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  • 3-aminobenzanthrone  (8)
  • 1
    Keywords: CANCER ; CELLS ; EXPRESSION ; IN-VIVO ; LUNG-CANCER ; DNA adducts ; RISK ; GENE ; LINES ; ACTIVATION ; DNA ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; AIR ; CARCINOGENESIS ; CYP1A2 ; CYTO-TOXIC METABOLITES ; DIESEL EXHAUST ; DNA ADDUCT FORMATION ; ENVIRONMENTAL CONTAMINANT 3-NITROBENZANTHRONE ; GENETIC POLYMORPHISMS ; HETEROCYCLIC AMINES ; HETEROLOGOUS EXPRESSION ; HUMAN CYTOSOLIC SULFOTRANSFERASES ; IONS ; metabolic activation ; NAT : SULT ; nitro-PAH ; P-32- postlabeling ; PHENOL SULFOTRANSFERASES ; POSTLABELING ANALYSIS
    Abstract: 3-Nitrobenzanthrone (3-NBA) is a potent mutagen and suspected human carcinogen identified in diesel exhaust and ambient air pollution. 3-Aminobenzanthrone (3-ABA), 3- acetylaminobenzanthrone (3-Ac-ABA) and N-acetyl-N-hydroxy-3- aminobenzanthrone (N-Ac-N-OH-ABA) have been identified as 3-NBA metabolites. Recently we found that 3-NBA and its metabolites (3-ABA, 3-Ac-ABA and N-Ac-N-OH-ABA) form the same DNA adducts in vivo in rats. In order to investigate whether human cytochrome P450 (CYP) enzymes (i.e., CYPIA2), human N,O- acetyltransferases (NATs) and sulfotransferases (SULTs) contribute to the metabolic activation of 3-NBA and its metabolites we developed a panel of Chinese hamster V79MZ-hIA2 derived cell lines expressing human CYPIA2 in conjunction with human NATI, NAT2, SULTIAI or SULTIA2, respectively. Cells were treated with 0.01, 0.1 or I muM 3-NBA, or its metabolites (3- ABA, 3-Ac-ABA and N-Ac-N-OH-ABA). Using both enrichment versions of the P-32-postlabeling assay, nuclease P I digestion and butanol extraction, essentially 4 major and 2 minor DNA adducts were detected in the appropriate cell lines with all 4 compounds. The major ones were identical to those detected in rat tissue; the adducts lack an N-acetyl group. Human CYPIA2 was required for the metabolic activation of 3-ABA and 3-Ac-ABA (probably via N-oxidation) and enhanced the activity of 3-NBA (probably via nitroreduction). The lack of acetylated adducts suggests N-deacetylation of 3-Ac-ABA and N-Ac-N-OH-ABA. Thus, N-hydroxy-3-aminobenzanthrone (N-OH-ABA) appears to be a common intermediate for the formation of the electrophilic arylnitrenium ions capable of reacting with DNA. Human NAT I and NAT2 as well as human SULTIAI and SULTIA2 strongly contributed to the high genotoxicity of 3-NBA and its metabolites. Moreover, N,O-acetyltransfer reactions catalyzed by human NATs leading to the corresponding N-acetoxyester may be important in the bioactivation of N-Ac-N-OH-ABA. As human exposure to 3-NBA is likely to occur primarily via the respiratory tract, expression of CYPs, NATs and SULTs in respiratory tissues may contribute significantly and specifically to the metabolic activation of 3-NBA and its metabolites. Consequently, polymorphisms in these genes could be important determinants of lung cancer risk from 3-NBA
    Type of Publication: Journal article published
    PubMed ID: 12740904
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  • 2
    Keywords: EXPRESSION ; human ; liver ; ENZYMES ; PROTEIN ; TIME ; ACTIVATION ; DNA ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; DIESEL EXHAUST ; DNA ADDUCT FORMATION ; AIR-POLLUTION ; INDUCTION ; LIVER-MICROSOMES ; RAT ; SUDAN-I ; CONTAMINANT 3-NITROBENZANTHRONE ; RATS ; RAT-LIVER ; HUMAN ACETYLTRANSFERASES ; BODY ; air pollution ; INCREASE ; WEIGHT ; LEVEL ; ENZYME ; P-32-postlabeling ; reductive activation ; P-32-POSTLABELING ANALYSIS ; BIOTRANSFORMATION ENZYMES ; NAD(P)H-QUINONE OXIDOREDUCTASE ; NITROPOLYCYCLIC AROMATIC-HYDROCARBONS
