Performing a hepatic timing signal: glucocorticoids induce gper1a and gper1b expression and repress gclock1a and gbmal1a in the liver of goldfish

Glucocorticoids have been recently proposed as input signals of circadian system, although the underlying molecular mechanism remains unclear. This work investigates the role of glucocorticoids as modulators of clock genes expression in the liver of goldfish. In fish maintained under a 12L:12D photo...

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Published in:Journal of comparative physiology. B, Biochemical, systemic, and environmental physiology Biochemical, systemic, and environmental physiology, 2016-01, Vol.186 (1), p.73-82
Main Authors: Sánchez-Bretaño, Aída, Callejo, María, Montero, Marta, Alonso-Gómez, Ángel L., Delgado, María J., Isorna, Esther
Format: Article
Language:English
Subjects:
Animal Physiology
Animals
Biochemistry
Biomedical and Life Sciences
Biomedicine
Body weight
Carassius auratus
Circadian rhythms
CLOCK Proteins - genetics
CLOCK Proteins - metabolism
Dexamethasone - administration & dosage
Dexamethasone - pharmacology
Drug Administration Schedule
Fish Proteins - genetics
Fish Proteins - metabolism
Freshwater
Gene expression
Gene Expression Regulation - drug effects
Gene Expression Regulation - physiology
Glucocorticoids - pharmacology
Goldfish - metabolism
Hormones
Human Physiology
Hydrocortisone - pharmacology
Injection
Life Sciences
Liver
Liver - metabolism
Metabolism
Original Paper
Oscillators
Period Circadian Proteins - genetics
Period Circadian Proteins - metabolism
RNA, Messenger - genetics
RNA, Messenger - metabolism
Zoology
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Summary:Glucocorticoids have been recently proposed as input signals of circadian system, although the underlying molecular mechanism remains unclear. This work investigates the role of glucocorticoids as modulators of clock genes expression in the liver of goldfish. In fish maintained under a 12L:12D photoperiod, an intraperitoneal injection at Zeitgeber Time 2 of a glucocorticoid analog, dexamethasone (1 μg/g body weight) induced per1 genes while decreased gbmal1a and gclock1a expression in the liver at 8 h post-injection. A 4-h in vitro exposure of goldfish liver to cortisol (0.1–10 μM) also induced gper1 genes in a concentration-dependent manner. Similarly, the exposure of the goldfish cultured liver to dexamethasone produced a concentration-dependent induction of gper1 genes. Moreover, this glucocorticoid analog led to a decrease in gbmal1a and gclock1a transcripts, while the other clock genes analyzed were unaffected. The induction of gper1a and gper1b by dexamethasone in vitro was observed at short times (2 h), whereas the reductions of gbmal1a and gclock1a transcripts needed longer exposure times (8 h) to the glucocorticoid to be significant. Additionally, a 2-h exposure to dexamethasone in the liver culture was enough to extend the induction of per genes for more than 12 h. Present results indicate that gper1 genes are targets for glucocorticoids in the regulation of goldfish hepatic oscillator, as previously reported in mammals, suggesting a conserved role of glucocorticoids in the functional organization of the peripheral circadian system in vertebrates. The repression of clock1a and bmal1a is not so well established, and suggests that other clock genes could be glucocorticoid targets in the goldfish liver.
ISSN:0174-1578
1432-136X
DOI:10.1007/s00360-015-0936-2