AI Article Synopsis

  • High-throughput screening (HTS) is a new way to check if chemicals are safe to use, and using cell-based models instead of animals is becoming popular.
  • Researchers created a new process to analyze small cell samples from human liver cells (HepaRG) quickly and effectively using advanced equipment.
  • The study showed that this method is good at detecting changes caused by toxic substances and can help in future testing to keep people safe from harmful chemicals.

Article Abstract

Introduction: High-throughput screening (HTS) is emerging as an approach to support decision-making in chemical safety assessments. In parallel, in vitro metabolomics is a promising approach that can help accelerate the transition from animal models to high-throughput cell-based models in toxicity testing.

Objective: In this study we establish and evaluate a high-throughput metabolomics workflow that is compatible with a 96-well HTS platform employing 50,000 hepatocytes of HepaRG per well.

Methods: Low biomass cell samples were extracted for metabolomics analyses using a newly established semi-automated protocol, and the intracellular metabolites were analysed using a high-resolution spectral-stitching nanoelectrospray direct infusion mass spectrometry (nESI-DIMS) method that was modified for low sample biomass.

Results: The method was assessed with respect to sensitivity and repeatability of the entire workflow from cell culturing and sampling to measurement of the metabolic phenotype, demonstrating sufficient sensitivity (> 3000 features in hepatocyte extracts) and intra- and inter-plate repeatability for polar nESI-DIMS assays (median relative standard deviation < 30%). The assays were employed for a proof-of-principle toxicological study with a model toxicant, cadmium chloride, revealing changes in the metabolome across five sampling times in the 48-h exposure period. To allow the option for lipidomics analyses, the solvent system was extended by establishing separate extraction methods for polar metabolites and lipids.

Conclusions: Experimental, analytical and informatics workflows reported here met pre-defined criteria in terms of sensitivity, repeatability and ability to detect metabolome changes induced by a toxicant and are ready for application in metabolomics-driven toxicity testing to complement HTS assays.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8743266PMC
http://dx.doi.org/10.1007/s11306-021-01867-3DOI Listing

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