    Abstract: 3-Nitrobenzanthrone (3-NBA), a suspected human carcinogen occurring in diesel exhaust and air pollution, and its human metabolite 3-aminobenzanthrone (3-ABA) were investigated for their ability to induce biotransformation enzymes in rat liver and the influence of such induction on DNA adduct formation by the compounds. Rats were treated (i.p.) with 0.4, 4, or 40 mg/kg body weight 3-NBA or 3-ABA. When hepatic cytosolic fractions from rats treated with 40 mg/kg body weight 3-NBA or 3-ABA were incubated with 3-NBA, DNA adduct formation, measured by P-32-postlabeling analysis, was 10-fold higher in incubations with cytosols from pretreated rats than with controls. The increase in 3-NBAderived DNA adduct formation corresponded to a dose-dependent increase in protein levels and enzymatic activity of NAD(P) H: quinone oxidoreductase (NQO1). NQO1 is the major enzyme reducing 3-NBA in human and rat livers. Incubations of 3-ABA with hepatic microsomes of rats treated with 3-NBA or 3-ABA (40 mg/ kg body weight) led to as much as a 12-fold increase in 3-ABA-derived DNA adduct formation compared with controls. The observed stimulation of DNA adduct formation by both compounds was attributed to their potential to induce protein expression and enzymatic activity of cytochromes P450 1A1 and/ or -1A2 (CYP1A1/2), the major enzymes responsible for 3-ABA activation in human and rat livers. Collectively, these results demonstrate for the first time, to our knowledge, that by inducing hepatic NQO1 and CYP1A1/2, both 3-NBA and 3-ABA increase the enzymatic activation of these two compounds to reactive DNA adduct-forming species, thereby enhancing their own genotoxic potential
    Type of Publication: Journal article published
    PubMed ID: 16714372
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  • 3
    Keywords: CELLS ; IN-VITRO ; CELL ; human ; IN-VIVO ; LUNG ; MODEL ; PATHWAY ; PATHWAYS ; VITRO ; VIVO ; SYSTEM ; liver ; MICE ; TIME ; ACTIVATION ; DNA ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; AIR ; CARCINOGENESIS ; DIESEL EXHAUST ; DNA ADDUCT FORMATION ; CONTAMINANT 3-NITROBENZANTHRONE ; BINDING ; bone marrow ; BONE-MARROW ; MOUSE ; MUTANT ; TRANSGENIC MICE ; ASSAY ; genetics ; genotoxicity ; DNA-BINDING ; METABOLIC-ACTIVATION ; NUCLEOTIDES ; POLYCYCLIC AROMATIC-HYDROCARBONS ; EPITHELIAL-CELLS ; ADDUCTS ; heredity ; BODIES ; RE ; air pollution ; INCREASE ; ADDUCT FORMATION ; LEVEL ; BONE ; ENGLAND ; PREDICT ; INCREASES ; ENVIRONMENTAL-POLLUTANT 3-NITROBENZANTHRONE ; NOV ; outcome ; MARROW ; NUCLEOTIDE ; CARCINOGEN 3-NITROBENZANTHRONE ; HUMAN METABOLITE ; URBAN AIR-POLLUTION
    Abstract: FE1 lung epithelial cells derived from Muta (TM) Mouse are a new model system to provide in vitro mutagenicity data with the potential to predict the outcome of an in vivo Muta (TM) Mouse test. 3-Nitrobenzanthrone (3-NBA) is a potent mutagen and suspected human carcinogen identified in diesel exhaust and urban air pollution. We investigated the mutagenicity and DNA binding of 3-NBA and its main metabolite 3-aminobenzanthrone (3-ABA) in vitro and in vivo in the Muta (TM) Mouse assay. Mice were treated with 3-NBA or 3-ABA (0, 2 or 5 mg/kg body weight/day) by gavage for 28 days and 28 days later lacZ mutant frequency (MF) was determined in liver, lung and bone marrow. For both compounds, dose-related increases in MF were seen in liver and bone marrow, but not in lung; mutagenic activity was similar to 2-fold lower for 3-ABA than for 3-NBA. With 3-NBA, highest DNA adduct levels (measured by P-32-post-labelling) were found in