Elsevier

Cytokine

Volume 59, Issue 3, September 2012, Page 506
Cytokine

O020 Influenza a virus protein PB1-F2 activates the NLRP3 inflammasome to induce inflammation

https://doi.org/10.1016/j.cyto.2012.06.051Get rights and content

Introduction

Characteristic of pandemic influenza A virus (IAV) strains is the hyper-inflammatory response associated with infections which can lead to severe clinical symptoms and death. PB1-F2 is a non-structural IAV protein that has gained attention in recent years mainly attributable via its ability to increase pathogenicity by disrupting macrophages. Critical to human health, most avian influenza and human H3N2 viruses carry the information for full-length PB1-F2 protein, whereas human non-pandemic H1N1 IAV strains harbour a truncated version. Importantly, PB1-F2 peptides form protein aggregates and the formation of PB1-F2 amyloid-like fibres are observed in infected cells. There is increasing awareness to the important role of PB1-F2 in enhanced pathogenesis, although the underlying mechanism for its role in inflammation and macrophage dysfunction is not understood.

Methods

We have elucidated the mechanism of PB1-F2 induced inflammation via the NRLP3-inflammasome using a series ofPB1-F2-deficient viral strains and PB1-F2 peptides combined with inflammasome-deficient macrophages.

Results

Mice treated with IAV lacking expression of PB1-F2 display decreased inflammation, neutrophil, macrophage and DC infiltration to the lung. Conversely, mice inoculated with PB1-F2 peptide display increased inflammatory cell infiltration and inflammation. Following on from this, we have found that PB1-F2 peptide induces maturation of IL-1β in human PBMCs, which is reduced by inhibition of phagocytosis and Caspase-1. PB1-F2 also induced IL-1b secretion in murine macrophages that is phagocytosis-dependent. Importantly, cells deficient in caspase-1, ASC and NLRP3 display ablated IL-1β maturation upon challenge with PB1-F2 indicating PB1-F2 induces inflammation via a NLRP3 inflammasome. These findings suggest a critical role for PB1-F2 in inducing the hyperinflammatory state characterised in pandemic IAV infections and its possible role in macrophage dysfunction via inflammasome-mediated pyroptosis.

Conclusion

Our findings identify a previously unknown role for PB1-F2-induced inflammation, via recognition by the NLRP3-inflammasome, leading to maturation of IL-1b. Activation of the inflammasome may also explain the observation of PB1-F2-mediated macrophage dysregulation, possibly via inflammasome-mediated pyroptosis. Elucidating mechanisms of the molecular basis for disease severity of emerging influenza viruses, especially those implicated in global outbreaks is essential to develop better treatment regimes to improve the clinical outcomes for patients with severe acute infections.

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