Titolo | Acrylamide-induced chromosomal damage in male mouse germ cells detected by cytogenetic analysis of one-cell zygotes |
---|---|
Tipo di pubblicazione | Articolo su Rivista peer-reviewed |
Anno di Pubblicazione | 1994 |
Autori | Pacchierotti, Francesca, Tiveron C., D'Archivio M., Bassani B., Cordelli Eugenia, Leter Giorgio, and Spanò M. |
Rivista | Mutation Research Regular Papers |
Volume | 309 |
Paginazione | 273-284 |
ISSN | 00275107 |
Parole chiave | acrylamide, Acrylamide, animal, animal cell, animal experiment, Animalia, article, Chromosome aberration, Chromosome aberrations, chromosome damage, controlled study, Cytotoxicity, Dose-Response Relationship, Drug, Female, Flow cytometry, germ cell, Inbred Strains, male, Metaphase, Mice, mouse, mutagenicity, Mutagens, Non-U.S. Gov't, nonhuman, priority journal, Sister Chromatid Exchange, spermatid, spermatogenesis, Superovulation, Support, testis, Zygote |
Abstract | Within a project coordinated by the Commission of the European Communities for the detection of germ cell mutagens, the cytogenetic analysis of first-cleavage metaphases was carried out to detect chromosomal damage induced by acrylamide (AA) in meiotic and postmeiotic stages of mouse spermatogenesis. Male mice were intraperitoneally injected with single acute doses of 75 or 125 mg/kg or treated with five daily injections of 50 mg/kg and mated either 7 or 28 days after the end of treatment. Chromosomal aberrations were scored in C-banded metaphases prepared from one-cell zygotes by a mass harvest technique. AA treatment of late spermatids-spermatozoa resulted in significant increases of structural aberrations at all doses tested. The data could be fitted to a curvilinear regression and a doubling dose of 23 mg/kg was calculated. The large majority of observed aberrations were of the chromosome type, including dicentrics, rings and translocations, in agreement with a mechanism of chromosomal damage mediated through the alkylation of DNA-associated protamines. Even though the frequency of aberrations 28 days after treatment was not significantly higher than the control value, the presence of multiple rearrangements in two cells suggested that AA might also have a minor effect on spermatocytes. The results of the cytogenetic analysis of first cleavage metaphases agreed well both qualitatively and quantitatively with the outcome of dominant lethal and heritable translocations assays. AA-induced cytotoxicity was monitored by flow cytometric DNA content analysis of testicular cells. By this method, a dose-dependent depletion of mature spermatids after treatment of spermatogonia and a toxic effect upon primary spermatocytes were detected. © 1994. |
Note | cited By 31 |
URL | https://www.scopus.com/inward/record.uri?eid=2-s2.0-0028145916&doi=10.1016%2f0027-5107%2894%2990102-3&partnerID=40&md5=5f1bf3ded2eb0d5ed008bc2ee9154303 |
DOI | 10.1016/0027-5107(94)90102-3 |
Citation Key | Pacchierotti1994273 |