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Reverse genetic manipulation of the overlapping coding regions for structural proteins of the type II porcine reproductive and respiratory syndrome virus.

机译:II型猪繁殖与呼吸综合征病毒结构蛋白的重叠编码区的逆向遗传操作。

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The overlapping genomic regions coding for structural proteins of porcine reproductive and respiratory syndrome virus (PRRSV) poses problems for molecular dissection of the virus replication process. We constructed five mutant full-length cDNA clones with the overlapping regions unwound and 1 to 3 restriction sites inserted between two adjacent ORFs (ORF1/2, ORF4/5, ORF5/6, ORF 6/7 and ORF7/3' UTR), which generated the recombinant viruses. Our findings demonstrated that 1) the overlapping structural protein ORFs can be physically separated, and is dispensable for virus viability; 2) such ORF separations did not interrupt the subgenomic RNA synthesis; 3) the plaque morphology, growth kinetics, and antigenicity of these mutant viruses were virtually indistinguishable from those of the parental virus in cultured cells; and 4) these mutant viruses remained genetic stable in vitro. This study lays a foundation for further molecular dissection of PRRSV replication process, and development of genetically tagged vaccines against PRRS.
机译:编码猪繁殖与呼吸综合征病毒(PRRSV)的结构蛋白的重叠基因组区域为病毒复制过程的分子解剖提出了问题。我们构建了五个突变的全长cDNA克隆,其中未重叠的重叠区域和在两个相邻ORF(ORF1 / 2,ORF4 / 5,ORF5 / 6,ORF 6/7和ORF7 / 3'UTR)之间插入了1-3个限制性位点,产生重组病毒。我们的发现表明:1)重叠的结构蛋白ORF可以物理分离,并且对于病毒的生存力是必不可少的; 2)此类ORF分离不会中断亚基因组RNA的合成; 3)在培养细胞中,这些突变病毒的噬菌斑形态,生长动力学和抗原性实际上与亲代病毒没有区别。 4)这些突变病毒在体外仍保持遗传稳定。这项研究为进一步PRRSV复制过程的分子解剖,以及开发针对PRRS的基因标记疫苗奠定了基础。

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