liver (similar to 230 adducts per 10(8) nucleotides) with levels 20- to 40-fold lower in bone marrow and lung. With 3-ABA, DNA adduct levels were again highest in the liver, but similar to 4-fold lower than for 3-NBA. FE1 cells were exposed to up to 10 mu g/ml 3-NBA or 3-ABA for 6 h with or without exogenous activation (S9) and harvested after 3 days. For 3-NBA, there was a dose-related increase in MF both with and without S9 mix, which was 〉 10 times higher than observed in vivo. At the highest concentration of 3-ABA (10 mu g/ml), we found only around a 2-fold increase in MF relative to controls. DNA adduct formation in FE1 cells was dose-dependent for both compounds, but 10- to 20-fold higher for 3-NBA compared to 3-ABA. Collectively, our data indicate that Muta (TM) Mouse FE1 cells are well suited for cost-effective testing of suspected mutagens with different metabolic activation pathways as a guide for subsequent in vivo Muta (TM) Mouse testing
    Type of Publication: Journal article published
    PubMed ID: 18635558
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  • 4
    Keywords: CELLS ; IN-VITRO ; human ; IN-VIVO ; LUNG ; PATHWAYS ; VIVO ; DNA adducts ; EXPOSURE ; liver ; ENZYMES ; TISSUE ; HEART ; ACTIVATION ; DNA ; kidney ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; CARCINOGENESIS ; DIESEL EXHAUST ; DNA ADDUCT FORMATION ; metabolic activation ; nitro-PAH ; RAT ; animals ; AROMATIC-AMINES ; BASE ; BIOMARKERS ; BODY-WEIGHT ; colon ; CONTAMINANT 3-NITROBENZANTHRONE ; ENRICHMENT ; HPLC ; P-32-postlabelling ; RATS ; TISSUES ; tumour
    Abstract: Diesel exhaust is known to induce tumours in animals and is suspected of being carcinogenic in humans. Of the compounds found in diesel exhaust, 3-nitrobenzanthrone (3-NBA) is an extremely potent mutagen and suspected human carcinogen forming multiple DNA adducts in vitro. 3-Aminobenzanthrone (3-ABA). 3- acetylaminobenzanthrone (3-Ac-ABA), and N-acetyl-N-hydroxy-3- aminobenzanthrone (N-Ac-N-OH-ABA) were identified as 3-NBA metabolites. In order to gain insight into the pathways of metabolic activation leading to 3-NBA-derived DNA adducts we treated Wistar rats intraperitoneally with 2 mg/kg body weight of 3-NBA, 3-ABA. 3-Ac-ABA, or N-Ac-N-OH-ABA and compared DNA adducts present in different organs, With each compound either four or five DNA adduct spots were detected by TLC in all tissues examined (lung, liver. kidney, heart, pancreas, and colon) using the nuclease P1 or butanol enrichment version of the P-32-postlabelling method, respectively. Using HPLC co- chromatographic analysis we showed that all major 3-NBA-DNA adducts produced in vivo in rats are derived from reductive metabolites bound to purine bases and lack an N-acetyl group. Our results indicate that 3-NBA metabolites (3-ABA, 3-Ac-ABA and AT-Ac-N-OH-ABA) undergo several biotransformations and that N-hydroxy-3-aminobenzanthrone (N-OH-ABA) appears to be the common intermediate in 3-NBA-derived DNA adduct formation. Therefore, 3-NBA-DNA adducts are useful biomarkers for exposure to 3-NBA and its metabolites and may help to identify enzymes involved in their metabolic activation. (C) 2002 Elsevier Science (USA). All rights reserved
    Type of Publication: Journal article published
    PubMed ID: 12480528
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  • 5
