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从 cDNA 构建体中恢复细胞病变性和非细胞病变性牛病毒性腹泻病毒。

Recovery of cytopathogenic and noncytopathogenic bovine viral diarrhea viruses from cDNA constructs.

作者信息

Meyers G, Tautz N, Becher P, Thiel H J, Kümmerer B M

机构信息

Department of Clinical Virology, Federal Research Centre for Virus Diseases of Animals, Tübingen, Germany.

出版信息

J Virol. 1996 Dec;70(12):8606-13. doi: 10.1128/JVI.70.12.8606-8613.1996.

Abstract

After cDNA cloning of the genome of bovine viral diarrhea virus (BVDV) isolate CP7, a full-length cDNA clone was constructed. RNA transcribed in vitro from this construct was shown to direct the generation of infectious BVDV upon transfection into bovine cells. To confirm the de novo generation of infectious BVDV from cloned cDNA a genetically tagged virus was constructed. In comparison with parental BVDV, the recombinant virus was slightly retarded in growth. The NS2 coding region of the CP7 genome contains a duplication of 27 nucleotides which is not present in the genome of its noncytopathogenic counterpart, NCP7. Exchange of a small fragment harboring this insertion against the corresponding part of the NCP7 sequence led to recovery of noncytopathogenic BVDV. Alteration of the construct by introduction of a fragment derived from a cytopathogenic BVDV defective interfering particle resulted in a chimeric defective interfering particle which exhibits a cytopathogenic phenotype. These findings confirm the hypothesis that the recombination-induced alterations in the genomes of cytopathogenic BVDV are responsible for the induction of cell lysis.

摘要

在对牛病毒性腹泻病毒(BVDV)分离株CP7的基因组进行cDNA克隆后,构建了一个全长cDNA克隆。从该构建体体外转录的RNA在转染到牛细胞后被证明可指导产生感染性BVDV。为了证实从克隆的cDNA中从头产生感染性BVDV,构建了一种基因标记病毒。与亲本BVDV相比,重组病毒的生长略有延迟。CP7基因组的NS2编码区包含一个27个核苷酸的重复序列,而其非致细胞病变对应物NCP7的基因组中不存在该重复序列。将含有此插入片段的小片段与NCP7序列的相应部分进行交换,导致非致细胞病变的BVDV的恢复。通过引入源自致细胞病变的BVDV缺陷干扰颗粒的片段来改变构建体,产生了一种具有致细胞病变表型的嵌合缺陷干扰颗粒。这些发现证实了以下假设:致细胞病变的BVDV基因组中重组诱导的改变是导致细胞裂解的原因。

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