Influenza A virus PB1-F2 protein prolongs viral shedding in chickens lengthening the transmission window

James, Joe; Howard, Wendy A.; Iqbal, Munir; Nair, Venugopal; Barclay, William; Shelton, Holly

doi:10.1099/jgv.0.000584

Cited by 45 publications

(54 citation statements)

References 39 publications

(57 reference statements)

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“…This sample also contained the PB1-F2 S66 marker, which has been associated with increased pathogenicity in mammals (Conenello et al, 2011). All sequenced PB1 segments showed either the 87 or 90 amino acid-long PB1-F2 protein sequence, which is common in isolates from avian species (James et al, 2016). We also found N and T at position 66; interestingly, PB1-F2 T66 was only found in samples (n = 3 samples) sequenced through swab-NGS.…”

Section: Discussionmentioning

confidence: 74%

Improved detection of influenza A virus from blue‐winged teals by sequencing directly from swab material

Ferreri

Ortiz

Geiger

et al. 2019

Ecology and Evolution

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The greatest diversity of influenza A virus (IAV) is found in wild aquatic birds of the orders Anseriformes and Charadriiformes. In these birds, IAV replication occurs mostly in the intestinal tract. Fecal, cloacal, and/or tracheal swabs are typically collected and tested by real‐time RT‐PCR (rRT‐PCR) and/or by virus isolation in embryonated chicken eggs in order to determine the presence of IAV. Virus isolation may impose bottlenecks that select variant populations that are different from those circulating in nature, and such bottlenecks may result in artifactual representation of subtype diversity and/or underrepresented mixed infections. The advent of next‐generation sequencing (NGS) technologies provides an opportunity to explore to what extent IAV subtype diversity is affected by virus isolation in eggs. In the present work, we evaluated the advantage of sequencing by NGS directly from swab material of IAV rRT‐PCR‐positive swabs collected during the 2013–14 surveillance season in Guatemala and compared to results from NGS after virus isolation. The results highlight the benefit of sequencing IAV genomes directly from swabs to better understand subtype diversity and detection of alternative amino acid motifs that could otherwise escape detection using traditional methods of virus isolation. In addition, NGS sequencing data from swabs revealed reduced presence of defective interfering particles compared to virus isolates. We propose an alternative workflow in which original swab samples positive for IAV by rRT‐PCR are first subjected to NGS before attempting viral isolation. This approach should speed the processing of samples and better capture natural IAV diversity. OPEN RESEARCH BADGES This article has earned an Open Data Badge for making publicly available the digitally‐shareable data necessary to reproduce the reported results. The data is available at https://doi.org/10.5061/dryad.3h2n106.

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Section: Discussionmentioning

confidence: 74%

Improved detection of influenza A virus from blue‐winged teals by sequencing directly from swab material

Ferreri

Ortiz

Geiger

et al. 2019

Ecology and Evolution

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“…Duck farming often involves raising and storing ducks in open bodies of water, which introduces the risk for wild waterfowl to mix with farmed ducks and transmit influenza viruses. In addition, studies have shown longer virus shedding times for LPAI‐infected ducks, up to 11.5 days, compared with LPAI‐infected chickens, up to 6 days (Hénaux & Samuel, ; James et al, ). Therefore, poultry traders with larger numbers of unsold ducks could increase the transmission window for ducks to infect chickens, especially as unsold ducks may have repeated exposures to wild waterfowl when traders store unsold ducks at home.…”

Section: Discussionmentioning

confidence: 99%

Poultry trading behaviours in Vietnamese live bird markets as risk factors for avian influenza infection in chickens

Sealy

Fournié

Trang

et al. 2019

Transbound Emerg Dis

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Vietnamese poultry are host to co‐circulating subtypes of avian influenza viruses, including H5N1 and H9N2, which pose a great risk to poultry productivity and to human health. AIVs circulate throughout the poultry trade network in Vietnam, with live bird markets being an integral component to this network. Traders at LBMs exhibit a variety of trading practices, which may influence the transmission of AIVs. We identified trading practices that impacted on AIV prevalence in chickens marketed in northern Vietnamese LBMs. We generated sequencing data for 31 H9N2 and two H5N6 viruses. Viruses isolated in the same LBM or from chickens sourced from the same province were genetically closer than viruses isolated in different LBMs or from chickens sourced in different provinces. The position of a vendor in the trading network impacted on their odds of having AIV‐infected chickens. Being a retailer and purchasing chickens from middlemen was associated with increased odds of infection, whereas odds decreased if vendors purchased chickens directly from large farms. Odds of infection were also higher for vendors having a greater volume of ducks unsold per day. These results indicate how the spread of AIVs is influenced by the structure of the live poultry trading network.

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“…Contact transmission relies on the transfer of particles to mucous membranes directly, or via a fomite intermediate. tropism [15,[71][72][73][74][75][76]. One of the key molecular markers that facilitates adaptation of an AIV from wild aquatic birds to poultry is the deletion of amino acids from the stalk domain of NA, which have been shown to mediate the switch to respiratory tropism in chickens [77,78].…”

Section: H9n2 Virus Transmission and Host Tropism In Poultrymentioning

confidence: 99%

“…One of the key molecular markers that facilitates adaptation of an AIV from wild aquatic birds to poultry is the deletion of amino acids from the stalk domain of NA, which have been shown to mediate the switch to respiratory tropism in chickens [77,78]. There is good evidence to suggest that many LPAIV strains transmit by the airborne route, the oral-faecal route and the waterborne route [15,75,79]. However, the favoured mechanism of transmission between individuals varies by host species and viral strain.…”

Section: H9n2 Virus Transmission and Host Tropism In Poultrymentioning

confidence: 99%

A Global Perspective on H9N2 Avian Influenza Virus

Peacock¹,

James²,

Sealy³

et al. 2019

Preprint

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H9N2 avian influenza viruses have become globally widespread in poultry over the last two decades and represent a genuine threat both to the global poultry industry but also humans through their high rates of zoonotic infection and pandemic potential. H9N2 viruses are generally hyperendemic in effected countries and have been found in poultry in many new regions in recent years. In this review we examine the current global spread of H9N2 avian influenza viruses as well as their host range, tropism, transmission routes and the risk posed by these viruses to human health.

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Influenza A virus PB1-F2 protein prolongs viral shedding in chickens lengthening the transmission window

Cited by 45 publications

References 39 publications

Improved detection of influenza A virus from blue‐winged teals by sequencing directly from swab material

Improved detection of influenza A virus from blue‐winged teals by sequencing directly from swab material

Poultry trading behaviours in Vietnamese live bird markets as risk factors for avian influenza infection in chickens

A Global Perspective on H9N2 Avian Influenza Virus

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