposite the lesion led to blockage, while incorrect incorporation of adenine allowed full-length extension. The in vitro experiments with polymerase I yielded base pair substitutions at the lesion site but not the 5'-neighbor substitutions observed in vivo [Bailey, E. A., Iyer, R. S., Stone, M. P., Harris, T. M., and Essigmann, J. M. (1996) Proc. Natl. Acad. Sci. U.S.A. 93, 1535-1539].

Published

2000

45. Cytochrome P450-mediated metabolism and cytotoxicity of aflatoxin B(1) in bovine hepatocytes.

Author

Kuilman ME, Maas RF, and Fink-Gremmels J

Subjects

Aflatoxin B1 analogs & derivatives, Aflatoxin B1 biosynthesis, Aflatoxin M1 biosynthesis, Animals, Benzoflavones pharmacology, Biotransformation, Cattle, Cell Survival drug effects, Cytochrome P-450 CYP1A1 antagonists & inhibitors, Cytochrome P-450 Enzyme Inhibitors, Dose-Response Relationship, Drug, Enzyme Inhibitors pharmacology, Female, Ketoconazole pharmacology, Liver cytology, Liver drug effects, Steroid Hydroxylases antagonists & inhibitors, Aflatoxin B1 toxicity, Cytochrome P-450 CYP1A1 metabolism, Cytochrome P-450 Enzyme System metabolism, Liver enzymology, Steroid Hydroxylases metabolism

Abstract

Aflatoxin B(1) (AFB(1)) biotransformation comprises cytochrome P450-mediated reactions resulting in hydroxylated and demethylated metabolites as well as AFB(1) epoxides. As the latter are highly nucleophilic, the species-specific rate of epoxidation and the ability for rapid conjugation to glutathione by glutathione S-transferase determines the individual susceptibility to AFB(1). Here we show the time- and dose-dependent rate of AFB(1)-metabolism in bovine hepatocytes. Aflatoxin M(1) (AFM(1)) is the most prominent metabolite formed within the first 2-8 hr of incubation, whereas AFB(1)-dhd is detectable in medium mainly after a prolonged incubation period. The delayed formation of AFB(1)-dhd corresponds to the cytotoxicity demonstrated by the MTT assay. alpha-Naphthoflavone and ketoconazole, inhibitors of CYP1A and CYP3A, respectively in humans, were used to evaluate the contribution of specific P450 isoenzymes in bovine biotransformation of AFB(1). Initial experiments confirmed that alpha-naphthoflavone and ketoconazole inhibited ethoxyresorufin O-deethylation and testosterone 6beta-hydroxylation also in bovine hepatocytes. Both inhibitors reduced AFM(1) and AFB(1)-dhd formation concentration dependently, suggesting that both enzyme groups contribute to the formation of these metabolites. However, the formation of AFM(1) was less inhibited by both compounds than the formation of AFB(1)-dhd.

Published

2000

46. Mu-class GSTs are responsible for aflatoxin B(1)-8, 9-epoxide-conjugating activity in the nonhuman primate macaca fascicularis liver.

Author

Wang C, Bammler TK, Guo Y, Kelly EJ, and Eaton DL

Subjects

Aflatoxin B1 metabolism, Amino Acid Sequence, Animals, Blotting, Western, Chondroitin Sulfates classification, Chondroitin Sulfates genetics, Chondroitin Sulfates isolation & purification, Chromatography, Affinity, Cloning, Molecular, DNA, Complementary metabolism, Disaccharides classification, Disaccharides genetics, Disaccharides isolation & purification, Male, Molecular Sequence Data, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Aflatoxin B1 analogs & derivatives, Carcinogens metabolism, Chondroitin Sulfates metabolism, Disaccharides metabolism, Liver enzymology, Macaca fascicularis

