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A long distance RT-PCR able to amplify the Pestivirus genome

机译:能够扩增瘟病毒基因组的长距离RT-PCR

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摘要

A method to amplify long genomic regions (up to ∼12.3 kb) from pestiviruses in one RT-PCR is described. The difficulty in designing conserved primers for the amplification of genomes from highly divergent isolates simply by means of overlapping segments is demonstrated using new bioinformatic tools. An alternative procedure consisting of optimizing the length of the genomic cDNA fragments and their subsequent amplification by polymerase chain reaction (PCR) using a limited set of specific primers is described. The amplification of long DNA fragments from a variety of sources, including genomic, mitochondrial, and viral DNAs as well as cDNA produced by reverse transcription (RT) has been achieved using this methodology, known as long distance PCR. In the case of viruses, it is necessary to obtain viral particles from infected cells prior to RT procedures. This work provides improvements in four steps of long distance RT-PCR (L-RT-PCR): (i) preparation of a viral stock, (ii) preparation of template RNA, (iii) reverse transcription and (iv) amplification of the cDNA by LD-PCR. The usefulness of L-RT-PCR is discussed in the light of current knowledge on pestivirus diversity. The genomic sequence of _ reference strain obtained using this method is presented and characterized.
机译:描述了一种在一次RT-PCR中从瘟疫病毒中扩增长基因组区域(最大约12.3kb)的方法。使用新的生物信息学工具证明了设计保守引物以简单地通过重叠区段从高度不同的分离物中扩增基因组的困难。描述了一种替代方法,包括优化基因组cDNA片段的长度,以及随后使用有限的一组特异性引物通过聚合酶链反应(PCR)对其进行的扩增。使用这种方法(称为长距离PCR)已实现了从多种来源的长DNA片段的扩增,包括基因组,线粒体和病毒DNA以及通过逆转录(RT)产生的cDNA。对于病毒,有必要在RT程序之前从感染的细胞中获得病毒颗粒。这项工作对长距离RT-PCR(L-RT-PCR)的四个步骤进行了改进:(i)制备病毒原液,(ii)制备模板RNA,(iii)逆转录和(iv)扩增通过LD-PCR的cDNA。根据有关瘟病毒多样性的最新知识,讨论了L-RT-PCR的有用性。介绍并表征了使用此方法获得的_参考菌株的基因组序列。

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