Compound cytotoxicity profiling using quantitative high-throughput screening

Menghang Xia; Ruili Huang; Kristine L Witt; Noel Southall; Jennifer Fostel; Ming-Hsuang Cho; Ajit Jadhav; Cynthia S Smith; James Inglese; Christopher J Portier; Raymond R Tice; Christopher P Austin

doi:10.1289/ehp.10727

Compound cytotoxicity profiling using quantitative high-throughput screening

Environ Health Perspect. 2008 Mar;116(3):284-91. doi: 10.1289/ehp.10727.

Authors

Menghang Xia¹, Ruili Huang, Kristine L Witt, Noel Southall, Jennifer Fostel, Ming-Hsuang Cho, Ajit Jadhav, Cynthia S Smith, James Inglese, Christopher J Portier, Raymond R Tice, Christopher P Austin

Affiliation

¹ NIH Chemical Genomics Center, National Institutes of Health, Department of Health and Human Services, Bethesda, Maryland 20892-3370, USA.

Abstract

Background: The propensity of compounds to produce adverse health effects in humans is generally evaluated using animal-based test methods. Such methods can be relatively expensive, low-throughput, and associated with pain suffered by the treated animals. In addition, differences in species biology may confound extrapolation to human health effects.

Objective: The National Toxicology Program and the National Institutes of Health Chemical Genomics Center are collaborating to identify a battery of cell-based screens to prioritize compounds for further toxicologic evaluation.

Methods: A collection of 1,408 compounds previously tested in one or more traditional toxicologic assays were profiled for cytotoxicity using quantitative high-throughput screening (qHTS) in 13 human and rodent cell types derived from six common targets of xenobiotic toxicity (liver, blood, kidney, nerve, lung, skin). Selected cytotoxicants were further tested to define response kinetics.

Results: qHTS of these compounds produced robust and reproducible results, which allowed cross-compound, cross-cell type, and cross-species comparisons. Some compounds were cytotoxic to all cell types at similar concentrations, whereas others exhibited species- or cell type-specific cytotoxicity. Closely related cell types and analogous cell types in human and rodent frequently showed different patterns of cytotoxicity. Some compounds inducing similar levels of cytotoxicity showed distinct time dependence in kinetic studies, consistent with known mechanisms of toxicity.

Conclusions: The generation of high-quality cytotoxicity data on this large library of known compounds using qHTS demonstrates the potential of this methodology to profile a much broader array of assays and compounds, which, in aggregate, may be valuable for prioritizing compounds for further toxicologic evaluation, identifying compounds with particular mechanisms of action, and potentially predicting in vivo biological response.

Keywords: 1,536-well; NTP 1,408 compound library; PubChem; RT-CES; cell viability; qHTS.

Publication types

Research Support, N.I.H., Extramural
Research Support, N.I.H., Intramural

MeSH terms

Animals
Cell Survival / drug effects
Cells, Cultured
Humans
In Vitro Techniques
Mice
Rats
Reproducibility of Results
Toxicity Tests / methods*
Xenobiotics / toxicity*

Substances

Xenobiotics

Grants and funding

Intramural NIH HHS/United States