Please use this identifier to cite or link to this item: http://cmuir.cmu.ac.th/jspui/handle/6653943832/71816
Title: Reverse genetics approach for developing rotavirus vaccine candidates carrying VP4 and VP7 genes cloned from clinical isolates of human rotavirus
Authors: Yuta Kanai
Misa Onishi
Takahiro Kawagishi
Pimfhun Pannacha
Jeffery A. Nurdin
Ryotaro Nouda
Moeko Yamasaki
Tina Lusiany
Pattara Khamrin
Shoko Okitsu
Satoshi Hayakawa
Hirotaka Ebina
Hiroshi Ushijima
Takeshi Kobayashi
Authors: Yuta Kanai
Misa Onishi
Takahiro Kawagishi
Pimfhun Pannacha
Jeffery A. Nurdin
Ryotaro Nouda
Moeko Yamasaki
Tina Lusiany
Pattara Khamrin
Shoko Okitsu
Satoshi Hayakawa
Hirotaka Ebina
Hiroshi Ushijima
Takeshi Kobayashi
Keywords: Agricultural and Biological Sciences;Immunology and Microbiology
Issue Date: 1-Jan-2021
Abstract: Copyright © 2020 American Society for Microbiology. All Rights Reserved. Species A rotaviruses (RVs) are a leading cause of severe acute gastroenteritis in infants and children younger than 5 years. Currently available RV vaccines were adapted from wild-type RV strains by serial passage of cultured cells or by reassortment between human and animal RV strains. These traditional methods require large-scale screening and genotyping to obtain vaccine candidates. Reverse genetics is a tractable, rapid, and reproducible approach to generating recombinant RV vaccine candidates carrying any VP4 and VP7 genes that provide selected antigenicity. Here, we developed a vaccine platform by generating recombinant RVs carrying VP4 (P[4] and P[8]), VP7 (G1, G2, G3, G8, and G9), and/or VP6 genes cloned from human RV clinical samples using the simian RV SA11 strain (G3P[2]) as a backbone. Neutralization assays using monoclonal antibodies and murine antisera revealed that recombinant VP4 and VP7 monoreassortant viruses exhibited altered antigenicity. However, replication of VP4 monoreassortant viruses was severely impaired. Generation of recombinant RVs harboring a chimeric VP4 protein for SA11 and human RV gene components revealed that the VP8* fragment was responsible for efficient infectivity of recombinant RVs. Although this system must be improved because the yield of vaccine viruses directly affects vaccine manufacturing costs, reverse genetics requires less time than traditional methods and enables rapid production of safe and effective vaccine candidates. IMPORTANCE Although vaccines have reduced global RV-associated hospitalization and mortality over the past decade, the multisegmented genome of RVs allows reassortment of VP4 and VP7 genes from different RV species and strains. The evolutionary dynamics of novel RV genotypes and their constellations have led to great genomic and antigenic diversity. The reverse genetics system is a powerful tool for manipulating RV genes, thereby controlling viral antigenicity, growth capacity, and pathogenicity. Here, we generated recombinant simian RVs (strain SA11) carrying heterologous VP4 and VP7 genes cloned from clinical isolates and showed that VP4- or VP7-substituted chimeric viruses can be used for antigenic characterization of RV outer capsid proteins and as improved seed viruses for vaccine production.
URI: https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=85098662886&origin=inward
http://cmuir.cmu.ac.th/jspui/handle/6653943832/71816
ISSN: 10985514
0022538X
Appears in Collections:CMUL: Journal Articles

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