J. P. Finn scite author profile

J. P. Finn

4Publications

103Citation Statements Received

59Citation Statements Given

How they've been cited

217

How they cite others

Affiliations

Genomics (United Kingdom), University of Saskatchewan, University of California, Davis

Publications

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The inflammatory response of rainbow trout*

Finn

Nielson²

1971

Journal of Fish Biology

120

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The basic responses of piscine tissues to inflammatory agents were investigated, using light microscopy. Tissue sections, smears and blood smears were examined. The period studied was from 3 h to 16 days after initial injury at 15" C . The piscine inflammatory response was compared to that of mammals, especially that of mice. The responses examined were basically similar to those of msmmals. They varied by being less intense and slower to appear and resolve.

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The effect of temperature variation on the inflammatory response of rainbow trout

Finn

Nielsen

1971

The Journal of Pathology

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Endocrine Disruption Screening by Protein and Gene Expression of Vitellogenin in Freshly Isolated and Cryopreserved Rainbow Trout Hepatocytes

Markell

Mingoia

Peterson

et al. 2014

Chem. Res. Toxicol.

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Xenobiotics may activate the estrogen receptor, resulting in alteration of normal endocrine functions in animals and humans. Consequently, this necessitates development of assay end points capable of identifying estrogenic xenobiotics. In the present study, we screened the potential estrogenicity of chemicals via their ability to induce vitellogenin (VTG) expression in cultured primary hepatocytes from male trout. A routine method for VTG detection measures the secretion of the protein by enzyme-linked immunosorbent assay (ELISA) in freshly isolated trout hepatocytes. However, this lengthy (6 days) culturing procedure requires that hepatocyte isolation is performed each time the assay is run. We optimized this methodology by investigating the utility of cryopreserved hepatocytes, shortening the incubation time, performing a quantitative real-time PCR (qPCR) method for VTG quantification, and verifying the model system with reference chemicals 17β-estradiol, estrone, diethylstilbestrol, hexestrol, genistein, and a negative control, corticosterone. To test the performance of both freshly isolated and cryopreserved hepatocytes, mRNA was collected from hepatocytes following 24 h treatment for VTG gene expression analysis, whereas cell culture media was collected for a VTG ELISA 96 h post-treatment. EC50 values were obtained for each reference chemical except for corticosterone, which exhibited no induction of VTG gene or protein level. Our results show linear concordance between ELISA and qPCR detection methods. Although there was approximately 50% reduction in VTG inducibility following cryopreservation, linear concordance of EC50 values was found between freshly isolated and cryopreserved hepatocytes, indicating that cryopreservation does not alter the functional assessment of estrogen receptor activation and therefore VTG expression. These studies demonstrate that qPCR is a sensitive and specific method for detecting VTG gene expression that can be used together with cryopreserved trout hepatocytes for screening estrogenic chemicals, resulting in a reduction of the time required to perform the assay and enabling greater access to the model system through the approach of cryopreservation.

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Brown fat tumours (hibernomas) in rats: histopathological and ultrastructural study

Zubaidy

Finn²

1983

Lab Anim

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J. P. Finn

The inflammatory response of rainbow trout*

The effect of temperature variation on the inflammatory response of rainbow trout

Endocrine Disruption Screening by Protein and Gene Expression of Vitellogenin in Freshly Isolated and Cryopreserved Rainbow Trout Hepatocytes

Brown fat tumours (hibernomas) in rats: histopathological and ultrastructural study

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