Comparação da mutagenicidade dos azo corantes Disperse Red 1, Disperse Orange 1 e Disperse Red 13 utilizando o teste de mutagenicidade com \'Salmonella\' / Comparison of the mutagenicity of the azo dyes Disperse Red 1, Disperse Orange 1 and Disperse Red 13 using Salmonella/microssome mutagenicity assay

Elisa Raquel Anastácio Ferraz

10 July 2008

Os azo corantes representam o maior grupo de corantes utilizados na indústria, principalmente no ramo têxtil. Sabe-se que grande parte desses produtos resiste aos sistemas de tratamento de efluente e assim, cerca de 10-15% dos corantes perdidos durante o processo de tingimento são lançados no efluente e atingem o meio ambiente. Alguns corantes desse grupo têm mostrado ser cancerígenos e mutagênicos para animais e humanos. Essa toxicidade se deve, em parte, à clivagem da ligação azo formando aminas aromáticas potencialmente cancerígenas. Ainda, a ação de sistema de metabolização nos grupamentos substituintes pode alterar a toxicidade destes compostos. Neste trabalho foram testados os azo corantes Disperse Orange 1 (4-(4--nitrofenilazo)difenilamina); pureza 96%; CAS no 2581-69-3), Disperse Red 1(N-etil-N(2-hidroxietil)-4-(4-nitrofenilazo)anilina; pureza 95%; CAS no. 2872-52-8) e Disperse Red 13 (2-[4-(2-cloro-4-nitrofenilazo)-N-etilfenilamino] etanol; pureza de 95%; CAS no 3180-81-2) usando o ensaio de mutagenicidade com Samonella. Foram utilizadas as linhagens tradicionais, TA98 e TA100 e suas respectivas derivadas com superprodução de nitroredutase e O-acetiltransferase, YG1041 e YG1042. Todos os corantes testados mostraram respostas mais altas com a linhagem TA98 em relação a TA100, o que sugere que esses compostos exercem seu efeito mutagênico principalmente por deslocamento do quadro de leitura do DNA. Para os três corantes, a resposta da linhagem YG1041 em relação a sua parental TA98 foi significativamente aumentada, mostrando a importância da nitroredutase e O-acetiltransferase na mutagenicidade desses corantes. Tal fato foi confirmado com as respostas da TA100 em relação a YG1042. O sistema de metabolização exógeno (S9) diminuiu a mutagenicidade de todos os corantes testados. Considerando os resultados obtidos com a linhagem YG1041, o corante Disperse Red 1 é o mais potente, seguido do Disperse Orange 1 e do Disperse Red 13. / Azo dyes constitute the largest group of colorants used in industry, mainly the textile one, and they pass through industrial wastewater treatment plants nearly unchanged due to their resistance to aerobic treatment. Therefore, it is estimated that 10-15% of the dyes are lost in the effluent during the dyeing process, reaching the environment. Some of these dyes have been shown to be carcinogenic and mutagenic to animals and humans. This toxic effect is, in part due to azo bond cleavage that forms potentially carcinogenic aromatic amines. The toxicity of the dyes can also be altered by the biotransformation of the substitutens. We tested the azo dyes Disperse Orange 1 (4-(4-Nitrophenylazo)diphenylamine); 96% purity; CAS number 2581-69-3), Disperse Red 1(N-Ethyl-N-(2-hydroxyethyl)-4-(4-nitrophenylazo)aniline; 95% purity; CAS number 2872-52-8) and Disperse Red 13 (2-[4-(2-Chloro-4-nitrophenylazo)-N-ethylphenylamino]ethanoll; 95% purity; CAS number 3180-81-2) using Salmonella/microssome mutagenicity assay. We used the traditional strains TA98 and TA100 and the strains with overproducing nitroreductase and O-acetyltransferase, YG1041 and YG1042, derivative of the TA 98 and TA100, respectively. All the dyes tested showed higher responses with the strain TA98 when compared with TA100, suggesting that these compounds induce mainly frameshift mutations. Moreover, we observed an increase in the mutagenicity with the overproducing nitroreductase and O-acetyltransferase strains, showing the importance of these enzymes in the mutagenicity of these dyes. In addition, for all the dyes the mutagenicity decreased after the S9 addition. According to mutagenic response with YG1041, Disperse Red 1 was the most potent, followed by Disperse Orange 1 and Disperse Red 13.

azo corantes

Disperse Orange 1

Disperse Red 1

Disperse Red 13

ensaio de mutagenicidade com Salmonella.

azo dyes

Disperse Orange 1

Disperse Red 1

Disperse Red 13

Salmonella mutagenicity assay.

