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Measurement and characterization of micronuclei in cultured primary lung cells of mice following inhalation exposure to benzene

TitleMeasurement and characterization of micronuclei in cultured primary lung cells of mice following inhalation exposure to benzene
Publication TypeArticolo su Rivista peer-reviewed
Year of Publication1998
AuthorsRanaldi, R., Bassani B., Villani Paola, Lombardi C.C., Tanzarella C., and Pacchierotti Francesca
JournalMutagenesis
Volume13
Pagination453-460
ISSN02678357
KeywordsAdministration, aneuploidy, animal cell, animal experiment, Animalia, Animals, article, Benzene, cell culture, Cells, centromere, Chromosome aberrations, chromosome analysis, chromosome breakage, chromosome loss, controlled study, Cultured, cytochalasin b, Dose-Response Relationship, Drug, Fibroblasts, fluorescence, genotoxicity, immunofluorescence test, Inbred C57BL, inhalation, Kinetochores, lung, lung fibroblast, male, Mice, micronucleus, micronucleus test, Micronucleus Tests, Microscopy, mouse, nonhuman, priority journal, Spleen
Abstract

The genotoxic effects of benzene in lung cells of mice exposed to single acute doses by inhalation have been estimated by cytogenetic analysis of micronuclei in primary cultures of lung fibroblasts. Mice were nose-only exposed to 1000 p.p.m. for 30 or 60 min or to 3500 p.p.m. for 30 min and sacrificed 24 h after the end of exposure. Lung fibroblasts were cultured attached to coverslips for 72 h, the last 48 h in the presence of 0.75 μg/ml cytochalasin B. Micronuclei were scored in binucleate cells. The mechanism(s) of micronucleus induction was characterized by immunofluorescent staining of kinetochore proteins (CREST staining), which allowed micronuclei due to chromosome loss (kinetochore-positive) to be distinguished from those produced by chromosome breakage (kinetochore-negative). Three- and 4-fold statistically significant increases in total micronucleus frequencies were observed in all benzene-exposed mice with respect to unexposed controls. The effect was neither concentration nor time dependent. This is compatible with a plateau dose-effect relationship for the effects on bone marrow, which is explained by saturation of metabolism. Both chromosome loss and chromosome breakage appear to contribute to micronucleus formation, suggesting that in addition to chromosome rearrangements, aneuploidy may be a relevant early genotoxic event associated with benzene carcinogenicity. Under the same treatment conditions no micronucleus induction could be shown in spleen lymphocytes, suggesting that with very short benzene exposures cells at the first contact site with local metabolizing capacity have a higher probability of genetic alterations potentially leading to neoplasia.

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URLhttps://www.scopus.com/inward/record.uri?eid=2-s2.0-0031712767&doi=10.1093%2fmutage%2f13.5.453&partnerID=40&md5=76e47c726d8133b95492e79f01c23f5f
DOI10.1093/mutage/13.5.453
Citation KeyRanaldi1998453