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A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs

Both the replication and transcription of the influenza virus are catalyzed by the viral polymerase complex. The polymerases of most avian influenza A viruses have poor performance in mammalian cells, which is considered to be one of the important species barriers. Pigs have been long considered as...

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Autores principales: Zhang, Haili, Li, Hongxin, Wang, Wenqiang, Wang, Yujie, Han, Guan-Zhu, Chen, Hualan, Wang, Xiaojun
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2020
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7055917/
https://www.ncbi.nlm.nih.gov/pubmed/32084248
http://dx.doi.org/10.1371/journal.ppat.1008330
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author Zhang, Haili
Li, Hongxin
Wang, Wenqiang
Wang, Yujie
Han, Guan-Zhu
Chen, Hualan
Wang, Xiaojun
author_facet Zhang, Haili
Li, Hongxin
Wang, Wenqiang
Wang, Yujie
Han, Guan-Zhu
Chen, Hualan
Wang, Xiaojun
author_sort Zhang, Haili
collection PubMed
description Both the replication and transcription of the influenza virus are catalyzed by the viral polymerase complex. The polymerases of most avian influenza A viruses have poor performance in mammalian cells, which is considered to be one of the important species barriers. Pigs have been long considered as important intermediate hosts for interspecies transmission of the avian influenza virus, because of their susceptibility to infection with both avian and mammalian influenza viruses. However, the molecular basis of influenza polymerase adaptation in pigs remains largely unknown. ANP32A and ANP32B proteins have been identified as playing fundamental roles in influenza virus replication and host range determination. In this study, we found that swine ANP32A (swANP32A), unlike swine ANP32B or other mammalian ANP32A or B, shows stronger supporting activity to avian viral polymerase. Knockout of ANP32A in pig cells PK15 dramatically reduced avian influenza polymerase activity and viral infectivity, suggesting a unique feature of swANP32A in supporting avian influenza viral polymerase. This species-specific activity is mapped to two key sites, 106V and 156S, in swANP32A. Interestingly, the amino acid 106V is unique to pigs among all the vertebrate species studied, and when combined with 156S, exhibits positive epistasis in pigs. Mutation of 106V and 156S to the signature found in ANP32As from other mammalian species weakened the interaction between swANP32A and chicken viral polymerase, and reduced polymerase activity. Understanding the molecular basis of ANP32 proteins may help to discover new antiviral targets and design avian influenza resistant genome edited pigs.
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spelling pubmed-70559172020-03-13 A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs Zhang, Haili Li, Hongxin Wang, Wenqiang Wang, Yujie Han, Guan-Zhu Chen, Hualan Wang, Xiaojun PLoS Pathog Research Article Both the replication and transcription of the influenza virus are catalyzed by the viral polymerase complex. The polymerases of most avian influenza A viruses have poor performance in mammalian cells, which is considered to be one of the important species barriers. Pigs have been long considered as important intermediate hosts for interspecies transmission of the avian influenza virus, because of their susceptibility to infection with both avian and mammalian influenza viruses. However, the molecular basis of influenza polymerase adaptation in pigs remains largely unknown. ANP32A and ANP32B proteins have been identified as playing fundamental roles in influenza virus replication and host range determination. In this study, we found that swine ANP32A (swANP32A), unlike swine ANP32B or other mammalian ANP32A or B, shows stronger supporting activity to avian viral polymerase. Knockout of ANP32A in pig cells PK15 dramatically reduced avian influenza polymerase activity and viral infectivity, suggesting a unique feature of swANP32A in supporting avian influenza viral polymerase. This species-specific activity is mapped to two key sites, 106V and 156S, in swANP32A. Interestingly, the amino acid 106V is unique to pigs among all the vertebrate species studied, and when combined with 156S, exhibits positive epistasis in pigs. Mutation of 106V and 156S to the signature found in ANP32As from other mammalian species weakened the interaction between swANP32A and chicken viral polymerase, and reduced polymerase activity. Understanding the molecular basis of ANP32 proteins may help to discover new antiviral targets and design avian influenza resistant genome edited pigs. Public Library of Science 2020-02-21 /pmc/articles/PMC7055917/ /pubmed/32084248 http://dx.doi.org/10.1371/journal.ppat.1008330 Text en © 2020 Zhang et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Zhang, Haili
Li, Hongxin
Wang, Wenqiang
Wang, Yujie
Han, Guan-Zhu
Chen, Hualan
Wang, Xiaojun
A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs
title A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs
title_full A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs
title_fullStr A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs
title_full_unstemmed A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs
title_short A unique feature of swine ANP32A provides susceptibility to avian influenza virus infection in pigs
title_sort unique feature of swine anp32a provides susceptibility to avian influenza virus infection in pigs
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7055917/
https://www.ncbi.nlm.nih.gov/pubmed/32084248
http://dx.doi.org/10.1371/journal.ppat.1008330
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