    Keywords: EXPRESSION ; human ; LUNG ; DNA adducts ; PROTEIN ; ACTIVATION ; DNA ; kidney ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; AIR ; DIESEL EXHAUST ; DNA ADDUCT FORMATION ; GENETIC POLYMORPHISMS ; PHENOL SULFOTRANSFERASES ; INDUCTION ; RAT ; animals ; CONTAMINANT 3-NITROBENZANTHRONE ; P-32-postlabelling ; RATS ; STIMULATION ; TARGET ; HUMAN ACETYLTRANSFERASES ; METABOLIC-ACTIVATION ; ADDUCTS ; protein expression ; cytochrome P450 ; DNA-ADDUCTS ; air pollution ; INCREASE ; LEVEL ; pharmacology ; cyclooxygenase ; PROSTAGLANDIN-H SYNTHASE ; animal ; enzymatic ; QUINONE OXIDOREDUCTASE ; ANTIOXIDANT-RESPONSE-ELEMENT ; NAD(P)H : quinone oxidoreductase ; cytochrome p450 1A1
    Abstract: 3-Nitrobenzanthrone (3-NBA) is a carcinogen occurring in diesel exhaust and air pollution. Using the P-32-postlabelling method, we found that 3-NBA and its human metabolite, 3-aminobenzanthrone (3-ABA), are activated to species forming DNA adducts by cytosols and/or microsomes isolated from rat lung, the target organ for 3-NBA carcinogenicity, and kidney. Each compound generated identical five DNA adducts. We have demonstrated the importance of pulmonary and renal NAD(P)H:quinone oxidoreductase (NQO1) to reduce 3-NBA to species that are further activated by N,O-acetyltransferases and sulfotransferases. Cytochrome P450 (CYP) 1A1 is the essential enzyme for oxidative activation of 3-ABA in microsomes of both organs, while cyclooxygenase plays a minor role. 3-NBA was also investigated for its ability to induce NQO1 and CYP1A1 in lungs and kidneys, and for the influence of such induction on DNA adduct formation by 3-NBA and 3-ABA. When cytosols from rats treated i.p. with 40 mg/kg bw of 3-NBA were incubated with 3-NBA, DNA adduct formation was up to 2.1-fold higher than in incubations with cytosols from control animals. This increase corresponded to an increase in protein level and enzymatic activity of NQO1. Incubations of 3-ABA with microsomes of 3-NBA-treated rats led to up to a fivefold increase in DNA adduct formation relative to controls. The stimulation of DNA adduct formation correlated with the potential of 3-NBA to induce protein expression and activity of CYP1A1. These results demonstrate that 3-NBA is capable to induce NQO1 and CYP1A1 in lungs and kidney of rats thereby enhancing its own genotoxic and carcinogenic potential. (C) 2008 Elsevier Ireland Ltd. All rights reserved
    Type of Publication: Journal article published
    PubMed ID: 18329153
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  • 6
    Keywords: CELLS ; IN-VITRO ; human ; IN-VIVO ; VITRO ; LUNG-CANCER ; DNA adducts ; liver ; MICE ; ACTIVATION ; DNA ; kidney ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; CARCINOGENESIS ; DIESEL EXHAUST ; AIR-POLLUTION ; CONTAMINANT 3-NITROBENZANTHRONE ; P-32-postlabelling ; BINDING ; METABOLITES ; BREAST ; DNA-BINDING ; HUMAN ACETYLTRANSFERASES ; METABOLIC-ACTIVATION ; cytochrome P450 ; V79 CELLS ; RE ; air pollution ; MYELOPEROXIDASE ; ENZYME ; CARCINOGENIC ARISTOLOCHIC ACIDS ; SULFOTRANSFERASES ; reductive activation ; in vivo ; PROSTAGLANDIN-H SYNTHASE
    Abstract: 3-Nitrobenzanthrone (3-NBA) is a suspected human carcinogen found in diesel exhaust and ambient air pollution. The main metabolite of 3-NBA, 3-aminobenzanthrone (3-ABA), was detected in the urine of salt mining workers occupationally exposed to diesel emissions. We evaluated the role of hepatic cytochrome P450 (CYP) enzymes in the activation of 3-ABA in vivo by treating hepatic cytochrome P450 oxidoreductase (POR)-null mice and wild-type littermates intraperitoneally with 0.2 and 2 mg/kg body weight of 3-ABA. Hepatic POR-null mice lack POR-mediated CYP enzyme activity in the liver. Using the P-32-postlabelling method, multiple 3-ABA-derived DNA adducts were observed in liver DNA from wild-type mice, qualitatively similar to those formed in incubations