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Turnover rate of NS3 proteins modulates bluetongue virus replication kinetics in a host-specific manner

J Virol. 2015-10; 
Ftaich N, Ciancia C, Viarouge C, Barry G, Ratinier M, van Rijn PA, Breard E, Vitour D, Zientara S, Palmarini M, Terzian C, Arnaud F
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Bacterial Expression System BTV-16RSA (GenBank accession number FJ713328), here referred to as Seg-10/-2 and Seg-10/-16, respectively, were synthesized and cloned into the pUC57 plasmid by GenScript. Seg-10/-2 and Seg-10/-16, encoding the same NS3 amino acid proteins as Seg-10/-1 and being referred to as Seg-10/-2AA and Seg-10/-16AA, respectively, also were synthesized by GenScript.,,Thus, to assess the effect of these NS3 amino acid variations, Seg-10/-2 and Seg-10/-16, encoding NS3 proteins with strictly identical amino acid residues of Seg-10/-1 (named Seg-10/-2AA and Seg-10/-16AA, respectively), were synthesized by GenScript, and the corresponding viruses, rBTV/-2AA and rBTV/-16AA, were produced by reverse genetics. Get A Quote

摘要

Bluetongue virus (BTV) is an arbovirus transmitted to livestock by midges of the Culicoides family and is the etiological agent of a hemorrhagic disease in sheep and other ruminants. In mammalian cells, BTV particles are released primarily by virus-induced cell lysis, while in insect cells they bud from the plasma membrane and establish a persistent infection. BTV possesses a ten-segmented double-stranded RNA genome, and NS3 proteins are encoded by segment 10 (Seg-10). The viral nonstructural protein 3 (NS3) plays a key role in mediating BTV egress as well as in impeding the in vitro synthesis of type I interferon in mammalian cells. In this study, we asked whether genetically distant NS3 proteins can alter BTV... More

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