The cellular localization of avian influenza virus PB1-F2 protein alters the magnitude of IFN2 promoter and NFκB-dependent promoter antagonism in chicken cells

被引:9
作者
James, Joe [1 ,2 ]
Smith, Nikki [3 ]
Ross, Craig [4 ]
Iqbal, Munir [1 ]
Goodbourn, Steve [4 ]
Digard, Paul [3 ]
Barclay, Wendy S. [2 ]
Shelton, Holly [1 ]
机构
[1] Pirbright Inst, Woking, Surrey, England
[2] Imperial Coll London, London, England
[3] Roslin Inst, Edinburgh, Midlothian, Scotland
[4] St Georges Univ London, London, England
基金
英国生物技术与生命科学研究理事会;
关键词
influenza virus; PB1-F2; IKK beta; MAVS; chicken; A VIRUS; ELECTROCHEMICAL DETECTION; MITOCHONDRIAL-MEMBRANE; INTERFERON; INFECTION; OUTBREAKS; SEQUENCE; IMPACTS;
D O I
10.1099/jgv.0.001220
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
The accessory protein, PB1-F2, of influenza A virus (IAV) functions in a chicken host to prolong infectious virus shedding and thus the transmission window. Here we show that this delay in virus clearance by PB1-F2 in chickens is accompanied by reduced transcript levels of type 1 interferon (IFN)-induced genes and NF kappa B-activated pro-inflammation cytokines. In vitro, two avian influenza isolate-derived PB1-F2 proteins, H9N2 UDL01 and H5N1 5092, exhibited the same antagonism of the IFN and pro-inflammation induction pathways seen in vivo, but to different extents. The two PB1-F2 proteins had different cellular localization in chicken cells, with H5N1 5092 being predominantly mitochondrial-associated and H9N2 UDL being cytoplasmic but not mitochondrial-localized. We hypothesized that PB1-F2 localization might influence the functionality of the protein during infection and that the protein sequence could alter cellular localization. We demonstrated that the sequence of the C-terminus of PB1-F2 determined cytoplasmic localization in chicken cells and this was linked with protein instability. Mitochondrial localization of PB1-F2 resulted in reduced antagonism of an NF kappa B-dependent promoter. In parallel, mitochondrial localization of PB1-F2 increased the potency of chicken IFN 2 induction antagonism. We suggest that mitochondrial localization of PB1-F2 restricts interaction with cytoplasmic-located IKK beta, reducing NF kappa B-responsive promoter antagonism, but enhances antagonism of the IFN2 promoter through interaction with the mitochondrial adaptor MAVS. Our study highlights the differential mechanisms by which IAV PB1-F2 protein can dampen the avian host innate signalling response.
引用
收藏
页码:414 / 430
页数:17
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