Avaliação toxicogenética e ecotoxicológica de corantes têxteis / Toxicogenetic and ecotoxicological assessment of textile dyes

Gisele Augusto Rodrigues de Oliveira

12 June 2013

O tingimento de tecidos começou há milhares de anos e a disponibilidade comercial de corantes é enorme e crescente. A indústria têxtil brasileira desempenha um papel de inquestionável importância, destacando-se entre as principais atividades econômicas do país. O processo de tingimento é um dos fatores fundamentais no sucesso comercial dos produtos têxteis, uma vez que o consumidor exige cores resistentes à exposição ao calor, à luz, à transpiração e às lavagens. Segundo a literatura, condições de transpiração intensa contribuem para uma alta taxa de migração e subseqüente penetração de corantes têxteis para a pele humana. Além disso, 2 a 50% desses compostos permanecem no banho de tingimento e são descartados nos efluentes industriais, contaminando o ambiente e colocando em risco a saúde humana, uma vez que os métodos convencionais de tratamento de efluentes são ineficientes na remoção da coloração e da mutagenicidade de alguns corantes. Dentro deste contexto, este trabalho teve como objetivo avaliar os efeitos toxicogenéticos do corante Direct Black (DB38) original e após extração por lixiviação com suor sintético, utilizando o teste do cometa com fibroblastos e queratinócitos de pele humana, o teste Anexina V com fibroblastos e o ensaio de mutagenicidade com Salmonella typhimurium. Adicionalmente, foi investigada a ecotoxicidade dos corantes têxteis Direct Black 38 e Reactive Blue 15 (RB15) originais por meio de ensaios com sementes, dapnhias, minhocas e zebrafish realizados na UTOX, em Barcelona. O corante DB38 original e lixiviado não induziram genotoxicidade em fibroblastos e queratinócitos de pele humana. O corante DB38 original foi mutagênico para as linhagens TA98 e TA100 de S. typhimurium na presença de S9. Entretanto, o corante lixiviado não induziu mutagenicidade para essas linhagens testadas, considerando que a maior taxa de migração do corante para a solução de suor foi de ~1% nas seguintes condições: tingimento sem ensaboamento, pH 8,0 e 8 horas de incubação à 42°C. O corante original é citotóxico para fibroblastos após 48 horas de exposição. No entanto, essa citotoxicidade não foi mais observada após a lixiviação no suor. Os corantes DB38 e RB15 originais não foram tóxicos para as sementes de pepino, alface e tomate, e nem para as minhocas Eisenia foetida. Ambos os corantes foram fracamente tóxicos para Daphnia magna, porém o RB15 apresenta maior potencial tóxico em relação ao DB38. Os corantes DB38 e RB15 induziram malformações em larvas de zebrafish Danio rerio, caracterizadas por falha na inflação da bexiga natatória e alteração na cauda. Portanto, nossos resultados mostram a importância de se fazer não só a análise individual de corantes têxteis, mas também dos tecidos que os contêm. Além da necessidade de se desenvolver técnicas de tingimento mais seguras em relação à solidez da cor sob condições úmidas e as perdas de corante para o ambiente durante a etapa de fixação, indicando maior atenção ao estudo de efeitos sub-letais na avaliação do impacto desses compostos no ecossistema aquático. / The fabrics dyeing began thousands of years ago and the commercial availability of dyes is increasingly. The Brazilian textile industry plays a role of high importance, highlighting among the main economic activities in the country. The dyeing process is one of the key factors in the commercial success of textile products, since consumers are demanding colors more resistant to heat, light exposure, perspiration and washing. According to the literature, conditions of intense perspiration contribute to the migration and subsequent penetration of textile dyes to human skin. Furthermore, 2 to 50% of the initial dye load is present in the dye bath effluent and these compounds are discharged in industrial effluents, contaminating the environment and endangering human health, since the wastewater treatment systems are ineffective in removing the color and mutagenicity of some dyes. In this context, this study aimed to evaluate the toxicogenetic effects of the Direct Black 38 (DB38) dye original and extracted by leaching with artificial sweat using Comet assay with fibroblasts and keratinocytes from human skin, Anexin V assay with fibroblasts and Salmonella mutagenicity test. Additionally, we investigated the ecotoxicity of textile dye Direct Black 38 and Reactive Blue 15 (RB15) using assays with seeds, dapnhias, worms and zebrafish performed in UTOX in Barcelona. The original and leached DB38 dye did not induce genotoxicity in fibroblasts and keratinocytes from human skin. The original DB38 was mutagenic for TA98 and TA100 of S. typhimurium with S9. However, the solution with the leached dye did not induce mutagenicity for these tested strains, since the highest migration rate of the dye to the solution of artificial sweat was ~ 1% in the following conditions: type of dyeing without rinsing, pH 8.0 and 8-hour incubation at 42°C. The original dye was cytotoxic for fibroblasts after 48 hours of exposure. However, this cytotoxicity was no longer observed after leaching in sweat. The original DB38 and RB15 dyes showed no toxicity for cucumber, lettuce and tomato seeds and for earthworms Eisenia foetida. Both dyes were weakly toxic for Daphnia magna, but the RB15 has a higher toxic potential compared to DB38. The dyes DB38 and RB15 induced malformations in larvae of zebrafish Danio rerio by failure of the swim bladder inflation and changes in the tail. Therefore, our results show the importance of making the individual analysis of textile dyes, but also of fabrics containing them. Furthermore, it is necessary to develop safer techniques of dyeing in relation to the color fastness under humid conditions and the loss of dyes into the environment during the fixation step, indicating more attention to the study of sub-lethal effects in the evaluation of the impact of these compounds in the aquatic ecosystem.

