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首页> 外文期刊>Journal of Clinical Microbiology >Comparison of Commercial Real-Time Reverse Transcription-PCR Assays for Reliable, Early, and Rapid Detection of Heterologous Strains of Porcine Reproductive and Respiratory Syndrome Virus in Experimentally Infected or Noninfected Boars by Use of Different Sample Types
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Comparison of Commercial Real-Time Reverse Transcription-PCR Assays for Reliable, Early, and Rapid Detection of Heterologous Strains of Porcine Reproductive and Respiratory Syndrome Virus in Experimentally Infected or Noninfected Boars by Use of Different Sample Types

机译:通过使用不同的样本类型,对在实验感染或未感染公猪中猪繁殖与呼吸综合征病毒的异源菌株进行可靠,早期和快速检测的商业实时逆转录PCR方法的比较

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The aims of this study were to compare three commercial porcine reproductive and respiratory syndrome virus (PRRSV) real-time reverse transcription-PCR (RT-PCR) assays for detection of genetically diverse PRRSV isolates in serum, semen, blood swabs, and oral fluids collected from experimentally infected boars and to evaluate the effects of sample pooling. Six groups of three boars negative for PRRSV were each inoculated with one of six PRRSV isolates (sharing 55 to 99% nucleotide sequence identity in ORF5). Samples were collected on days ?2, 1, 3, 5, 7, 14, and 21 postinoculation (p.i.) and tested by one of three commercially available real-time RT-PCR assays (VetMax from Applied Biosystems, Foster City, CA [abbreviated AB]; VetAlert from Tetracore, Rockville, MD [TC]; and AcuPig from AnDiaTec GmbH, Kornwestheim, Germany [AD]). At day 1 p.i., all assays detected at least one positive sample in each group. The highest detection rates were on days 3 and 5 p.i. Between days 1 and 7 p.i., serum samples had the highest detection rate (90%) with 100% agreement between tests, followed by blood swabs (kappa value of 0.97) and semen (kappa value of 0.80). Oral fluids had the lowest detection rates (AB, 55%; TC, 41%; AD, 46%) and the highest disagreement between kits (kappa value of 0.63). Pools of five samples did not reduce the detection rates if there was one positive sample with a large amount (cycle threshold, <30) of viral RNA in the pool. Serum and blood swab samples had shorter turnaround times for RNA extraction. The AB assay had a 1.6-times-shorter PCR time. In summary, serum and blood swabs had the best performance with highest detection rates and agreement between assays and the shortest turnaround times.
机译:这项研究的目的是比较三种商业猪繁殖与呼吸综合征病毒(PRRSV)实时逆转录PCR(RT-PCR)检测方法,以检测血清,精液,拭子和口腔液中遗传多样的PRRSV分离株从实验感染的公猪收集并评估样品合并的效果。六组PRRSV阴性的三头公猪分别接种了六个PRRSV分离株之一(在ORF5中共有55至99%的核苷酸序列同一性)。在接种后第2、2、1、3、5、7、14和21天收集样品,并通过三种市售实时RT-PCR分析方法之一(来自美国加利福尼亚州Foster City的Applied Biosystems的VetMax [缩写AB];来自Tetracore,Rockville,MD [TC]的VetAlert;以及来自德国Kornwestheim,AnDiaTec GmbH [AD]的AcuPig。在下午1天时,所有测定法均在每组中检测出至少一个阳性样品。最高的发现率是在第3天和第5天。在下午1到7天之间,血清样本的检出率最高(90%),两次检测之间的一致性达到100%,其次是拭子(kappa值为0.97)和精液(kappa值为0.80)。口服液的检出率最低(AB为55%; TC为41%; AD为46%),试剂盒之间的分歧最高(Kappa值为0.63)。如果池中有一个阳性样品中含有大量(循环阈值,<30)病毒RNA,则五个样品池不会降低检测率。血清和血液拭子样本的RNA提取周转时间较短。 AB分析的PCR时间短了1.6倍。总之,血清和血液拭子具有最佳的性能,最高的检出率,测定之间的一致性以及最短的周转时间。

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