Pilot testing and optimization of a larval fathead minnow high throughput transcriptomics assay

Daniel L Villeneuve; Michelle Le; Monique Hazemi; Adam Biales; David C Bencic; Kendra Bush; Robert Flick; John Martinson; Mackenzie Morshead; Kelvin Santana Rodriguez; Kelsey Vitense; Kevin Flynn

doi:10.1016/j.crtox.2022.100099

Pilot testing and optimization of a larval fathead minnow high throughput transcriptomics assay

Curr Res Toxicol. 2022 Dec 22:4:100099. doi: 10.1016/j.crtox.2022.100099. eCollection 2023.

Affiliations

¹ US Environmental Protection Agency, Great Lakes Toxicology and Ecology Division, Duluth, MN 55804, USA.
² Oak Ridge Institute for Science and Education (ORISE) Research Participant, US Environmental Protection Agency Great Lakes Toxicology and Ecology Division, Duluth, MN 55804, USA.
³ US Environmental Protection Agency, Great Lakes Toxicology and Ecology Division, Cincinnati, OH 45220, USA.
⁴ US Environmental Protection Agency, Scientific Computing and Data Curation Division, Duluth, MN 55804, USA.

Abstract

Concentrations at which global gene expression profiles in cells or animals exposed to a test substance start to differ significantly from those of controls have been proposed as an alternative point of departure for use in screening level hazard assessment. The present study describes pilot testing of a high throughput compatible transcriptomics assay with larval fathead minnows. One day post hatch fathead minnows were exposed to eleven different concentrations of three metals, three selective serotonin reuptake inhibitors, and four neonicotinoid-like compounds for 24 h and concentration response modeling was applied to whole body gene expression data. Transcriptomics-based points of departure (tPODs) were consistently lower than effect concentrations reported in apical endpoint studies in fish. However, larval fathead minnow-based tPODs were not always lower than concentrations reported to elicit apical toxicity in other aquatic organisms like crustaceans or insects. Random in silico subsampling of data from the pilot assays was used to evaluate various assay design and acceptance considerations such as transcriptome coverage, number of replicate individuals to sequence per treatment, and minimum number of differentially expressed genes to produce a reliable tPOD estimate. Results showed a strong association between the total number of genes for which a concentration response relationship could be derived and the overall variability in the resulting tPOD estimates. We conclude that, for our current assay design and analysis pipeline, tPODs based on fewer than 15 differentially expressed genes are likely to be unreliable for screening and that interindividual variability in gene expression profiles appears to be a more significant driver of tPOD variability than sample size alone. Results represent initial steps toward developing high throughput transcriptomics assays for use in ecological hazard screening.

Keywords: BMD, Benchmark dose; Benchmark dose; Computational toxicology; DEGs, Differentially expressed genes; ECOTOX knowledgebase; Fish; HTTr, High throughput transcriptomics; RIN, RNA integrity number; RNA sequencing; RNAseq, RNA sequencing; SSRI, Selective serotonin reuptake inhibitor; ToxCast, US EPA Toxicity Forecaster; Transcriptomics-based point of departure; cDNA, Complementary DNA; eco-HTTr, Ecological high throughput transcriptomics; tPOD, Transcriptomics-based point of departure.