Literature DB >> 28053101

Generation of a Genetically Stable High-Fidelity Influenza Vaccine Strain.

Tadasuke Naito1, Kotaro Mori2,3,4, Hiroshi Ushirogawa5, Naoki Takizawa2, Eri Nobusawa6, Takato Odagiri6, Masato Tashiro6, Ryosuke L Ohniwa3,7, Kyosuke Nagata8, Mineki Saito5.   

Abstract

Vaccination is considered the most effective preventive means for influenza control. The development of a master virus with high growth and genetic stability, which may be used for the preparation of vaccine viruses by gene reassortment, is crucial for the enhancement of vaccine performance and efficiency of production. Here, we describe the generation of a high-fidelity and high-growth influenza vaccine master virus strain with a single V43I amino acid change in the PB1 polymerase of the high-growth A/Puerto Rico/8/1934 (PR8) master virus. The PB1-V43I mutation was introduced to increase replication fidelity in order to design an H1N1 vaccine strain with a low error rate. The PR8-PB1-V43I virus exhibited good replication compared with that of the parent PR8 virus. In order to compare the efficiency of egg adaptation and the occurrence of gene mutations leading to antigenic alterations, we constructed 6:2 genetic reassortant viruses between the A(H1N1)pdm09 and the PR8-PB1-V43I viruses; hemagglutinin (HA) and neuraminidase (NA) were from the A(H1N1)pdm09 virus, and the other genes were from the PR8 virus. Mutations responsible for egg adaptation mutations occurred in the HA of the PB1-V43I reassortant virus during serial egg passages; however, in contrast, antigenic mutations were introduced into the HA gene of the 6:2 reassortant virus possessing the wild-type PB1. This study shows that the mutant PR8 virus possessing the PB1 polymerase with the V43I substitution may be utilized as a master virus for the generation of high-growth vaccine viruses with high polymerase fidelity, low error rates of gene replication, and reduced antigenic diversity during virus propagation in eggs for vaccine production.IMPORTANCE Vaccination represents the most effective prophylactic option against influenza. The threat of emergence of influenza pandemics necessitates the ability to generate vaccine viruses rapidly. However, as the influenza virus exhibits a high mutation rate, vaccines must be updated to ensure a good match of the HA and NA antigens between the vaccine and the circulating strain. Here, we generated a genetically stable master virus of the A/Puerto Rico/8/1934 (H1N1) backbone encoding an engineered high-fidelity viral polymerase. Importantly, following the application of the high-fidelity PR8 backbone, no mutation resulting in antigenic change was introduced into the HA gene during propagation of the A(H1N1)pdm09 candidate vaccine virus. The low error rate of the present vaccine virus should decrease the risk of generating mutant viruses with increased virulence. Therefore, our findings are expected to be useful for the development of prepandemic vaccines and live attenuated vaccines with higher safety than that of the present candidate vaccines.
Copyright © 2017 American Society for Microbiology.

Entities:  

Keywords:  RNA polymerases; fidelity; influenza; influenza vaccines; reverse genetic analysis

Mesh:

Substances:

Year:  2017        PMID: 28053101      PMCID: PMC5331824          DOI: 10.1128/JVI.01073-16

Source DB:  PubMed          Journal:  J Virol        ISSN: 0022-538X            Impact factor:   5.103


  55 in total

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4.  A Polymerase mechanism-based strategy for viral attenuation and vaccine development.

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5.  A reassortment-incompetent live attenuated influenza virus vaccine for protection against pandemic virus strains.

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7.  Replication and plaque assay of influenza virus in an established line of canine kidney cells.

Authors:  C R Gaush; T F Smith
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8.  The N-terminal region of influenza virus polymerase PB1 adjacent to the PA binding site is involved in replication but not transcription of the viral genome.

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10.  Nucleic acid polymerases use a general acid for nucleotidyl transfer.

Authors:  Christian Castro; Eric D Smidansky; Jamie J Arnold; Kenneth R Maksimchuk; Ibrahim Moustafa; Akira Uchida; Matthias Götte; William Konigsberg; Craig E Cameron
Journal:  Nat Struct Mol Biol       Date:  2009-01-18       Impact factor: 15.369

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1.  Rational Control of Poliovirus RNA-Dependent RNA Polymerase Fidelity by Modulating Motif-D Loop Conformational Dynamics.

Authors:  Jingjing Shi; Jacob M Perryman; Xiaorong Yang; Xinran Liu; Derek M Musser; Alyson K Boehr; Ibrahim M Moustafa; Jamie J Arnold; Craig E Cameron; David D Boehr
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2.  Tyr82 Amino Acid Mutation in PB1 Polymerase Induces an Influenza Virus Mutator Phenotype.

Authors:  Tadasuke Naito; Kazumasa Shirai; Kotaro Mori; Hidetaka Muratsu; Hiroshi Ushirogawa; Ryosuke L Ohniwa; Kousuke Hanada; Mineki Saito
Journal:  J Virol       Date:  2019-10-29       Impact factor: 5.103

3.  Enterovirus A71 Containing Codon-Deoptimized VP1 and High-Fidelity Polymerase as Next-Generation Vaccine Candidate.

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Review 4.  Recent Progress in Recombinant Influenza Vaccine Development Toward Heterosubtypic Immune Response.

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5.  Epistatic Interactions within the Influenza A Virus Polymerase Complex Mediate Mutagen Resistance and Replication Fidelity.

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Journal:  mSphere       Date:  2017-08-16       Impact factor: 4.389

6.  Influenza Virus Polymerase Mutation Stabilizes a Foreign Gene Inserted into the Virus Genome by Enhancing the Transcription/Replication Efficiency of the Modified Segment.

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Review 7.  The influenza virus RNA polymerase as an innate immune agonist and antagonist.

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8.  Polymerase Fidelity Contributes to Foot-and-Mouth Disease Virus Pathogenicity and Transmissibility In Vivo.

Authors:  Chen Li; Jiabao Shi; Haiwei Wang; Efraín E Rivera-Serrano; Decheng Yang; Guohui Zhou; Chao Sun; Craig E Cameron; Li Yu
Journal:  J Virol       Date:  2020-12-09       Impact factor: 5.103

  8 in total

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