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来自猪繁殖与呼吸综合征病毒克隆全长cDNA的感染性转录本。

Infectious transcripts from cloned genome-length cDNA of porcine reproductive and respiratory syndrome virus.

作者信息

Meulenberg J J, Bos-de Ruijter J N, van de Graaf R, Wensvoort G, Moormann R J

机构信息

Institute for Animal Science and Health, Lelystad, The Netherlands.

出版信息

J Virol. 1998 Jan;72(1):380-7. doi: 10.1128/JVI.72.1.380-387.1998.

DOI:10.1128/JVI.72.1.380-387.1998
PMID:9420236
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC109385/
Abstract

The 5'-terminal end of the genomic RNA of the Lelystad virus isolate (LV) of porcine reproductive and respiratory syndrome virus was determined. To construct full-length cDNA clones, the 5'-terminal sequence was ligated to cDNA clones covering the complete genome of LV. When RNA that was transcribed in vitro from these full-length cDNA clones was transfected into BHK-21 cells, infectious LV was produced and secreted. The virus was rescued by passage to porcine alveolar lung macrophages or CL2621 cells. When infectious transcripts were transfected to porcine alveolar lung macrophages or CL2621 cells, no infectious virus was produced due to the poor transfection efficiency of these cells. The growth properties of the viruses produced by BHK-21 cells transfected with infectious transcripts of LV cDNA resembled the growth properties of the parental virus from which the cDNA was derived. Two nucleotide changes leading to a unique PacI restriction site directly downstream of the ORF7 gene were introduced in the genome-length cDNA clone. The virus recovered from this mutated cDNA clone retained the PacI site, which confirmed the de novo generation of infectious LV from cloned cDNA. These results indicate that the infectious clone of LV enables us to mutagenize the viral genome at specific sites and that it will therefore be useful for detailed molecular characterization of the virus, as well as for the development of a safe and effective live vaccine for use in pigs.

摘要

确定了猪繁殖与呼吸综合征病毒莱利斯塔德病毒分离株(LV)基因组RNA的5'末端。为构建全长cDNA克隆,将5'末端序列连接到覆盖LV完整基因组的cDNA克隆上。当将从这些全长cDNA克隆体外转录的RNA转染到BHK-21细胞中时,产生并分泌了有感染性的LV。通过传代至猪肺泡巨噬细胞或CL2621细胞来拯救该病毒。当将感染性转录本转染到猪肺泡巨噬细胞或CL2621细胞中时,由于这些细胞的转染效率低而未产生有感染性的病毒。用LV cDNA感染性转录本转染的BHK-21细胞产生的病毒的生长特性类似于衍生出cDNA的亲本病毒的生长特性。在基因组长度的cDNA克隆中引入了两个导致在ORF7基因直接下游出现独特PacI限制性位点的核苷酸变化。从该突变cDNA克隆中回收的病毒保留了PacI位点,这证实了从克隆的cDNA从头产生有感染性的LV。这些结果表明,LV的感染性克隆使我们能够在特定位点诱变病毒基因组,因此它将有助于对该病毒进行详细的分子特征分析,以及开发用于猪的安全有效的活疫苗。

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