Abstract

Mice are resistant to the carcinogenic effects of the mycotoxin aflatoxin B(1) (AFB(1)) because they constitutively express an alpha-class glutathione S-transferase (mGSTA3-3) that has high (approximately 200,000 pmol/min/mg) activity toward aflatoxin B(1)-8, 9-epoxide (AFBO). Rats do not constitutively express a GST with high AFBO-conjugating activity and are sensitive to AFB(1)-induced hepatocarcinogenesis. Constitutively expressed human hepatic alpha-class GSTs (hGSTA1-1 and hGSTA2-2) possess little or no AFBO-detoxifying activity (<2 pmol/min/mg). Recently, we found that the nonhuman primate, Macaca fascicularis (Mf), exhibits significant (approximately 300 pmol/min/mg) constitutive hepatic GST activity towards AFBO. To determine which specific GST isoenzyme(s) is (are) responsible for this activity, MF: GSTs were purified from liver tissue and characterized and, Mf mu-class GST cDNAs were cloned by reverse transcriptase-coupled polymerase chain reaction (RT-PCR). Purification by glutathione agarose (GSHA) affinity chromatography yielded a protein, GSHA-GST, that exhibited relatively high AFBO-conjugating activity (239 pmol/min/mg) compared to other GST-containing peaks. Western blotting and enzymatic activity analyses revealed that GSHA-GST belongs to the mu class. Two distinct mu-class GST cDNAs, mfaGSTM1 (GenBank accession # AF200709) and mfaGSTM2 (GenBank accession # AF200710), were generated by RT-PCR. CDNA-derived amino acid sequence analysis revealed that mfaGSTM1 and mfaGSTM2 share 97% and 96% homology with the human mu-class GSTs hGSTM4 and hGSTM2, respectively. In contrast to recombinant mfaGSTM1-1, which had no detectable AFBO-conjugating activity, mfaGSTM2-2 exhibited this activity at 333 pmol/min/mg. Activity profiles for the stereoisomers exo- and endo-AFBO, and of 1-chloro-2,4-dinitrobenzene of the purified protein GSHA-GST and recombinant mfaGSTM2-2, suggested that they are two distinct enzymes. Our results indicate that, in contrast to rodents, mu-class GSTs are responsible for the majority of AFBO-conjugating activity in the liver of Macaca fascicularis.

Published

2000

47. Retroviral expression of the hepatitis B virus x gene promotes liver cell susceptibility to carcinogen-induced site specific mutagenesis.

Author

Sohn S, Jaitovitch-Groisman I, Benlimame N, Galipeau J, Batist G, and Alaoui-Jamali MA

Subjects

7,8-Dihydro-7,8-dihydroxybenzo(a)pyrene 9,10-oxide metabolism, 7,8-Dihydro-7,8-dihydroxybenzo(a)pyrene 9,10-oxide toxicity, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Aflatoxin B1 toxicity, Apoptosis drug effects, Carcinogens metabolism, Cell Cycle drug effects, Cell Line, Codon genetics, DNA Mutational Analysis, Disease Susceptibility, Genes, p53 genetics, Genetic Vectors genetics, Humans, Liver cytology, Liver virology, Mutagens metabolism, Mutagens toxicity, Mutation genetics, Polymerase Chain Reaction, Trans-Activators genetics, Transduction, Genetic, Viral Regulatory and Accessory Proteins, Carcinogens toxicity, Hepatitis B virus genetics, Hepatitis B virus pathogenicity, Liver drug effects, Liver metabolism, Mutagenesis, Site-Directed drug effects, Trans-Activators metabolism

Abstract

Mutational inactivation of the tumor suppressor gene p53 is common in hepatocellular carcinomas (HCC). AGG to AGT transversion in codon 249 of exon 7 of the p53 gene occurs in over 50% of HCC from endemic regions, where both chronic infection with the hepatitis B virus (HBV) and exposure to carcinogens such as aflatoxin B1 (AFB1) prevail. In this study, we report the effect of the HBV x protein (HBx) on carcinogen-induced cytotoxicity and AGG to AGT mutation in codon 249 of the p53 gene in the human liver cell line CCL13. Expression of HBx, as revealed by its transactivation function, results in enhanced cell susceptibility to cytotoxicity induced by the AFB1 active metabolite, AFB1-8,9-epoxide, and benzo(a)pyrene diol-epoxide. Under similar conditions, expression of HBx promotes apoptosis in a subset of cell population. Exposure to AFB1-8, 9-epoxide alone induces a low frequency of AGG to AGT mutation in codon 249 of the p53 gene, as determined by an allele-specific polymerase chain reaction (AS-PCR) assay. However, expression of HBx enhances the frequency of AFB1-epoxide-induced AGG to AGT mutation compared to control cells. In summary, this study demonstrates that expression of HBx enhances liver cell susceptibility to carcinogen-induced mutagenesis, possibly through alteration of the balance between DNA repair and apoptosis, two cellular defense mechanisms against genotoxic stress.

