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Open AccessJournal ArticleDOI

Newcastle disease virus (NDV)-based assay demonstrates interferon-antagonist activity for the NDV V protein and the Nipah virus V, W, and C proteins.

TLDR
It is shown that expression of the NDV V protein or the Nipah virus V, W, or C proteins rescues NDV-GFP replication in the face of the transfection-induced IFN response, and that the NDVs could be used to screen proteins expressed from plasmids for the ability to counteract the host cellIFN response.
Abstract
We have generated a recombinant Newcastle disease virus (NDV) that expresses the green fluorescence protein (GFP) in infected chicken embryo fibroblasts (CEFs). This virus is interferon (IFN) sensitive, and pretreatment of cells with chicken alpha/beta IFN (IFN-α/β) completely blocks viral GFP expression. Prior transfection of plasmid DNA induces an IFN response in CEFs and blocks NDV-GFP replication. However, transfection of known inhibitors of the IFN-α/β system, including the influenza A virus NS1 protein and the Ebola virus VP35 protein, restores NDV-GFP replication. We therefore conclude that the NDV-GFP virus could be used to screen proteins expressed from plasmids for the ability to counteract the host cell IFN response. Using this system, we show that expression of the NDV V protein or the Nipah virus V, W, or C proteins rescues NDV-GFP replication in the face of the transfection-induced IFN response. The V and W proteins of Nipah virus, a highly lethal pathogen in humans, also block activation of an IFN-inducible promoter in primate cells. Interestingly, the amino-terminal region of the Nipah virus V protein, which is identical to the amino terminus of Nipah virus W, is sufficient to exert the IFN-antagonist activity. In contrast, the anti-IFN activity of the NDV V protein appears to be located in the carboxy-terminal region of the protein, a region implicated in the IFN-antagonist activity exhibited by the V proteins of mumps virus and human parainfluenza virus type 2.

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Importance of the anti-interferon capacity of Sendai virus C protein for pathogenicity in mice.

TL;DR: It was found that the anti-IFN capacity of the SeV C protein was indispensable for pathogenicity in mice, and the results show that the innate immunity contributed to elimination of SeV in early stages of infection in the absence of anti- IFN capacity.
Journal ArticleDOI

Nipah Virus C and W Proteins Contribute to Respiratory Disease in Ferrets

TL;DR: Using a ferret model, the roles of the NiV C and W proteins in pathogenesis are demonstrated, where lack of either the C or the W protein independently decreased the severity of clinical respiratory disease but did not decrease lethality.
Journal ArticleDOI

Transcriptional response of avian cells to infection with Newcastle disease virus.

TL;DR: Comparative analyses show that a majority of genes that were transcriptionally regulated during infection with another common respiratory pathogen of poultry, the avian pneumovirus, remained unaltered during NDV infection, suggesting that even phylogenetically related viruses elicit unique or "signature" patterns of host transcriptional profiles during infection of host cells.
Journal ArticleDOI

NS1 Protein Mutation I64T Affects Interferon Responses and Virulence of Circulating H3N2 Human Influenza A Viruses.

TL;DR: Analysis of NS1 protein variability within influenza A (IAV) H3N2 viruses infecting humans during the 2012-2013 season and the effect of the mutations in innate immune responses and virus pathogenesis demonstrates the importance of influenza virus surveillance in identifying new mutations in the NS1 Protein.
Journal ArticleDOI

The NS1 protein of influenza A virus suppresses interferon-regulated activation of antigen-presentation and immune-proteasome pathways.

TL;DR: It is shown that the C-terminally truncated NS1 mutant virus is less efficient at suppressing IFN-regulated gene expression associated with activation of antigen-presentation and immune-proteasome pathways.
References
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Journal ArticleDOI

Efficient selection for high-expression transfectants with a novel eukaryotic vector

TL;DR: The results showed that high concentrations of G418 efficiently yielded L cell and CHO cell transfectants stably producing IL-2 at levels comparable with those previously attained using gene amplification.
Journal ArticleDOI

Nipah Virus: A Recently Emergent Deadly Paramyxovirus

TL;DR: Electron microscopic, serologic, and genetic studies indicate that the Nipah virus belongs to the family Paramyxoviridae and is most closely related to the recently discovered Hendra virus, and it is suggested that these two viruses are representative of a new genus within the familyparamyxviridae.
Journal ArticleDOI

Influenza A Virus Lacking the NS1 Gene Replicates in Interferon-Deficient Systems

TL;DR: In this paper, a viable transfectant influenza A virus (delNS1) which lacks the NS1 gene has been generated through the use of reverse genetics, and it has been shown that the NS 1 protein plays a crucial role in inhibiting interferon-mediated antiviral responses of the host.
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