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Enhancement of the chromosome-damaging action of ascorbate by transition metals.
87
Citations
25
References
1979
Year
OocyteCytogeneticsGeneticsMolecular BiologyRedox BiologyOxidative StressInduced Chromosome AberrationsChromosome AberrationsBiological Inorganic ChemistryBiochemistryCell DivisionMeiosisCell BiologyChromatinNatural SciencesTransition MetalsMetalloproteinBioactive MetalChromosome BiologyPrepared AscorbateMedicine
Freshly prepared ascorbate inhibited mitosis and induced chromosome aberrations in cultured Chinese hamster ovary cells. Cu(II) and Mn(II) (10(-4) or 10(-5) M) enhanced both actions. Fe(II) and Fe(III) (10(-4) or 10(-5) M) reduced or abolished the mitosis-inhibiting action of ascorbate. At 10(-4) M, Fe(II) and Fe(III) strongly enhanced the chromosome-damaging capacity of ascorbate. Up to 100% of all examined metaphase plates had multiple chromosome exchanges or breaks. Since the cytostatic and clastogenic effect of ascorbate of H2O2 to induce chromosome aberrations was examined. H2O2 and a H2O2: Fe(II) mixture (Fenton reagent) induced chromosome breaks and exchanges but to a lesser degree than did ascorbate: Cu(II), Mn(II), Fe(II), or Fe(III) mixtures. Whether the strong chromosome damaging capacity of ascorbate plus transition metals as seen in the in vitro test system poses a health hazard only properly designed in vivo studies can reveal.
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