Published

2000

48. Kinetic studies of aflatoxin B1-glutathione conjugate formation in liver and kidneys of adult and weanling rats.

Author

Allameh A, Farahani M, and Zarghi A

Subjects

Aflatoxin B1 metabolism, Animals, Animals, Newborn growth & development, Chromatography, High Pressure Liquid, Glutathione metabolism, Kinetics, Male, Rats, Rats, Wistar, Aflatoxin B1 analogs & derivatives, Aging metabolism, Animals, Newborn metabolism, Glutathione analogs & derivatives, Kidney metabolism, Liver metabolism, Weaning

Abstract

Aflatoxin B1(AFB1)-glutathione(GSH) conjugation is the major pathway for the detoxification of aflatoxin metabolites. This reaction is catalysed by GSH S-transferase (GST) and play a major role in modulation of AFB1 adduct formation to nuclear DNA. Changes recorded in hepatic GST activity during development of rats can alter the balance between AFB1-GSH conjugation and AFB1-DNA adduct formation. Measurment of cytosolic GST using 1-chloro-2,4-dinitrobenzene (CDNB) as the substrate showed that the enzyme activity is initially lower in weanling tissues as compared to that of adults. But nevertheless hepatic and renal cytosolic GST activity is increased significantly in growing rats pretreated with AFB1. Kinetic studies of AFB1-GSH conjugate formation in kidneys and livers of the two-age groups of rats treated with a single i.p. dose of AFB1 (400 microg/kg b.w.) revealed that at the end of 24 h of AFB1 administration the rate of the conjugate formation in kidneys of immature rats was approximately twice of that measured in adults. Age-related differences in the GST activity as well as AFB1-GSH conjugation was more pronounced in kidneys. The conjugate formation in kidneys of growing rats during 6-24 h following AFB1 administration shows that urinary excretion of aflatoxin metabolites is relatively rapid in growing rats. The major portion of the AFB1-GSH is formed in liver but contribution of the renal tissue to the formation of detoxification metabolites can not be ruled out. These data demonstrate that aflatoxin metabolites are eliminated more efficiently from kidneys of a growing rat. AFB1-induced GST induction in renal tissues of growing animals during 24 h of the carcinogen administration could be considered as an important mechanism for GSH conjugate formation and aflatoxin detoxification. Therefore GST induction in response to hepatotoxic drugs can confer resistance to young animals being exposed for the first time to such drugs. It is also worthmentioning that the GST activity measured before AFB1 administration does not reflect the rate of AFB1 detoxification via GSH conjugation.

Published

2000

49. Biochemical basis for the extreme sensitivity of turkeys to aflatoxin B(1).

Author

Klein PJ, Buckner R, Kelly J, and Coulombe RA Jr

Subjects

Animals, Biotransformation, Carcinogens toxicity, Cytochrome P-450 CYP1A2 metabolism, Cytochrome P-450 CYP3A, Cytochrome P-450 Enzyme System metabolism, Humans, Inactivation, Metabolic, Male, Microsomes, Liver drug effects, Microsomes, Liver metabolism, Mixed Function Oxygenases metabolism, Species Specificity, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Aflatoxin B1 toxicity, Turkeys

