Temporary protection of rainbow trout gill epithelial cells from infection with viral haemorrhagic septicaemia virus IVb
被引:11
作者:
Al-Hussinee, L.
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Univ Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Al-Hussinee, L.
[1
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Pham, P. H.
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Univ Waterloo, Dept Biol, Waterloo, ON, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Pham, P. H.
[2
]
Russell, S.
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Novartis Anim Hlth Inc, Victoria, PE, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Russell, S.
[3
]
Tubbs, L.
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Novartis Anim Hlth Inc, Victoria, PE, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Tubbs, L.
[3
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Tafalla, C.
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CISA, INIA, Madrid, SpainUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Tafalla, C.
[4
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Bols, N. C.
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Univ Waterloo, Dept Biol, Waterloo, ON, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Bols, N. C.
[2
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Dixon, B.
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Univ Waterloo, Dept Biol, Waterloo, ON, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Dixon, B.
[2
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Lumsden, J. S.
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Univ Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, CanadaUniv Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
Lumsden, J. S.
[1
]
机构:
[1] Univ Guelph, Ontario Vet Coll, Dept Pathobiol, Fish Pathol Lab, Guelph, ON, Canada
[2] Univ Waterloo, Dept Biol, Waterloo, ON, Canada
The branchial epithelium is not only a primary route of entry for viral pathogens, but is also a site of viral replication and subsequent shedding may also occur from the gill epithelium. This study investigated the potential of agents known to stimulate innate immunity to protect rainbow trout epithelial cells (RTgill-W1) from infection with VHSV IVb. RTgill-W1 cells were pretreated with poly I:C, FuGENE((R)) HD+poly I:C, lipopolysaccharide (LPS), LPS+poly I:C or heat-killed VHSV IVb and then infected with VHSV IVb 4 days later. Cytopathic effect (CPE) was determined at 2, 3, 4, 7 and 11days post-infection. Virus in cells and supernatant was detected using quantitative reverse transcriptase polymerase chain reaction (qRT-PCR). All of the treatments delayed the onset of CPE (per cent of monolayer destruction), compared with untreated controls; however, killed VHSV or poly I:C combined with LPS was the most effective. Similarly, the detection of viral RNA in the supernatant was delayed, and the quantity was significantly (P<0.05) reduced by all treatments with the exception of LPS alone (4 days). Unlike many of the other treatments, pretreatment of RTgill-W1 with heat-killed VHSV did not upregulate interferon 1, 2 or MX 1 gene expression.