Environmental monitoring of urban streams using a primary fish gill cell culture system (FIGCS)

The primary fish gill cell culture system (FIGCS) is an in vitro technique which has the potential to replace animals in whole effluent toxicity tests. In the current study FIGCS were transported into the field and exposed to filtered (0.2μm) river water for 24h from 4 sites, on 2 different sampling...

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Bibliographic Details
Published in:Ecotoxicology and environmental safety 2015-10, Vol.120, p.279-285
Main Authors: Schnell, Sabine, Bawa-Allah, Kafilat, Otitoloju, Adebayo, Hogstrand, Christer, Miller, Thomas H., Barron, Leon P., Bury, Nic R.
Format: Article
Language:English
Subjects:
3Rs
Animals
Cell culture
Cells, Cultured
cyp1a1
cyp3
Cytochrome P-450 CYP1A1 - genetics
Cytochrome P-450 CYP1A1 - metabolism
Environmental monitoring
Environmental Monitoring - methods
Fish
Fishes
Gene Expression Regulation
Gills - cytology
Gills - drug effects
Gills - metabolism
Metallothionein
Metallothionein - genetics
Metallothionein - metabolism
Rivers - chemistry
Toxicity Tests
United Kingdom
Water Pollutants, Chemical - analysis
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Summary:The primary fish gill cell culture system (FIGCS) is an in vitro technique which has the potential to replace animals in whole effluent toxicity tests. In the current study FIGCS were transported into the field and exposed to filtered (0.2μm) river water for 24h from 4 sites, on 2 different sampling dates. Sites 1 and 2 are situated in an urban catchment (River Wandle, London, UK) with site 1 downstream of a sewage treatment work; site 3 is located in a suburban park (River Cray, Kent, UK), and site 4 is more rural (River Darent, Kent, UK). The change in transepithelial electrical resistance (TER), the expression of the metal responsive genes metallothionein A (mta) and B (mtb), cytochrome P450 1A1 (cyp1a1) and 3A27 (cyp3a27), involved in phase 1 metabolism, were assessed following exposure to sample water for 24h. TER was comparable between FIGCS exposed to 0.2μm filtered river water and those exposed to synthetic moderately soft water for 24h. During the first sampling time, there was an increase in mta, cyp1a1 and cyp3a27 gene expression in epithelium exposed to water from sites 1 and 2, and during the second sampling period an increase in cyp3a27 gene expression at sites 1 and 4. Urban river water is a complex mixture of contaminants (e.g., metals, pesticides, pharmaceuticals and polyaromatic hydrocarbons) and the increase in the expression of genes encoding mta, cyp1a1 and cyp3a27 in FIGCS is indicative of the presence of biologically active pollutants. •A primary gill cell cultures system tolerates filtered urban river water.•The gill cells showed an increase in metallothionein gene expression.•The gill cells showed an increase in cyp1a1 and cyp3a27 gene expression.•The response of the gill cell culture system could be used for environmental monitoring purposes.
ISSN:0147-6513
1090-2414
DOI:10.1016/j.ecoenv.2015.06.012