Chimeric O1K foot-and-mouth disease virus with SAT2 outer capsid as an FMD vaccine candidate

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作者
Abhay Kotecha
Eva Perez-Martin
Yongjie Harvey
Fuquan Zhang
Serban L Ilca
Elizabeth E. Fry
Ben Jackson
Francois Maree
Katherine Scott
Corey W. Hecksel
Michiel M. Harmsen
Valérie Mioulet
Britta Wood
Nick Juleff
David I. Stuart
Bryan Charleston
Julian Seago
机构
[1] The Pirbright Institute,Transboundary Animal Disease Programme
[2] Woking,Wageningen Bioveterinary Research
[3] ARC-Onderstepoort Veterinary Institute,Diamond Light Source
[4] Private Bag X05,undefined
[5] Division of Structural Biology,undefined
[6] Wellcome Trust Centre for Human Genetics,undefined
[7] University of Oxford,undefined
[8] Division Virology,undefined
[9] P.O. Box 65,undefined
[10] Harwell Science and Innovation Campus,undefined
来源
Scientific Reports | / 8卷
关键词
Foot-and-mouth Disease Virus (FMDV); SAT2 Virus; Southern African Territories (SAT); Chimeric Virus; FMDV Capsid;
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摘要
Foot-and-mouth disease virus (FMDV) is highly contagious and infects cloven-hoofed domestic livestock leading to foot-and-mouth disease (FMD). FMD outbreaks have severe economic impact due to production losses and associated control measures. FMDV is found as seven distinct serotypes, but there are numerous subtypes within each serotype, and effective vaccines must match the subtypes circulating in the field. In addition, the O and Southern African Territories (SAT) serotypes, are relatively more thermolabile and their viral capsids readily dissociate into non-immunogenic pentameric subunits, which can compromise the effectiveness of FMD vaccines. Here we report the construction of a chimeric clone between the SAT2 and O serotypes, designed to have SAT2 antigenicity. Characterisation of the chimeric virus showed growth kinetics equal to that of the wild type SAT2 virus with better thermostability, attributable to changes in the VP4 structural protein. Sequence and structural analyses confirmed that no changes from SAT2 were present elsewhere in the capsid as a consequence of the VP4 changes. Following exposure to an elevated temperature the thermostable SAT2-O1K chimera induced higher neutralizing-antibody titres in comparison to wild type SAT2 virus.
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