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猪繁殖与呼吸综合征病毒基因组RNA 3'末端的分子克隆与核苷酸测序

Molecular cloning and nucleotide sequencing of the 3'-terminal genomic RNA of the porcine reproductive and respiratory syndrome virus.

作者信息

Meng X J, Paul P S, Halbur P G

机构信息

Veterinary Medical Research Institute, College of Veterinary Medicine, Iowa State University, Ames 50011.

出版信息

J Gen Virol. 1994 Jul;75 ( Pt 7):1795-801. doi: 10.1099/0022-1317-75-7-1795.

DOI:10.1099/0022-1317-75-7-1795
PMID:8021610
Abstract

The genomic RNA of a porcine reproductive and respiratory syndrome virus (PRRSV) isolate from the U.S.A., VR 2385 (ATCC), was copied into cDNA after priming with oligo(dT) and cloned into phage lambda. The cDNA clones representing the 3'-terminal genomic RNA of the virus were isolated and sequenced. The genome is a positive-stranded, polyadenylated RNA with an estimated size of 15 kb. Analysis of the resulting sequence identified three complete open reading frames (ORFs) with the potential to encode polypeptides with predicted M(r)s of 22.2K (ORF 5), 19.1K (ORF 6) and 13.6K (ORF 7). ORF 7, which is closest to the 3' end, is predicted to encode a highly basic nucleocapsid protein displaying 58% amino acid identity to the corresponding protein of the Lelystad virus (LV), a European PRRSV isolate. ORFs 6 and 5, preceding ORF 7, are each predicted to encode proteins containing several hydrophobic domains that are thought to be membrane-associated. The VR 2385 ORF 6 protein is the most conserved structural protein. It has 78% amino acid identity to the equivalent LV protein, and ORF 5 shares only 54% of its amino acid sequence. Northern blot analysis revealed a 3'-coterminal nested set of six subgenomic RNAs in VR 2385 virus-infected CRL 11171 cells. Our results indicate that VR 2385, like LV, is a member of the newly proposed arterivirus group. However, the striking genetic variation and the difference in pathogenicity between LV and VR 2385 suggest that the viruses causing PRRS in the U.S.A. and Europe are highly variable and they may represent different genotypes.

摘要

一株来自美国的猪繁殖与呼吸综合征病毒(PRRSV)分离株VR 2385(ATCC)的基因组RNA,在用寡聚(dT)引发后被转录成cDNA,并克隆到噬菌体λ中。分离并测序了代表该病毒3'端基因组RNA的cDNA克隆。该基因组是一种正链、多聚腺苷酸化的RNA,估计大小为15 kb。对所得序列的分析确定了三个完整的开放阅读框(ORF),它们有可能编码预测分子量分别为22.2K(ORF 5)、19.1K(ORF 6)和13.6K(ORF 7)的多肽。最靠近3'端的ORF 7预计编码一种高度碱性的核衣壳蛋白,与欧洲PRRSV分离株莱利斯塔德病毒(LV)的相应蛋白具有58%的氨基酸同一性。位于ORF 7之前的ORF 6和ORF 5预计各自编码含有几个疏水结构域的蛋白质,这些结构域被认为与膜相关。VR 2385的ORF 6蛋白是最保守的结构蛋白。它与LV的等效蛋白具有78%的氨基酸同一性,而ORF 5仅共享其54%的氨基酸序列。Northern印迹分析显示,在VR 2385病毒感染的CRL 11171细胞中存在一组3'端共末端的六个亚基因组RNA。我们的结果表明,VR 2385与LV一样,是新提出的动脉炎病毒属的成员。然而,LV和VR 2385之间显著的遗传变异和致病性差异表明,在美国和欧洲引起PRRS的病毒具有高度变异性,它们可能代表不同的基因型。

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