using human hepatic microsomes. The adduct pattern was also similar to those formed by the nitroaromatic counterpart 3-NBA and which derive from reductive metabolites of 3-NBA bound to purine bases in DNA. DNA binding by 3-ABA in the livers of the null mice was undetectable at the lower dose and substantially reduced (by up to 80%), relative to wild-type mice, at the higher dose. These data indicate that POR-mediated CYP enzyme activities are important for the oxidative activation of 3-ABA in livers, confirming recent results indicating that CYP-1A1 and -1A2 are mainly responsible for the metabolic activation of 3-ABA in human hepatic microsomes. No difference in DNA binding was found in kidney and bladder between null and wild-type mice, suggesting that cells in these extrahepatic organs have the metabolic capacity to oxidize 3-ABA to species forming the same 3-ABA-derived DNA adducts, independently from the CYP-mediated oxidation in the liver. We determined that different model peroxidases are able to catalyse DNA adduct formation by 3-ABA in vitro. Horseradish peroxidase (HRP), lactoperoxidase (LPO), myeloperoxidase (MPO), and prostaglandin H synthase (PHS) were all effective in activating 3-ABA in vitro, forming DNA adducts qualitatively similar to those formed in vivo in mice treated with 3-ABA and to those found in DNA reacted with N-hydroxy-3-aminobenzanthrone (N-OH-ABA). Collectively, these results suggest that both CYPs and peroxidases may play an important role in metabolizing 3-ABA to reactive DNA adduct forming species. (c) 2005 Elsevier Ireland Ltd. All rights reserved
    Type of Publication: Journal article published
    PubMed ID: 15885895
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  • 7
    Keywords: IN-VITRO ; human ; IN-VIVO ; LUNG ; VITRO ; SYSTEM ; DNA adducts ; TISSUE ; MICE ; DNA ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; CARCINOGENESIS ; DIESEL EXHAUST ; ENVIRONMENTAL CONTAMINANT 3-NITROBENZANTHRONE ; POSTLABELING ANALYSIS ; RAT ; RATS ; TISSUES ; METABOLITES ; IDENTIFICATION ; HUMAN ACETYLTRANSFERASES ; METABOLIC-ACTIVATION ; MUTAGENICITY ; rodent ; PERFORMANCE LIQUID-CHROMATOGRAPHY ; SURFACE SOIL ; V79 CELLS ; RE ; air pollution ; ENZYME ; P-32-postlabeling ; in vivo ; DEOXYGUANOSINE ; LIQUID ; P-32-POSTLABELING ANALYSIS ; xanthine oxidase
    Abstract: 3-Nitrobenzanthrone (3-NBA) is a potent mutagen and potential human carcinogen identified in diesel exhaust and ambient air particulate matter. Previously, we detected the formation of 3-NBA-derived DNA adducts in rodent tissues by P-32-postlabeling, all of which are derived from reductive metabolites of 3-NBA bound to purine bases, but structural identification of these adducts has not yet been reported. We have now prepared 3-NBA-derived DNA adduct standards for P-32-postlabeling by reacting N-acetoxy-3-aminobenzanthrone (N-Aco-ABA) with purine nucleotides. Three deoxyguanosine (dG) adducts have been characterised as N-(2'-deoxy-guanosin-8-yl)-3-aminobenzanthrone-3'-phosphate (dG3'p-C8-N-ABA), 2-(2'-deoxyguanosin-N-2 -yl)-3-aminobenzanthrone-3'-phosphate (dG3'p-N-2-ABA) and 2-2'-(deoxygtianosin-8-yl)-3-aminobenzanthrone-3'-phosphate (dG3'p-C8-C2-ABA), and a deoxyadenosine (dA) adduct was characterised as 2-(2'-deoxyadenosm-N-6-yl)-3-aminobenzanthrone-3'-phosphate (dA3'p-N-6-ABA). 