2005
DOI: 10.1128/jvi.79.12.7535-7543.2005
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Mutations in the NS1 Protein of Swine Influenza Virus Impair Anti-Interferon Activity and Confer Attenuation in Pigs

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Cited by 222 publications
(272 citation statements)
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“…In pigs vaccinated with the attenuated NS1 126 TX98 mutant, the mean viral titers did not exceed 10 TCID 50 /ml on days 2 or 4, and no virus was detected on day 6. This disparity in wild type TX98 and NS1 126 TX98 replication in vivo is consistent with the attenuated phenotype in previously reported results [17].…”
Section: Vaccine Virus Replication In Naïve Pigssupporting
confidence: 92%
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“…In pigs vaccinated with the attenuated NS1 126 TX98 mutant, the mean viral titers did not exceed 10 TCID 50 /ml on days 2 or 4, and no virus was detected on day 6. This disparity in wild type TX98 and NS1 126 TX98 replication in vivo is consistent with the attenuated phenotype in previously reported results [17].…”
Section: Vaccine Virus Replication In Naïve Pigssupporting
confidence: 92%
“…However, given the very low level of NS1 126 TX98 virus detected in pigs' nasal swabs after intranasal inoculation, it is also possible that the vaccine did not supply enough endogenous antigen to prime a large population of CD4 -CD8 + T cells. Viruses engineered with even shorter NS1 proteins than that of NS1 126 TX98 are paradoxically less attenuated, in both pigs and mice [17,30]. It is reasonable to predict that mutants such as those would elicit greater CD4 -CD8 + T cell responses.…”
Section: Discussionmentioning
confidence: 99%
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“…Interferon inhibition assays were performed according to the general methodology established by Rehwinkel et al to trigger IFN production using an active influenza virus RNA-dependent RNA polymerase (vRdRp) (44) and a bioassay established by Solorzano et al (45), using the VSV-GFP developed by Stojdl et al (46). Briefly, HEK293FT cells were transfected with various combinations of plasmids, including those needed to produce a functional vRdRp [here referred to as PolII(PB2ϩPB1ϩPAϩNP)] and a construct transcribing the PB2 gene segment under an RNA polymerase I promoter in the reverse complementary direction [here referred to as PolI(PB2)].…”
Section: Methodsmentioning
confidence: 99%