Citotoxicidade

Direct Black 38

Ecotoxicidade

Fibroblastos (NDHF)

Genotoxicidade

Mutagenicidade

Queratinócitos (HaCat)

Reactive Blue

Suor sintético

Artificial sweat

Cytotoxicity

Direct Black 38

Ecotoxicity

Fibroblast (NDHF)

Genotoxicity

Keratinocyte (HaCat)

Mutagenicity

Reactive Blue

Health Effects of Occupational Exposure of Wildland Firefighters to Smoke from Biomass Burning

Wu, Chieh-Ming

January 2020

No description available.

Occupational Health

Environmental Health

Public Health

Wildland firefighters

Wildland fire smoke

Particulate matter

CO

Black carbon

Trace metals

Cardiovascular effects

Blood pressure

Heart rate

Oxidative stress

8-isoprostane

MDA

Ox-GS

Urinary mutagenicity

Studium metabolismu vzdušných polutantů a mutagenů 3-nitrobenzanthronu a 2-nitrobenzanthronu / Study of metabolism air pollutants and mutagens 3-nitrobenzanthrone and 2-nitrobenzanthrone

Čechová, Tereza

January 2012

Nitroaromatic compounds are mutagenic and carcinogenic substances present in environment. Most of nitroaromatic compounds are potent mutagens in bacterial and mammalian systems. They are also carcinogens causing development of tumors, primarily in the liver, lung and mammary glands. 3-Nitrobenzanthrone (3-NBA, 3-nitro-7H-benz [de] anthracene-7-one) is one of the polycyclic aromatic nitro compounds possesing high toxic effects. 3-NBA is an environmental pollutant present in diesel exhaust and was also detected in soil and in rain water. 2-Nitrobenzanthrone (2-NBA, 2-nitro-7H-benz [de] anthracene-7-one) is an isomer 3-NBA, which also occurs as a pollutant in air. Although the 2-NBA is a weakly toxic substance, its high abundance in air could exhibit a high health risk to humans. This thesis investigates the metabolism of 3-NBA and its isomeric derivate, isomer 2 NBA, under anaerobic and aerobic conditions. To study the metabolism of these compounds, microsomal systems isolated from the liver of rats pretreated with Sudanem I, -naphthoflavone, phenobarbital, ethanol and pregnenolon 16-carbonitrile (PCN), the inducers of cytochromes P450 1A, 2B, 2E1 and 3A, were used. We also used mouse models, a control mouse line (wild type WT) and mice with deleted gene of NADPH:CYP reductase in the liver, thus absenting...

Anwendung des Comet Assay (Einzelzell-Gelelektrophorese) an Zellen von Fischen zum Nachweis gentoxischer Wirkungen im aquatischen Biomonitoring / Wasserprobentest in vitro, Blutzelltest ex vivo und methodische Optimierung

