Résumé
Introducción. Los mutágenos contenidos en mezclas complejas presentan interacciones de sinergismo, aditivas o antagónicas. Se han desarrollado enfoques experimentales que permitan dilucidar el responsable de las interacciones en la mezcla. Objetivo. Desarrollar un diseño experimental para comprender los procesos que se llevan a cabo entre los compuestos presentes en las mezclas complejas. Materiales y métodos. Se expusieron linfocitos humanos a mezclas binarias de mutágenos B[a]P, DMBA, Trp-P-1 y MX durante una hora, con activación metabólica y sin ella. La viabilidad se evaluó con azul de tripano y, la genotoxicidad, con cometa alcalino. Resultados. Ningún hidrocarburo tuvo efecto con furanona. Con S9 y sin él, se observó que se presentaban interacciones tóxicas entre hidrocarburos. Se observó sinergismo sin S9 entre B[a]P y Trp-P-1 y, con actividad metabólica, entre DMBA y Trp-P-1. Sin S9 se observó interacción antagónica entre Trp-P-1 y DMBA y, con S9, entre Trp-P-1 y MX y entre MX y DMBA. Se observó un incremento dependiente de la dosis en la longitud de la cola. Hubo daño genotóxico medio y aumento de las células dañadas. Para todas las mezclas se pudo determinar la concentración mínima en la que se observaban efectos adversos y solo para algunas se determinó la concentración máxima en la cual no se observaron efectos adversos. Conclusión. Se hace un aporte para comprender los procesos que ocurren cuando en una mezcla hay presentes, al menos, dos mutágenos y se valida un modelo de análisis que permite dilucidar el compuesto que tiene efecto sobre otro. También, se demostró que según el tipo de compuestos en la mezcla, se tendrá o no un umbral de riesgo.
Introduction. Mutagens contained in complex mixtures can present synergistic interactions, either additive or antagonistic. Therefore, development of experimental approaches is necessary to elucidate which is the responsible agent for the effect in the mixtures. Objective. An experimental design was developed that allowed an understanding of the processes between the compounds of complex mixtures. Materials and methods. Human lymphocytes were exposed to binary mixtures of the mutagens B[a]P, DMBA, Trp-P-1 and MX for 1 hour with or without S9. Viability was assessed with trypan blue dye and the genotoxicity by the comet assay. Results. All of the hydrocarbon showed an effect with furanone. With and without S9, the most toxic interactions were observed between hydrocarbons. Synergistic interaction was observed without S9 between B [a] P and Trp-P-1 and between DMBA and Trp-P-1 with metabolic activity. Without S9 antagonistic interaction was observed only between Trp-P-1+DMBA, and with S9 between Trp-P-1+MX and MX+DMBA. It observed an increase dose dependent in tail length. Half the cultures showed genotoxic damage and increased cell damage. For each mixture, minimum concentrations were determined at which adverse effects are observed; for some only the maximum concentration was determined at which no adverse effects are observed. Conclusion. The processes between mutagens present in a mixture have become better understood, and the results validated an analytical model that determined which component had an effect on another. The results also showed that the type of compounds in the mixture determined whether or not a risk threshold was present.
Sujets)
Adulte , Humains , Mâle , Test des comètes , Techniques in vitro , Lymphocytes/effets des médicaments et des substances chimiques , Mutagènes/toxicité , /administration et posologie , /pharmacologie , /toxicité , Biotransformation , Benzo[a]pyrène/administration et posologie , Benzo[a]pyrène/pharmacologie , Benzo[a]pyrène/toxicité , Survie cellulaire , Carbolines/administration et posologie , Carbolines/pharmacologie , Carbolines/toxicité , Cellules cultivées/effets des médicaments et des substances chimiques , Cellules cultivées/ultrastructure , Altération de l'ADN , Interactions médicamenteuses , Furanes/administration et posologie , Furanes/pharmacologie , Furanes/toxicité , Lymphocytes/ultrastructure , Microsomes du foie/métabolisme , Mutagènes/administration et posologie , Mutagènes/pharmacologieRésumé
PURPOSE: To evaluate the influence of pulmonary instillation of Benzo[a]pyrene in lung apoptosis of Wistar rats. METHODS: Male Rattus norvegicus albinus, Wistar lineage was carried through an intra-pulmonary instillation of the Benzo[a]pyrene (B[a]P) dilution in alcohol 70 percent. Three experimental groups had been formed with 08 animals each: Control Group (Alcohol 70 percent); B[a]P Group 40 mg/kg; e B[a]P Group 80mg/kg, submitted to euthanasia 16 and 18 weeks after the experimental procedure. The pulmonary sections had been processed by TUNEL method and submitted to the histomorphometric analysis to quantify the apoptotic cell number. RESULTS: After 16 weeks, mean of apoptotic cells number in control group (19,3±3,2) was greater than 40mg/Kg group (11,8±1,9; p<0,01) and 80mg/Kg group (7,0±1,4; p<0,01). Significant difference also observed between 40mg/Kg and 80mg/Kg (p<0,05). After 18 weeks, mean of apoptotic cells number in control group (18,0±2,2) was greater than 40mg/Kg group (8,8±1,7; p<0,01) and 80mg/Kg group (5,5±1,3; p<0,01). Significant difference wasn't observed between 40mg/Kg and 80mg/Kg (ns). CONCLUSION: Intra-pulmonary instillation of Benzo[a]pyrene induces significant decrease of apoptotic activity in lung tissue.
OBJETIVO: Avaliar a influência da instilação intrapulmonar de Benzo[a]pireno na apoptose pulmonar de ratos Wistar. MÉTODOS: Rattus norvegicus albinus, linhagem Wistar machos foram submetidos à instilação intra-pulmonar da diluição em álcool 70 por cento de Benzo[a]pireno (B[a]P). Foram formados três grupos experimentais com 08 animais cada: Grupo Controle (álcool 70 por cento); Grupo B[a]P 40 mg/kg; e Grupo B[a]P 80mg/kg, submetidos a eutanásia 16 e 18 semanas após o procedimento experimental. As secções pulmonares foram processadas pelo método TUNEL e submetidas à análise histomorfométrica para quantificação do número de células apoptóticas. RESULTADOS: Após 16 semanas, a média do número de células apoptóticas do grupo controle (19,3±3,2) mostrou-se maior que o grupo 40mg/Kg (11,8±1,9; p<0,01) e 80mh/Kg (7,0±1,4; p<0,01). Diferença significante foi também observada entre os grupos 40mg/Kg e 80mg/Kg (p<0,05). Após 18 semanas, a média do número de células apoptóticas do grupo controle (18,0±2,2) mostrou-se maior que o grupo 40mg/Kg (8,8±1,7; p<0,01) e 80mh/Kg (5,5±1,3; p<0,01). Não foi observada diferença significante entre os grupos 40 e 80mg/Kg (ns). CONCLUSÃO: A instilação intrapulmonar de Benzo[a]pireno induziu diminuição significativa da atividade apoptótica em tecido pulmonar.