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首页> 外文期刊>Journal of Virological Methods >Simplified recombinational approach for influenza A virus reverse genetics.
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Simplified recombinational approach for influenza A virus reverse genetics.

机译:甲型流感病毒反向遗传学的简化重组方法。

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Influenza A virus (FLUAV) reverse genetics requires the cloning of all eight viral genome segments into genomic expression plasmids using restriction enzyme cleavage and ligation. Herein is described the construction of a pair of plasmid vectors and their use in RecA Escherichia coli for direct recombination with influenza cDNA for reverse genetics. This approach is simpler; avoiding restriction digestion and ligation while maintaining the required orientation of genome segments. For this recombinational approach two plasmid constructs were generated, pHH21A and pHH21G, that both possess a 25 nucleotide recombination cassette comprised of the consensus 5' and 3' ends of the negative strand divided by a StuI cleavage site, but that differ at position 4 from the 3' end due to the presence of an A or G nucleotide (plus sense) to correspond to differences among genome segments. Using the described procedure it was possible to clone viral cDNA genomes of several avian and human FLUAVs into genomic expression plasmids in a single recombination step. This novel approach to generating sets of genomic plasmid constructs for reverse genetics reduces the time and complexity of procedures thus avoiding complications that would delay rescue of viral genomes for vaccine production or biological characterization and analysis.
机译:甲型流感病毒(FLUAV)反向遗传学要求使用限制酶切割和连接将所有八个病毒基因组片段克隆到基因组表达质粒中。本文描述了一对质粒载体的构建及其在RecA大肠杆菌中与流感cDNA直接重组用于反向遗传学的用途。这种方法比较简单。避免限制性消化和连接,同时保持所需的基因组片段方向。对于这种重组方法,生成了两个质粒构建体,pHH21A和pHH21G,它们都具有25个核苷酸的重组盒,由负链的共有5'和3'末端除以StuI切割位点组成,但在第4位与3'端由于存在A或G核苷酸(正向)而与基因组片段之间的差异相对应。使用所描述的方法,有可能在单个重组步骤中将几种禽和人FLUAV的病毒cDNA基因组克隆到基因组表达质粒中。这种产生用于逆向遗传学的基因组质粒构建体组的新颖方法减少了程序的时间和复杂性,从而避免了会延误病毒基因组抢救用于疫苗生产或生物学表征和分析的并发症。

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