Lack of induction of micronuclei in human peripheral blood lymphocytes treated with hydroquinone

doi:10.1093/mutage/15.6.479

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Mutagenesis, Vol. 15, No. 6, 479-487, November 2000
© 2000 UK Environmental Mutagen Society/Oxford University Press

Lack of induction of micronuclei in human peripheral blood lymphocytes treated with hydroquinone

Candace Lippoli Doepker, Karen Wonder Dumont, John O'Donoghue and J.Caroline English¹

Health and Environment Laboratories, Eastman Kodak Company, 1100 Ridgeway Avenue, Rochester, NY 14652-6272, USA

Hydroquinone (HQ) has been reported to produce chromosomal effectsin some in vivo and in vitro animal models. Its potential forinducing similar effects in human lymphocytes is less clear.The purpose of this study was to examine human lymphocytes treatedwith HQ for the presence of chromosomal anomalies, using anaccepted assay for micronuclei. In addition, the stability ofHQ in culture medium was determined to verify exposures. Lymphocytecultures were obtained from eight donors so that variable responsesamongst individuals could be assessed. The micronucleus assaysutilized were a common 72 h assay with no wash, as well as twoassay variations to maximize cell division. Assay variationsconsisted of either cell washing at 44 h or allowing unwashedcultures an extra 24 h recovery period before harvest. In allassays treatment was at 24 h post-mitogenic stimulation andcytochalasin B was added to stop dividing cells from undergoingcytokinesis. Thus, cells that were scored had undergone onedivision in the presence of the chemical. Stability resultsshowed that while HQ was detectable in cultures at least for15 h, it was considerably more stable at 25 than at 100 or 250µM treatment levels. Results generated using any of thethree micronucleus assay variations showed no significant increasein micronuclei in cultures treated with 12.5–200 µMHQ. Colchicine, the positive control and a known spindle disrupter,produced elevated levels of micronuclei. At certain HQ concentrations,a block in cell division was observed, as evidenced by a decreasein percent binucleated cells and replicative index end-points.By varying the assay conditions, cell cultures overcame thisblock in division and divided at HQ concentrations up to 200µM, depending on the donor. The reversible block in celldivision observed may be a protective response, allowing cellsto recover without gross chromosomal damage. This study hassubstantially expanded the database with regard to the effectsof HQ treatment on lymphocytes.

¹ To whom correspondence should be addressed. Tel: +1 716 5884417; Fax: +1 716 722 7561; Email: j.caroline.english{at}kodak.com

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