Nehls, Sebastian

14 October 2013

Gewässer sind Lebensgrundlage, jedoch gleichzeitig Schadstoffsenken für eine Vielzahl von Kontaminanten. Biologische Wirkungstests und das Biomonitoring aquatischer Proben sind daher besonders wichtig, um Umwelt-Gefahrenpotenziale erkennen zu können. Der "Comet Assay" (Einzelzell-Gelelektrophorese) ist ein Indikator von DNA-Strangbrüchen und wurde hier als Test auf gentoxische Wirkungen erprobt und angewandt. Mit bekannten, gentoxischen Substanzen wurden Nachweisgrenzen und Dosis-Wirkungs-Beziehungen für die Zelllinien RTG-2 und RTL-W1 (aus der Regenbogenforelle, Oncorhynchus mykiss) in vitro ermittelt und methodische Parameter an die Zellen angepasst. Der Test reagierte sehr sensitiv auf 4-Nitrochinolin-1-oxid. Die Substanz war daher geeignet, um in weiteren Versuchen als Positivkontrolle zu dienen. Zur Bewertung der Messdaten wurde ein geeignetes statistisches Verfahren gefunden, das auch historische Kontrollen mit einbezog. Der zeitliche Verlauf der DNA-Schädigung des Testsystems mit RTG-2-Zellen wurde ermittelt, und durch Inhibition der DNA-Reparatur mit Aphidicolin wurden Zusammenhänge zwischen der Entstehung von DNA-Strangbrüchen, der DNA-Reparaturkapazität sowie der Metabolisierungskapazität untersucht. In einer zweiten Phase wurden unbehandelte Wasserproben aus Rhein, Elbe sowie weitere Oberflächenwasserproben mit dem Comet Assay an RTG-2-Zellen getestet. Bei 15 von 49 Proben zeigten sich gentoxische Effekte. In einer dritten Phase wurden Erythrozyten von freilebenden Döbeln, Leuciscus cephalus, aus der Mosel mit dem Comet Assay untersucht. Die Fische von drei Messstellen zeigten erhöhte Werte von DNA-Schädigungen, gegenüber einer vierten, stromabwärts gelegenen Messstation. Korrelationen mit den Ergebnissen zusätzlicher Biomarker ergaben sich nur teilweise. Chemische Analysen von Wasser- oder Gewebeproben ließen keine Rückschlüsse auf verursachende Kontaminanten zu - gerade dies unterstreicht jedoch die Wichtigkeit biologischer Tests bei komplexen Proben. / Bodies of Water are both vital resources and pollutant sinks for a multitude of contaminants. Therefore, biological effect tests and biomonitoring of aquatic samples are of particular importance to detect potential environmental hazards. The "comet assay" (single cell gel electrophoresis) is an indicator for DNA strand breaks and was explored and applied as a genotoxicity test in the present study. Known genotoxic substances were used to determine the detection limits and dose-response relationships for the cell lines RTG-2 and RTL-W1 (from rainbow trout, Oncorhynchus mykiss) in vitro, and to adapt methodological parameters to the cells. The test was very sensitive to 4-Nitroquinoline-1-oxide. This substance was therefore well-suited to serve as positive control in further experiments. In order to evaluate the measurement data, an appropriate statistical procedure was developed, which also took "historical" controls into account. The time course of DNA damage in the test system using RTG-2 cells was determined, and relationships between the origin of DNA strand breaks, DNA repair capacity and the metabolizing capacity of the cells was investigated by means of inhibition of DNA repair with Aphidicoline. In the second stage, native water samples from the rivers Rhine and Elbe and further surface waters were tested with the comet assay, using RTG-2 cells. 15 out of 49 samples showed genotoxic effects. In a third stage, erythrocytes of feral chub, Leuciscus cephalus, from the Moselle river were examined with the comet assay. The fish from three measuring stations showed elevated values of DNA damage compared to fish sampled from a downstream station. There were only partly correlations with the results from additional biomarkers. Chemical analyses of water and tissue samples did not permit conclusions on effect-causing substances.However, this emphasizes the importance of biological tests in dealing with complex environmental samples.

Comet Assay

Flüsse

Biomonitoring

DNA-Reparatur

DNA-Schäden

Fische

Gentoxizität

Gentoxizitätstest

In vitro-Test

Leuciscus cephalus

Mutagenität

Ökotoxikologie

Oncorhynchus mykiss

RTG-2-Fischzelllinie

RTL-W1-Fischzelllinie

Umweltverschmutzung

Wasserverschmutzung

DNA repair

Biomonitoring

Comet assay

DNA damage

Ecotoxicology

Environmental pollution

Fish

Genotoxicity

Genotoxicity test

In vitro test

Leuciscus cephalus

Mutagenicity

Oncorhynchus mykiss

Rivers

RTG-2 fish cell line

RTL-W1 fish cell line

Water pollution

570 Biologie

32 Biologie

WC 3440

ddc:570