A short low-level exposure to metavanadate during a cell cycle-specific interval of time is sufficient to permanently derange the differentiative properties of Mel cells

doi:10.1093/mutage/16.5.395

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Mutagenesis, Vol. 16, No. 5, 395-400, September 2001
© 2001 UK Environmental Mutagen Society/Oxford University Press

A short low-level exposure to metavanadate during a cell cycle-specific interval of time is sufficient to permanently derange the differentiative properties of Mel cells

M. Foresti¹^,, S. Scippa, F. Mele, G. Palladino and M. de Vincentiis

Dipartimento di Genetica, Biologia Generale e Molecolare, Università degli Studi di Napoli `Federico II', Naples, Italy

Mouse erythroleukemia (Mel) cells have a cell cycle-dependenthigh sensitivity to chemical and physical mutagens. This reportshows that a 5 h exposure to 0.1 or 0.01 µg/ml metavanadateduring the initial period of erythroid differentiation inductionwas sufficient to permanently damage the ability of treatedMel cells and their progeny to undergo erythroid differentiation,without affecting cell viability and proliferation. Conversely,a 5 h pulse of metavanadate at 1 or 10 µg/ml inhibitedboth differentiation and cell proliferation. The cell cycle-dependentperiod of mutagenesis was essential for fixation of damage inthe cell genome and the progeny of the cells treated with 0.1or 0.01 µg/ml metavanadate stably inherited an impairedcapacity to differentiate. The efficiency of the DNA repairsynthesis machinery during the specific period of exposure ofMel cells seemed directly involved in damage fixation. In fact,the mutagenic effects of a 0.1 µg/ml metavanadate pulsewas further increased in the presence of 1 mM hydroxyurea, aninhibitor of DNA repair synthesis. In contrast, 5 µg/mlvanillin, an antimutagenic agent that stimulates repair, completelyrestored the capacity of progeny of cells treated with 0.1 µg/mlmetavanadate to complete differentiation. Determination of [³H]deoxythymidinein acid-insoluble DNA indicated that incorporation was stimulatedby metavanadate alone and was further increased by metavanadateplus vanillin; conversely, incorporation of thymidine was reducedin the presence of hydroxyurea. The capacity of metavanadateto permanently damage Mel cell erythroid differentiation appearedto depend on the cell cycle-related efficiency of the DNA repairsystems, activated to correct the induced alteration, ratherthan on a specific concentration.

¹ To whom correspondence should be addressed. Tel: +39 81 2535010;Fax: +39 81 2535000; Email: foresti{at}dgbm.unina.it

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