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Infectious foot-and-mouth disease virus derived from a cloned full-length cDNA.

机译:源于克隆全长cDNA的传染性口蹄疫病毒。

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摘要

A full-length cDNA plasmid of foot-and-mouth disease virus has been constructed. RNA synthesized in vitro by means of a bacteriophage SP6 promoter inserted in front of the cDNA led to the production of infectious particles upon transfection of BHK-21 cells. These particles were also found to be highly infectious for primary bovine kidney cells as well as for baby mice. The difficulty in cloning the foot-and-mouth disease virus cytidyl tract in Escherichia coli was circumvented by joining two separate cloned parts, representing the S and L fragments of the genome, and, in a second step, inserting a dC-dG homopolymer. Homopolymeric sequences of up to 25 cytidyl residues did not lead to the production of virus. Replicons containing poly(C) tracts long enough to permit virus replication were first established in yeast cells. One of these constructs could also be maintained in E. coli and was used to produce infectious RNA in vitro. The length of the poly(C) sequence in this cDNA plasmid was 32 nucleotides. However, the poly(C) tracts of two recombinant viruses found in transfected BHK-21 cells were 60 and 80 nucleotides long, respectively. Possible mechanisms leading to the enlargement of the poly(C) tract during virus replication are discussed.
机译:已经构建了口蹄疫病毒的全长cDNA质粒。通过插入cDNA前面的噬菌体SP6启动子在体外合成的RNA导致在转染BHK-21细胞后产生感染性颗粒。还发现这些颗粒对原代牛肾细胞和小小鼠具有高度传染性。通过将代表基因组S和L片段的两个分离的克隆部分连接起来,并在第二步中插入dC-dG均聚物,可以避免在大肠杆菌中克隆口蹄疫病毒胞苷基的困难。最多25个胞苷基残基的均聚物序列不会导致病毒的产生。首先在酵母细胞中建立了含有足以允许病毒复制的多聚(C)片段的复制子。这些构建体之一也可以保留在大肠杆菌中,并用于体外产生感染性RNA。该cDNA质粒中poly(C)序列的长度为32个核苷酸。但是,在转染的BHK-21细胞中发现的两种重组病毒的poly(C)片段分别长60和80个核苷酸。讨论了在病毒复制过程中导致poly(C)管道扩大的可能机制。

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