首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Development of a Heteroduplex Mobility Assay To Identify Field Isolates of Porcine Reproductive and Respiratory Syndrome Virus with Nucleotide Sequences Closely Related to Those of Modified Live-Attenuated Vaccines
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Development of a Heteroduplex Mobility Assay To Identify Field Isolates of Porcine Reproductive and Respiratory Syndrome Virus with Nucleotide Sequences Closely Related to Those of Modified Live-Attenuated Vaccines

机译:异源双链移动性分析方法的发展以鉴定具有与修饰的活弱疫苗相近的核苷酸序列的猪繁殖与呼吸综合征病毒的野外分离株

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摘要

Porcine reproductive and respiratory syndrome has been devastating the swine industry since the late 1980s. The disease has been controlled, to some extent, through the use of modified live-attenuated (MLV) vaccines once available. However, such a practice periodically resulted in isolation or detection of vaccine-like viruses from pigs as determined by a partial genomic sequencing. In this study, we developed a heteroduplex mobility assay (HMA) for quickly identifying porcine reproductive and respiratory syndrome virus (PRRSV) isolates with significant nucleotide sequence identities (≥98%) with the modified live-attenuated vaccines. The major envelope gene (ORF5) of 51 PRRSV field isolates recovered before and after the introduction of the vaccines was amplified, denatured, and reannealed with the HMA reference vaccine strains Ingelvac PRRS MLV and Ingelvac PRRS ATP, respectively. Nine of the 51 field isolates and the VR2332 parent virus of Ingelvac PRRS MLV, which were all highly related to Ingelvac PRRS MLV with ≤2% nucleotide sequence divergence as determined by sequence analysis, were all identified by the HMA to form homoduplexes with the reference Ingelvac PRRS MLV. No homoduplex-forming field isolate was identified when Ingelvac PRRS ATP was used as the HMA reference except for its parent virus JA142. Other field isolates with more than 2% nucleotide sequence divergence with the respective reference vaccine strain resulted in the formation of heteroduplexes with reduced mobility in polyacrylamide gel electrophoresis. The HMA results also correlated well with the results of phylogenetic analyses. The data indicated that the HMA developed in the study may be a rapid and efficient method for large-scale screening of potential vaccine-like PRRSV field isolates for further genetic characterization.
机译:自1980年代后期以来,猪繁殖与呼吸综合症就一直在破坏着养猪业。通过使用改良的减毒活疫苗在某种程度上已经控制了该病。但是,通过部分基因组测序确定,这种做法会定期导致从猪中分离或检测疫苗样病毒。在这项研究中,我们开发了一种异源双链迁移分析(HMA),用于通过改良的减毒活疫苗快速鉴定具有显着核苷酸序列同一性(≥98%)的猪繁殖与呼吸综合征病毒(PRRSV)分离株。在导入疫苗之前和之后回收的51个PRRSV野外分离株的主要包膜基因(ORF5)分别进行了扩增,变性和分别与HMA参考疫苗株Ingelvac PRRS MLV和Ingelvac PRRS ATP退火。 HMA鉴定了51个与Ingelvac PRRS MLV高度分离的野外分离株和VR2332亲本病毒,它们均与Ingelvac PRRS MLV高度相关,通过序列分析确定其≤2%核苷酸序列差异,并与参考文献形成同源双链体。 Ingelvac PRRS MLV。当将Ingelvac PRRS ATP用作HMA参照物时,除其同源病毒JA142外,未鉴定到同源双链体形成场。与相应的参考疫苗株相比,具有超过2%核苷酸序列差异的其他野外分离株导致形成异源双链体,聚丙烯酰胺凝胶电泳的迁移率降低。 HMA结果也与系统发育分析结果紧密相关。数据表明,该研究中开发的HMA可能是一种快速有效的方法,可用于大规模筛选潜在的疫苗样PRRSV现场分离株,以进行进一步的基因表征。

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