Abstract

Poultry are the most susceptible food animal species to the toxic effects of the mycotoxin aflatoxin B(1) (AFB(1)). Feed contaminated with even small amounts of AFB(1) results in significant adverse health effects in poultry. The purpose of this study was to explain the biochemical mechanism(s) for this extreme sensitivity. We measured microsomal activation of AFB(1) to the AFB(1)-8,9-epoxide (AFBO), the putative toxic intermediate, as well as cytosolic glutathione S-transferase (GST)-mediated detoxification of AFBO, in addition to other hepatic phase I and phase II enzyme activities, in 3-week-old male Oorlop strain turkeys. Liver microsomes prepared from these turkeys activated AFB(1) in vitro with an apparent K(m) of 109 microM and a V(max) of 1.25 nmol/mg/min. Preliminary evidence for the involvement of cytochromes P450 (CYP) 1A2 and, to a lesser extent, 3A4 for AFB(1) activation was assessed by the use of specific mammalian CYP inhibitors. The possible presence of avian orthologues of these CYPs was supported by activity toward ethoxyresorufin and nifedipine, as well as by Western immunoblotting using antibodies to human CYPs. Cytosol prepared from turkey livers exhibited GST-mediated conjugation of 1-chloro-2,4-dinitrobenzene (CDNB) and 3,4-dichloronitrobenzene (DCNB), but at a much lower rate than that observed in other species. Western immunoblotting indicated the presence of alpha and sigma class GSTs and another AFB(1)-detoxifying enzyme, AFB(1)-aldehyde reductase (AFAR). Turkey liver cytosol also had quinone oxidoreductase (QOR) activity. Importantly, cytosol exhibited no measurable GST-mediated detoxification of microsomally activated AFB(1), indicating that turkeys are deficient in the most crucial AFB(1)-detoxification pathway. In total, our data indicate that the extreme sensitivity of turkeys to AFB(1) may be attributed to a combination of efficient AFB(1) activation and deficient detoxification by phase II enzymes, such as GSTs., (Copyright 2000 Academic Press.)

Published

2000

50. DNA-damaging effects of genotoxins in mixture: modulation of covalent binding to DNA.

Author

Ross MK, Said B, and Shank RC

Subjects

2-Acetylaminofluorene analogs & derivatives, 2-Acetylaminofluorene metabolism, 2-Acetylaminofluorene pharmacology, Aflatoxin B1 analogs & derivatives, Aflatoxin B1 metabolism, Aflatoxin B1 pharmacology, Animals, Binding, Competitive, Cattle, DNA Adducts metabolism, Guanine analogs & derivatives, Guanine metabolism, Mutagens metabolism, Sulfuric Acid Esters metabolism, Sulfuric Acid Esters pharmacology, DNA metabolism, DNA Adducts drug effects, DNA Damage drug effects, Mutagens pharmacology

Abstract

Modulation of DNA adduct formation by pre-existing adducts was examined in synthetic oligonucleotides and genomic DNA (calf thymus); genotoxins studied were N-acetoxy-acetylaminofluorene (N-AcO-AAF), aminofluorene (AF), aflatoxin B1-8,9-epoxide (AFB1-8,9-epoxide), and dimethylsulfate (DMS). Oligodeoxynucleotides containing either guanine-C8-AAF (Gua-C8-AAF) or Gua-C8-AF adducts and a neighboring unadducted guanine (G) (target G), located 1, 2, or 4 nucleotides from the adduct, were reacted, as single- (ss) or double-stranded (ds) substrates, with dimethylsulfate (DMS) or AFB1-8,9-epoxide. A modified Maxam-Gilbert technique showed that the presence of the AAF adduct lowered the extent to which AFB1-8,9-epoxide, but not DMS, reacted with target G. Binding of AFB1-8,9-epoxide to the target G was attenuated (> or =5-fold) when the target was located immediately adjacent to an AAF, but not AF, adduct in ds-DNA. Reaction with AFB1-8,9-epoxide increased when the target G was located 2 or 4 nucleotides from the AAF adduct. Pretreatment of calf thymus DNA with AAF (0-1.8% nucleotides modified) reduced levels of Gua-N7-AFB1 adducts formed after subsequent treatment with AFB1-8,9-epoxide. Pretreatment of calf thymus DNA with AFB1 did not alter levels of adducts formed after subsequent treatment with N-AcO-AAF. The supposition that aflatoxin B1-binding to DNA may be altered by conformational changes in the helix, due to the presence of a pre-existing AAF adduct, is supported by the absence of an effect by AF and confirmation of local denaturation of the oligomer helix by use of chemical probes hydroxylamine and diethylpyrocarbonate. Nonetheless, the importance of changes in the nucleophilicity of neighboring nucleotides and local steric effects cannot be ruled out.

Published

2000