| Literature DB >> 32867820 |
Alison M Pecquet1, Andrew Maier2, Susan Kasper1, Saulius Sumanas3,4, Jagjit Yadav5.
Abstract
OBJECTIVE: Perfluorooctanoic acid (PFOA) is a ubiquitous environmental contaminant and a known immune suppressant in humans and experimental animal models. Studies on PFOA have focused on suppression of the adaptive immune response; however, little is known of the impact on innate immunity, especially during embryogenesis. Therefore, we utilized the zebrafish chemotaxis assay coupled with in situ hybridization for myeloperoxidase expression to determine the effects of PFOA exposure on neutrophil migration in the developing zebrafish embryo. Zebrafish embryos are a well-established in vivo model that exhibit high homology with the development of human innate immunity.Entities:
Keywords: Chemotaxis; Immunotoxicity; In situ hybridization; In vivo; Lethal concentration in 50% of embryos (LC50); Myeloperoxidase; Neutrophil; PFOA; Wounding; Zebrafish
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Year: 2020 PMID: 32867820 PMCID: PMC7460781 DOI: 10.1186/s13104-020-05255-3
Source DB: PubMed Journal: BMC Res Notes ISSN: 1756-0500
Fig. 1Concentration–response graph showing acute toxicity and the 48-h LC50 of PFOA in zebrafish embryos. Concentration of PFOA (X-axis) plotted by the probability of mortality (Y-axis) in zebrafish embryos exposed for 48 h resulted in a derived LC50 of 300 mg/L using the ecotoxicity package in R. Each data point represents the average of the replicates from one experiment, and data are presented from five repeated experiments using a range of PFOA concentrations. Each concentration was tested a minimum of three times. Note that the high concentrations all had 100% mortality and those data points overlap
Fig. 2Zebrafish embryos treated with PFOA showed a significant decrease in neutrophil accumulation following wounding. The zebrafish chemotaxis assay showed that PFOA treatment reduced the neutrophil number migrating to the wound site in 48-hpf zebrafish embryos. a–c, Representative images of ISH-tagged neutrophils migrating to the wound region (dotted line), where a wounded embryos treated with vehicle control (DMSO) (n = 36); b wounded embryos treated with PFOA concentration at 0.5 mg/L (n = 35); and c wounded embryos treated with PFOA concentration at 5.0 mg/L (n = 31). d) The averaged quantification of neutrophil migration in each treatment (error bars represent standard deviation across three replicate experiments). Neutrophil migration in both 0.5 and 5.0 mg/L PFOA was significantly decreased when compared to control using ANOVA, with p-values of 0.0025 and < 0.0001, respectively. The DMSO control never exceeded 0.5% v/v and was constant across all treatments. See Additional file 1: File S1 for detailed methodology