Thimerosal Induces DNA Breaks, Caspase-3 Activation, Membrane Damage, and Cell Death in Cultured Human Neurons and Fibroblasts

Thimerosal Induces DNA Breaks, Caspase-3 Activation, Membrane Damage, and Cell Death in Cultured Human Neurons and Fibroblasts

Thimerosal is an organic mercurial compound used as a preservative in biomedical preparations. Little is known about the reactions of human neuronal and skin cells to its micro- and nanomolar concentrations, which can occur after using thimerosal-containing products. A useful combination of fluoresc...

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Veröffentlicht in:Toxicological sciences 2003-08, Vol.74 (2), p.361-368
Hauptverfasser: Baskin, David S., Ngo, Hop, Didenko, Vladimir V.
Format: Artikel
Sprache:eng
Schlagworte:
active caspase-3
apoptosis
Apoptosis - drug effects
Biological and medical sciences
Caspase 3
Caspase Inhibitors
Caspases - biosynthesis
Cell Membrane - drug effects
Cell Nucleus - drug effects
Cell Nucleus - pathology
Cell Survival - drug effects
Cells, Cultured
Cerebral Cortex - cytology
Cerebral Cortex - drug effects
DAPI
DNA breaks
DNA Damage
Dose-Response Relationship, Drug
Drug toxicity and drugs side effects treatment
fibroblasts
Fibroblasts - drug effects
Fibroblasts - enzymology
Fibroblasts - pathology
Humans
In Situ Nick-End Labeling
Infant, Newborn
Male
Medical sciences
membrane damage
neurons
Neurons - drug effects
Neurons - enzymology
Neurons - pathology
Pharmacology. Drug treatments
Preservatives, Pharmaceutical - toxicity
Skin - cytology
Skin - drug effects
thimerosal
Thimerosal - toxicity
toxicity
Toxicity: nervous system and muscle
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Zusammenfassung:Thimerosal is an organic mercurial compound used as a preservative in biomedical preparations. Little is known about the reactions of human neuronal and skin cells to its micro- and nanomolar concentrations, which can occur after using thimerosal-containing products. A useful combination of fluorescent techniques for the assessment of thimerosal toxicity is introduced. Short-term thimerosal toxicity was investigated in cultured human cerebral cortical neurons and in normal human fibroblasts. Cells were incubated with 125-nM to 250-μM concentrations of thimerosal for 45 min to 24 h. A 4′, 6-diamidino-2-phenylindole dihydrochloride (DAPI) dye exclusion test was used to identify nonviable cells and terminal transferase-based nick-end labeling (TUNEL) to label DNA damage. Detection of active caspase-3 was performed in live cell cultures using a cell-permeable fluorescent caspase inhibitor. The morphology of fluorescently labeled nuclei was analyzed. After 6 h of incubation, the thimerosal toxicity was observed at 2 μM based on the manual detection of the fluorescent attached cells and at a 1-μM level with the more sensitive GENios Plus Multi-Detection Microplate Reader with Enhanced Fluorescence. The lower limit did not change after 24 h of incubation. Cortical neurons demonstrated higher sensitivity to thimerosal compared to fibroblasts. The first sign of toxicity was an increase in membrane permeability to DAPI after 2 h of incubation with 250 μM thimerosal. A 6-h incubation resulted in failure to exclude DAPI, generation of DNA breaks, caspase-3 activation, and development of morphological signs of apoptosis. We demonstrate that thimerosal in micromolar concentrations rapidly induce membrane and DNA damage and initiate caspase-3–dependent apoptosis in human neurons and fibroblasts. We conclude that a proposed combination of fluorescent techniques can be useful in analyzing the toxicity of thimerosal.
ISSN:1096-6080
1096-0929
DOI:10.1093/toxsci/kfg126