Gemcitabine (2 ' ,2 ' -difluoro-2 ' -deoxycytidine, or dFdC) is a promising anticancer agent with demonstrated clinical activity in solid tumours currently undergoing clinical trials. Despite extensive studies on the biochemical mechanism of action, cell cycle perturbations induced by dFdC have not yet been thoroughly investigated, apart from the expected inhibition of DNA synthesis. The aim of our study was to clarify whether cell population kinetics is a vital factor in the cytotoxicity of dFdC in single or repeated treatments and in the dfdC-cisplatin combination. Ovarian cancer cells growing in vitro were treated with dFdC for I hr in a range of concentrations from 10 nM to 10 pM. Cell kinetics was investigated by DNA-bromodeoxyuridine flow cytometry, using different experimental protocols to measure either the time course of DNA-synthesis inhibition or the fate of cells in G,, S or G,M at the time of dFdC treatment or 24 hr later, A modified sulforhodamine B test was used to assess the growth inhibition caused by dFdC given alone or with cisplatin, Although dFdC promptly inhibited DNA synthesis, cytotoxicity on proliferating cells was not specific for cells initially in the S phase. DNA synthesis was restored after a G, block of variable, dose-dependent length, but recycling cells were intercepted at the subsequent checlkpoints, resulting in delays in the G,M and G, phases. The activity of repeated treatment with dFdC+dFdC or dfdC+cisplatin was highly dependent on the interval length between them. These results suggest that the kinetics of cell recycling from a first dFdC treatment strongly affects the outcome of a second treatment with either dFdC itself or cisplatin. (C) 2001 Wiley-Liss, Inc.

Cell cycle effects of gemcitabine

D'Incalci M;
2001-01-01

Abstract

Gemcitabine (2 ' ,2 ' -difluoro-2 ' -deoxycytidine, or dFdC) is a promising anticancer agent with demonstrated clinical activity in solid tumours currently undergoing clinical trials. Despite extensive studies on the biochemical mechanism of action, cell cycle perturbations induced by dFdC have not yet been thoroughly investigated, apart from the expected inhibition of DNA synthesis. The aim of our study was to clarify whether cell population kinetics is a vital factor in the cytotoxicity of dFdC in single or repeated treatments and in the dfdC-cisplatin combination. Ovarian cancer cells growing in vitro were treated with dFdC for I hr in a range of concentrations from 10 nM to 10 pM. Cell kinetics was investigated by DNA-bromodeoxyuridine flow cytometry, using different experimental protocols to measure either the time course of DNA-synthesis inhibition or the fate of cells in G,, S or G,M at the time of dFdC treatment or 24 hr later, A modified sulforhodamine B test was used to assess the growth inhibition caused by dFdC given alone or with cisplatin, Although dFdC promptly inhibited DNA synthesis, cytotoxicity on proliferating cells was not specific for cells initially in the S phase. DNA synthesis was restored after a G, block of variable, dose-dependent length, but recycling cells were intercepted at the subsequent checlkpoints, resulting in delays in the G,M and G, phases. The activity of repeated treatment with dFdC+dFdC or dfdC+cisplatin was highly dependent on the interval length between them. These results suggest that the kinetics of cell recycling from a first dFdC treatment strongly affects the outcome of a second treatment with either dFdC itself or cisplatin. (C) 2001 Wiley-Liss, Inc.
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11699/67293
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