Cytosolic Ca§ssup§2+§esup§ shifts as early markers of cytotoxicity

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Abstract

The determination of the cytotoxic potential of new and so far unknown compounds as well as their metabolites is fundamental in risk assessment. A variety of strategic endpoints have been defined to describe toxin-cell interactions, leading to prediction of cell fate. They involve measurement of metabolic endpoints, bio-energetic parameters or morphological cell modifications. Here, we evaluated alterations of the free cytosolic Ca§ssup§2+§esup§ homeostasis using the Fluo-4 dye and compared results with the metabolic cell viability assay Alamar Blue. We investigated a panel of toxins (As§ssub§2§esub§O§ ssub§3§esub§, gossypol, H§ssub§2§esub§O§ ssub§2§esub§, staurosporine, and titanium(IV)-salane complexes) in four different mammalian cell lines covering three different species (human, mouse, and African green monkey). All tested compounds induced an increase in free cytosolic Ca§ssup§2+§esup§ within the first 5 s after toxin application. Cytosolic Ca§ssup§2+§esup§ shifts occurred independently of the chemical structure in all tested cell systems and were persistent up to 3 h. The linear increase of free cytosolic Ca§ssup§2+§esup§ within the first 5 s of drug treatment correlates with the EC§ssub§25§esub§ and EC§ssub§75§esub§ values obtained in Alamar Blue assays one day after toxin exposure. Moreover, a rise of cytosolic Ca§ssup§ 2+§esup§ was detectable independent of induced cell death mode as assessed by caspase and poly(ADP-ribose) polymerase (PARP) activity in HeLa versus MCF-7 cells at very low concentrations. In conclusion, a cytotoxicity assay based on Ca§ssup§2+§esup§ shifts has a low limit of detection (LOD), is less time consuming (at least 24 times faster) compared to the cell viability assay Alamar Blue and is suitable for high-troughput- screening (HTS). © 2013 Wyrsch et al.; licensee BioMed Central Ltd.

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Wyrsch, P., Blenn, C., Pesch, T., Beneke, S., & Althaus, F. R. (2013). Cytosolic Ca§ssup§2+§esup§ shifts as early markers of cytotoxicity. Cell Communication and Signaling, 11(1). https://doi.org/10.1186/1478-811X-11-11

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