Diethylsulphate and methylnitrosourea affect different targets in Chinese hamster fibroblasts: possible mechanisms of aneuploidy induction by these agents

doi:10.1093/mutage/geg012

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Mutagenesis vol. 18 no. 5 pp. 405-410, September 2003
© 2003 UK Environmental Mutagen Society/Oxford University Press

Diethylsulphate and methylnitrosourea affect different targets in Chinese hamster fibroblasts: possible mechanisms of aneuploidy induction by these agents

M. Campagna, P. Beffy¹, R. Del Carratore¹, L. Hauri¹, S. Simi¹, S. Bonatti¹ and M. Simili¹^,2

International Center for Genetic Engineering and Biotechnology, Padriciano, Trieste, Italy and ¹Institute of Clinical Physiology, National Research Council, Via Moruzzi 1, I-56124 Pisa, Italy

It has been shown that the ethylating agent diethylsulphate(DES) induces centromere-containing micronuclei with kineticssuggesting that molecules other than DNA could be targets. Inquiescent Chinese hamster fibroblasts CHEF/18, O⁶-alkylatedbases inhibit ribosomal protein S6 kinase (S6K1), the terminalmember of a kinase cascade responsible for an increased rateof protein synthesis, but not extracellular signal-activatedkinases (ERK1/2) or terminal kinases of a second cascade whichactivates transcription. The inhibition correlates with theappearance of abnormal metaphases at the following mitosis,suggesting that alkylation of the nucleotide pool and inhibitionof S6K1 could be one of the mechanisms leading to chromosomeloss by alkylating agents. To clarify the role of protein kinasesin chromosome loss induced by alkylating agents, we have studiedthe effects of DES and methylnitrosourea (MNU) on S6K1 and ERK1/2activation by growth factors. The alkylating agents were studiedin a battery of Chinese hamster fibroblasts (CHEF/18, CHO andClB) with normal and mutated p53 to control for DNA damage-inducedactivation of p53, which could indirectly inhibit protein kinases.The role of repair in induction of micronuclei was studied inmismatch repair-proficient CHO and repair-deficient ClB cells.Our results indicate that DES induced micronuclei in a mismatchrepair-independent manner, within 8 h of treatment, in agreementwith a role for S6K1 inhibition in micronucleus formation. MNUinduced centromere-containing micronuclei only in CHO cells,one cell cycle after treatment, without any detectable influenceson either kinase cascade, suggesting a role for mismatch repairin chromosome loss.

²To whom correspondence should be addressed. Tel: +39 0503152780; Fax: +39 0503153367; Email: marcella.simili{at}ifc.cnr.it

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