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分子检测方法的选择决定了蛙病毒的检测概率以及对流行率和发生率的推断。

Choice of molecular assay determines ranavirus detection probability and inferences about prevalence and occurrence.

作者信息

Wynne Felicity J, Puschendorf Robert, Knight Mairi E, Price Stephen J

机构信息

School of Biological and Marine Sciences, University of Plymouth, Drake Circus, Plymouth, Devon, PL4 8AA, UK.

出版信息

Dis Aquat Organ. 2020 Sep 24;141:139-147. doi: 10.3354/dao03518.

DOI:10.3354/dao03518
PMID:32969346
Abstract

Ranaviruses are emerging pathogens that can cause morbidity, mortality and population declines in ectothermic hosts; however, there is no standardized approach to diagnostics. Here, we compared the inter-assay variation and intra-assay precision among 2 commonly used quantitative PCRs (qPCRs), a conventional and a nested PCR assay (used as a gold standard), using laboratory-propagated ranavirus (FV3 and CMTV) and field-collected samples. A qPCR assay ('Leung') detected viral DNA in dilutions 2 orders of magnitude lower than other assays regardless of the viral lineage of the cultured isolate (FV3/CMTV). The second qPCR ('Brunner') was slightly more sensitive than the conventional PCR ('Mao' assay). For field samples, the Leung qPCR detected all known positives, while the Mao assay PCR only detected 2.5% of the positive samples. Amplicon sequences from the 2 conventional PCRs were shown to be useful for inferring viral lineage. Inaccurate results will bias estimates of the distribution and prevalence of ranaviruses, and together these findings emphasize that molecular assays should be chosen carefully in the context of study aims.

摘要

蛙病毒是新出现的病原体,可导致变温动物宿主发病、死亡和种群数量下降;然而,目前尚无标准化的诊断方法。在此,我们使用实验室繁殖的蛙病毒(FV3和CMTV)以及野外采集的样本,比较了两种常用定量PCR(qPCR)、一种常规PCR和一种巢式PCR检测方法(用作金标准)之间的检测间差异和检测内精密度。一种qPCR检测方法(“Leung”)在比其他检测方法低两个数量级的稀释度下就能检测到病毒DNA,无论培养分离株(FV3/CMTV)的病毒谱系如何。第二种qPCR(“Brunner”)比常规PCR(“Mao”检测方法)稍敏感一些。对于野外样本,Leung qPCR检测到了所有已知阳性样本,而Mao检测方法的PCR仅检测到2.5%的阳性样本。两种常规PCR的扩增子序列显示可用于推断病毒谱系。不准确的结果会使蛙病毒分布和流行率的估计产生偏差,这些发现共同强调,应根据研究目的谨慎选择分子检测方法。

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