3-NBA-derived DNA adducts formed experimentally in vivo and in vitro were compared with the chemically synthesised adducts. The major 3-NBA-derived DNA adduct formed in rat lung cochromatographed with dG3'p-N-2-ABA in two independent systems (thin layer and high-performance liquid chromatography). This is also the major adduct formed in tissue of rats or mice treated with 3-aminobenzanthrone (3-ABA), the major human metabolite of 3-NBA. Similarly, dG3'p-C8-N-ABA and dA3'p-N-6-ABA cochromatographed with two other adducts formed in various organs of rats or mice treated either with 3-NBA or 3-ABA, whereas dG3'p-C8-C2-ABA did not cochromatograph with my of the adducts found in vivo. Utilizing different enzymatic systems in vitro, including human hepatic microsomes and cytosols, and purified and recombinant enzymes, we found that a variety of enzymes [NAD(P)H:quinone oxidoreductase, xanthine oxidase, NADPH:cytochrome P450 oxidoreductase, cytochrome P450s 1A1 and 1A2, N,O-acetyltransferases 1 and 2, sulfotransferases 1A1 and 1A2, and myeloperoxidase] are able to catalyse the formation of 2-(2-deoxyguanosin-N-2-yl)3-aminobenzanthrone, N-(2'-deoxyguanosin-8-yl)-3-aminobenzanthrone and 2-(2'-deoxyadenosin-N-6-yl)-3-aminobenzanthrone in DNA, after incubation with 3-NBA and/or 3-ABA. (c) 2005Wiley-Liss, Inc
    Type of Publication: Journal article published
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  • 8
    Keywords: APOPTOSIS ; CELLS ; CELL ; PATHWAY ; PATHWAYS ; TOXICITY ; SYSTEM ; DEATH ; NF-KAPPA-B ; ACTIVATION ; DNA ; 3-aminobenzanthrone ; 3-nitrobenzanthrone ; CARCINOGENESIS ; DIESEL EXHAUST ; ENVIRONMENTAL CONTAMINANT 3-NITROBENZANTHRONE ; PHOSPHORYLATION ; cytokines ; MOUSE ; CELL-DEATH ; genetics ; DAMAGE ; HUMAN ACETYLTRANSFERASES ; METABOLIC-ACTIVATION ; POLYCYCLIC AROMATIC-HYDROCARBONS ; DNA-DAMAGE ; NETHERLANDS ; TRANSLOCATION ; FLOW-CYTOMETRY ; AKT ; CYTOKINE ; MAPK ; SCIENCE ; ADDUCT FORMATION ; cell death ; DNA damage ; DNA ADDUCT ; ERK ; CARCINOGEN 3-NITROBENZANTHRONE ; AIR-POLLUTANT 3-NITROBENZANTHRONE ; Genetic ; IMMUNE ; 3-Ammobenzanthrone ; LUNG EPITHELIAL-CELLS
    Abstract: 3-Nitrobenzanthrone (3-NBA) is a mutagenic and carcinogenic environmental pollutant found in diesel exhaust and urban air pollution. In the present work we have characterised the effects of 3-NBA and its metabolite 3-aminobenzanthrone (3-ABA) on cell death and cytokine release in mouse hepatoma Hepa1c1c7 cells. These effects were related to induced DNA damage and changes in cell signalling pathways. 3-NBA resulted in cell death and caused most DNA damage as judged by the amount of DNA adducts (P-32-postlabelling assay), single strand (ss)DNA breaks and oxidative DNA lesions (comet assay) detected. An increased phosphorylation of H2AX, chk1, chk2 and partly ATM was observed using flow cytometry and/or Western blotting. Both compounds increased phosphorylation of p53 and MAPKs (ERK, p38 and JNK). However, only 3-NBA caused an accumulation of p53 in the nucleus and a translocation of Bax to the mitochondria. The p53 inhibitor pifithrin-alpha inhibited 3-NBA-induced apoptosis, indicating that cell death was a result of the triggering of DNA signalling pathways. The highest phosphorylation of Akt and degradation of I kappa B-alpha (suggesting activation of NF-kappa B) were also seen after treatment with 3-NBA. In contrast 3-ABA increased IL-6 release, but caused little or no toxicity. Cytokine release was inhibited by PD98059 and curcumin, suggesting that ERK and NF-kappa B play a role in this process. in conclusion, 3-NBA seems to have a higher potency to induce DNA damage compatible with its cytotoxic effects, while 3-ABA seems to have a greater effect on the immune system. (C) 2009 Elsevier B.V. All rights reserved
    Type of Publication: Journal article published
    PubMed ID: 19941874
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