Transcriptional changes in oysters Crassostrea brasiliana exposed to phenanthrene at different salinities

Flávia Lucena Zacchi; Daína de Lima; Fabrício Flores-Nunes; Jacó Joaquim Mattos; Karim Hahn Lüchmann; Carlos Henrique Araújo de Miranda Gomes; Márcia Caruso Bícego; Satie Taniguchi; Silvio Tarou Sasaki; Afonso Celso Dias Bainy

doi:10.1016/j.aquatox.2016.12.016

Transcriptional changes in oysters Crassostrea brasiliana exposed to phenanthrene at different salinities

Aquat Toxicol. 2017 Feb:183:94-103. doi: 10.1016/j.aquatox.2016.12.016. Epub 2016 Dec 21.

Affiliations

¹ Laboratory of Biomarkers of Aquatic Contamination and Immunochemistry - LABCAI, Federal University Santa Catarina, Florianópolis, Brazil.
² Aquaculture Pathology Research Center - NEPAQ, Federal University of Santa Catarina, Florianópolis, Brazil.
³ Laboratory of Biochemistry and Molecular Biology - LBBM, Fishery Engineering Department, Santa Catarina State University, Laguna, Brazil.
⁴ Laboratory of Marine Mollusks - LMM, Federal University of Santa Catarina, Florianópolis, Brazil.
⁵ Laboratory of Marine Organic Chemistry - LABQOM, Oceanographic Institute, University of São Paulo, São Paulo, Brazil.
⁶ Laboratory of Biomarkers of Aquatic Contamination and Immunochemistry - LABCAI, Federal University Santa Catarina, Florianópolis, Brazil. Electronic address: afonso.bainy@ufsc.br.

PMID: 28040644
DOI: 10.1016/j.aquatox.2016.12.016

Abstract

Euryhaline animals from estuaries, such as the oyster Crassostrea brasiliana, show physiological mechanisms of adaptation to tolerate salinity changes. These ecosystems receive constant input of xenobiotics from urban areas, including polycyclic aromatic hydrocarbons (PAHs), such as phenanthrene (PHE). In order to understand the influence of salinity on the molecular responses of C. brasiliana exposed to PHE, oysters were acclimatized to different salinities (35, 25 and 10) for 15days and then exposed to 100μgL^-1 PHE for 24h and 96h. Control groups were kept at the same salinities without PHE. Oysters were sampled for chemical analysis and the gills were excised for mRNA quantification by qPCR. Transcript levels of different genes were measured, including some involved in oxidative stress pathways, phases I and II of the xenobiotic biotransformation systems, amino acid metabolism, fatty acid metabolism and aryl hydrocarbon receptor nuclear translocator putative gene. Higher transcript levels of Sulfotransferase-like gene (SULT-like) were observed in oysters exposed to PHE at salinity 10 compared to control (24h and 96h); cytochrome P450 isoforms (CYP2AU1, CYP2-like1) were more elevated in oysters exposed for 24h and CYP2-like2 after 96h of oysters exposed to PHE at salinity 10 compared to control. These results are probably associated to an enhanced Phase I biotransformation activity required for PHE detoxification under hyposmotic stress. Higher transcript levels of CAT-like, SOD-like, GSTm-like (96h) and GSTΩ-like (24h) in oysters kept at salinity 10 compared to organisms at salinities 25 and/or 35 are possibly related to enhaced ROS production. The transcription of these genes were not affected by PHE exposure. Amino acid metabolism-related genes (GAD-like (24h), GLYT-like, ARG-like (96h) and TAUT-like at 24h and 96h) also showed different transcription levels among organisms exposed to different salinities, suggesting their important role for oyster salinity adaptation, which is not affected by exposure to these levels of PHE.

Keywords: Estuaries; Mangrove oyster; PAHs; Phenanthrene; Salinity; qPCR.

MeSH terms

Animals
Biotransformation
Crassostrea / drug effects*
Crassostrea / genetics
Cytochrome P-450 Enzyme System / genetics
Estuaries
Gills / drug effects
Gills / metabolism
Phenanthrenes / toxicity*
Salinity*
Transcription, Genetic / drug effects
Water Pollutants, Chemical / toxicity*
Xenobiotics / metabolism

Substances

Phenanthrenes
Water Pollutants, Chemical
Xenobiotics
phenanthrene
Cytochrome P-450 Enzyme System