Literature detail

Differential Impact of Specific Amino Acid Residues on the Characteristics of Avian Influenza Viruses in Mammalian Systems.

Dayly Mashaal¹ Sara H Mahmoud² Christin Müller³ Noura M Abo Shama² Amal Abo Kamer¹ Ahmed A Abdelaziz¹ Mohamed A Ali² Stephan Pleschka^3,4 Ahmed Mostafa²

Affiliations 4 institutions

Pharmaceutical Microbiology Department, Faculty of Pharmacy, Tanta University, Tanta 31527, Egypt.
Center of Scientific Excellence for Influenza Viruses, National Research Centre, Giza 12622, Egypt.
Institute of Medical Virology, Justus Liebig University Giessen, Schubertstrasse 81, 35392 Giessen, Germany.
German Center for Infection Research (DZIF), Partner Site Giessen-Marburg-Langen, 35392 Giessen, Germany.

PMID 36422635 2022 Pathogens eng epublish

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Article

Publication summary

Avian influenza virus (AIV) H9N2 was declared to be endemic in birds of the Middle East, in particular in Egypt, with multiple cases of human infections. Despite concerns about the pandemic threat posed by H9N2 AIV, due to the fact that its receptor specificity is similar to that of human influenza viruses, its morbidity and mortality rates in humans are so far negligible. However, the acquisition of specific adaptive amino acid (aa) mutations in the viral polymerase can enhance cross-species transmission of the virus itself or of reassortants, which gained these changes. The polymerase basic protein 2 (PB2) is one of the key determinants for AIV adaptation towards mammals. Although mammalian pathogenicity-related mutations (MPMs) in PB2 genes were identified in different AIVs, the specific effect of single or multiple mutations on viral fitness has not been compared so far. Here, we studied the effect of the aa K at position 591, which was frequently reported in the PB2 of Egyptian H9N2 isolates, on the proliferation efficiency and polymerase activity of an H5N1 (clade 2.2.1.2) AIV already carrying the mammalian adaptive mutation 627K. Using reverse genetics, we generated a set of recombinant parental strains and H5N1 variants carrying the avian-like 591Q/627E or mammalian-like adaptive mutations 591K/627K (H5N1EGY, H9N2EGY, H5N1PB2-H9N2EGY, H5N1H9N2_PB2_K591Q, H5N1PB2_K627E, H5N1PB2_K627E/591K, H5N1PB2_627K/591K). Regardless of the avian-like 627E or the mammalian-adaptive 627K, both variants carrying the 591K (H5N1PB2_K627E/591K, H5N1PB2_627K/591K) and the reassortant H5N1PB2-H9N2EGY replicated to significantly higher levels in mammalian continuous MDCK and Calu-3 cell lines and primary normal human bronchial epithelial cells than the parental H5N1EGY virus (carrying solely the 627K adaptive mutation). Expectedly, the H5N1 variants carrying avian-like PB2 mutations (H5N1H9N2_PB2_K591Q, H5N1PB2_K627E) replicated to significantly lower levels than the parental H5N1EGY virus in the predefined primary and continuous mammalian cell line systems. Consistently, the activity of H5N1 subtype AIV polymerase complexes comprising PB2 segments with singular 591K or combined with 627K was significantly enhanced when compared to parental H5N1EGY and H9N2EGY. This study emphasizes the significant impact of 591K containing PB2 segments in the background of H5N1 polymerase on viral fitness in addition to the well-known MPM 627K in vitro.

591K 627K H5N1 H9N2 mammalian-adaptive marker

Structured evidence records

Evidence records

6 total

Genomic Evolution 2 records

Genomic Evolution Extraction confidence 0.70

Key finding

PB2 substitutions 591K and 627K in H5N1 and H9N2 avian influenza viruses enhanced polymerase activity and replication efficiency in mammalian cells compared with avian-like variants, indicating genomic adaptation toward mammalian hosts.

Virus

Host

Location

Supporting text

We studied the effect of the aa K at position 591, which was frequently reported in the PB2 of Egyptian H9N2 isolates, on the proliferation efficiency and polymerase activity of an H5N1 (clade 2.2.1.2) AIV already carrying the mammalian adaptive mutation 627K. Using reverse genetics, we generated recombinant H5N1 variants carrying combinations of PB2 mutations (591K, 627K, 627E, 591Q) and compared their replication levels and polymerase activity in mammalian cells.

