Author: Park, J W; Moon, C H; Harmache, A; Wargo, A R; Purcell, M K; Bremont, M; Kurath, G
Title: Restricted growth of Uâ€type infectious haematopoietic necrosis virus (IHNV) in rainbow trout cells may be linked to casein kinase II activity Cord-id: 6j56ba9i Document date: 2011_1_17
ID: 6j56ba9i
Snippet: Previously, we demonstrated that a representative M genogroup type strain of infectious haematopoietic necrosis virus (IHNV) from rainbow trout grows well in rainbow troutâ€derived RTGâ€2 cells, but a U genogroup type strain from sockeye salmon has restricted growth, associated with reduced genome replication and mRNA transcription. Here, we analysed further the mechanisms for this growth restriction of Uâ€type IHNV in RTGâ€2 cells, using strategies that assessed differences in viral genes,
Document: Previously, we demonstrated that a representative M genogroup type strain of infectious haematopoietic necrosis virus (IHNV) from rainbow trout grows well in rainbow troutâ€derived RTGâ€2 cells, but a U genogroup type strain from sockeye salmon has restricted growth, associated with reduced genome replication and mRNA transcription. Here, we analysed further the mechanisms for this growth restriction of Uâ€type IHNV in RTGâ€2 cells, using strategies that assessed differences in viral genes, host immune regulation and phosphorylation. To determine whether the viral glycoprotein (G) or nonâ€virion (NV) protein was responsible for the growth restriction, four recombinant IHNV viruses were generated in which the G gene of an infectious IHNV clone was replaced by the G gene of U†or Mâ€type IHNV and the NV gene was replaced by NV of U†or Mâ€type IHNV. There was no significant difference in the growth of these recombinants in RTGâ€2 cells, indicating that G and NV proteins are not major factors responsible for the differential growth of the U†and Mâ€type strains. Poly I:C pretreatment of RTGâ€2 cells suppressed the growth of both U†and Mâ€type IHNV, although the M virus continued to replicate at a reduced level. Both viruses induced type 1 interferon (IFN1) and the IFN1 stimulated gene Mx1, but the expression levels in Mâ€infected cells were significantly higher than in Uâ€infected cells and an inhibitor of the IFN1â€inducible protein kinase PKR, 2â€aminopurine (2â€AP), did not affect the growth of U†or Mâ€type IHNV in RTGâ€2 cells. These data did not indicate a role for the IFN1 system in the restricted growth of Uâ€type IHNV in RTGâ€2 cells. Prediction of kinaseâ€specific phosphorylation sites in the viral phosphoprotein (P) using the NetPhosK program revealed differences between U†and Mâ€type P genes at five phosphorylation sites. Pretreatment of RTGâ€2 cells with a PKC inhibitor or a p38MAPK inhibitor did not affect the growth of the U†and Mâ€type viruses. However, 100 μm of the casein kinase II (CKII) inhibitor, 5,6â€dichloroâ€1â€Î²â€dâ€ribofuranosylbenzimidazole (DRB), reduced the titre of the U type 8.3â€fold at 24 h postâ€infection. In contrast, 100 μm of the CKII inhibitor reduced the titre of the M type only 1.3â€fold at 48 h postâ€infection. Our data suggest that the different growth of U†and Mâ€type IHNV in RTGâ€2 cells may be linked to a differential requirement for cellular protein kinases such as CKII for their growth.
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