A Systematic Assessment of Mitochondrial Function Identified Novel Signatures for Drug-Induced Mitochondrial Disruption in Cells | Zendy

Nianyu Li | Zendy; Elisa Oquendo | Zendy; Roderick Capaldi | Zendy; J. Paul Robinson | Zendy; Yudong D. He | Zendy; Hisham K. Hamadeh | Zendy; Cynthia A. Afshari | Zendy; Ruth Lightfoot-Dunn | Zendy; Padma Kumar Narayanan | Zendy

Open Access

A Systematic Assessment of Mitochondrial Function Identified Novel Signatures for Drug-Induced Mitochondrial Disruption in Cells

Author(s) -

Nianyu Li,

Elisa Oquendo,

Roderick Capaldi,

J. Paul Robinson,

Yudong D. He,

Hisham K. Hamadeh,

Cynthia A. Afshari,

Ruth Lightfoot-Dunn,

Padma Kumar Narayanan

Publication year - 2014

Publication title -

toxicological sciences

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 1.352

H-Index - 183

eISSN - 1096-6080

pISSN - 1096-0929

DOI - 10.1093/toxsci/kfu176

Subject(s) - viability assay , mitochondrion , mitochondrial ros , biology , reactive oxygen species , mitochondrial respiratory chain , microbiology and biotechnology , glutathione , cell culture , inner mitochondrial membrane , mitochondrial matrix , respiratory chain , mitochondrial permeability transition pore , biochemistry , cell , apoptosis , programmed cell death , cytosol , genetics , enzyme

Mitochondrial perturbation has been recognized as a contributing factor to various drug-induced organ toxicities. To address this issue, we developed a high-throughput flow cytometry-based mitochondrial signaling assay to systematically investigate mitochondrial/cellular parameters known to be directly impacted by mitochondrial dysfunction: mitochondrial membrane potential (MMP), mitochondrial reactive oxygen species (ROS), intracellular reduced glutathione (GSH) level, and cell viability. Modulation of these parameters by a training set of compounds, comprised of established mitochondrial poisons and 60 marketed drugs (30 nM to 1mM), was tested in HL-60 cells (a human pro-myelocytic leukemia cell line) cultured in either glucose-supplemented (GSM) or glucose-free (containing galactose/glutamine; GFM) RPMI-1640 media. Post-hoc bio-informatic analyses of IC50 or EC50 values for all parameters tested revealed that MMP depolarization in HL-60 cells cultured in GSM was the most reliable parameter for determining mitochondrial dysfunction in these cells. Disruptors of mitochondrial function depolarized MMP at concentrations lower than those that caused loss of cell viability, especially in cells cultured in GSM; cellular GSH levels correlated more closely to loss of viability in vitro. Some mitochondrial respiratory chain inhibitors increased mitochondrial ROS generation; however, measuring an increase in ROS alone was not sufficient to identify mitochondrial disruptors. Furthermore, hierarchical cluster analysis of all measured parameters provided confirmation that MMP depletion, without loss of cell viability, was the key signature for identifying mitochondrial disruptors. Subsequent classification of compounds based on ratios of IC50s of cell viability:MMP determined that this parameter is the most critical indicator of mitochondrial health in cells and provides a powerful tool to predict whether novel small molecule entities possess this liability.

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