Genes or proteins: PB2
Analysis methods: reverse genetics; comparative mutation analysis

Genomic Evolution Extraction confidence 0.70

Key finding

The PB2 segment from Egyptian H9N2 carrying residue 591K increases polymerase activity and replication fitness in mammalian cells, contributing to genomic adaptation potential when reassorted into H5N1.

Virus

Host

Location

Supporting text

The aa K at position 591 was frequently reported in the PB2 of Egyptian H9N2 isolates and was tested by introducing this PB2 segment into H5N1 backgrounds, showing enhanced replication and polymerase activity in mammalian continuous and primary cell lines compared to parental viruses.

Genes or proteins: PB2
Analysis methods: reverse genetics; comparative mutation analysis

Molecular Adaptation 2 records

Molecular Adaptation Extraction confidence 1.00

Key finding

PB2 mutations 591K and 627K enhance polymerase activity and replication efficiency of H5N1 avian influenza virus in mammalian cells, demonstrating molecular adaptation toward mammalian hosts.

Virus

Host

Location

Supporting text

The activity of H5N1 subtype AIV polymerase complexes comprising PB2 segments with singular 591K or combined with 627K was significantly enhanced when compared to parental H5N1EGY and H9N2EGY, and H5N1 variants carrying the 591K replicated to significantly higher levels in mammalian MDCK, Calu-3, and primary human bronchial epithelial cells.

Genes or proteins: PB2
Mutations: PB2 K591; PB2 K627
Mechanism types: polymerase_activity; replication_efficiency

Molecular Adaptation Extraction confidence 1.00

Key finding

The PB2 K591 mutation identified in H9N2 enhances replication and polymerase activity of H5N1 avian influenza virus in mammalian cells, indicating an adaptive molecular change facilitating cross-species adaptation.

Virus

Host

Location

Supporting text

We studied the effect of the aa K at position 591, which was frequently reported in the PB2 of Egyptian H9N2 isolates, on the proliferation efficiency and polymerase activity of an H5N1 AIV already carrying the mammalian adaptive mutation 627K; the 591K mutation increased viral replication and polymerase activity in mammalian systems.

Genes or proteins: PB2
Mutations: PB2 K591
Mechanism types: polymerase_activity; replication_efficiency

Host Range Experiment 1 records

Host Range Experiment Extraction confidence 0.95

Key finding

H5N1 variants containing PB2 591K showed enhanced replication efficiency in mammalian continuous MDCK and Calu-3 cell lines and primary human bronchial epithelial cells compared to parental H5N1.

Virus

Host

Location

Supporting text

Both variants carrying the 591K (H5N1PB2_K627E/591K, H5N1PB2_627K/591K) and the reassortant H5N1PB2-H9N2EGY replicated to significantly higher levels in mammalian continuous MDCK and Calu-3 cell lines and primary normal human bronchial epithelial cells than the parental H5N1EGY virus.

Method: reverse genetics; replication assay
Sample type: cell lines; primary human bronchial epithelial cells
Experimental system: in vitro cell culture

Recombination Or Reassortment 1 records

Recombination Or Reassortment Extraction confidence 0.90

Key finding

The reassortant H5N1_PB2-H9N2EGY containing the PB2 segment from Egyptian H9N2 showed increased replication efficiency in mammalian cells compared with the parental H5N1_EGY strain, indicating reassortment can enhance mammalian adaptation.

Virus

Host

Location

Supporting text

Both variants carrying the 591K (H5N1_PB2_K627E/591K, H5N1_PB2_627K/591K) and the reassortant H5N1_PB2-H9N2EGY replicated to significantly higher levels in mammalian continuous MDCK and Calu-3 cell lines and primary normal human bronchial epithelial cells than the parental H5N1_EGY virus (carrying solely the 627K adaptive mutation).

Event type: reassortment
Genes or segments: PB2

Citation context

References

30 references

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Evidence overview

Evidence 6

Types 4

Virus 2

Host 3

Evidence types

Genomic Evolution 2 Molecular Adaptation 2 Host Range Experiment 1 Recombination Or Reassortment 1

Linked entities

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Locations

Publication metadata

Journal: Pathogens (Basel, Switzerland)
Volume / Issue / Pages: 11 / 11 / -
ISSN: 2076-0817
Journal country: Switzerland
DOI: 10.3390/pathogens11111385