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通过实时聚合酶链反应对实验感染和自然感染马匹鼻分泌物中马疱疹病毒1型载量进行定量的四种方法的比较

Comparison of four methods to quantify Equid herpesvirus 1 load by real-time polymerase chain reaction in nasal secretions of experimentally and naturally infected horses.

作者信息

Pusterla Nicola, Hussey Stephen B, Mapes Samantha, Leutenegger Christian M, Madigan John E, Ferraro Gregory L, Wilson W David, Lunn D Paul

机构信息

Department of Medicine and Epidemiology, School of Veterinary Medicine, University of California, Davis, CA 95616, USA.

出版信息

J Vet Diagn Invest. 2009 Nov;21(6):836-40. doi: 10.1177/104063870902100611.

DOI:10.1177/104063870902100611
PMID:19901285
Abstract

The objective of the current study was to compare the performance of 4 methods to quantify Equid herpesvirus 1 (EHV-1) by real-time polymerase chain reaction (PCR) in nasal secretions from experimentally and naturally infected horses. Nasal secretions were collected on the challenge day and daily thereafter for 13 days from 4 experimentally infected horses. Additional nasal swabs were collected from 30 horses with clinical signs consistent with natural EHV-1 infection. Absolute quantitation of EHV-1 target molecules was performed using standard curves for EHV-1 and equine glyceraldehyde-3-phosphate dehydrogenase, and DNA yield, and was expressed as EHV-1 glycoprotein B (gB) gene copies per million nucleated nasal cells, EHV-1 gB gene copies per entire swab, EHV-1 gB gene copies per 1 microl of purified DNA, and EHV-1 gB gene copies per 1 ng of template DNA. The study results showed that all 4 calculation methods yielded comparable results between experimentally and naturally infected horses, and that the different methods were significantly correlated with each other. Reporting of quantitative results for EHV-1 viral load in nasal swabs collected from infected horses constitutes an important advance in both the research and diagnostic fields, allowing one to determine the infectious risk of affected horses, disease stage, or response to antiviral therapy. However, protocols that normalize the PCR results against a preselected volume of DNA or nasal secretions are likely to be more prone to variations than protocols that calculate the load for the entire swab, incorporate a housekeeping gene, or use a constant amount of extracted DNA.

摘要

本研究的目的是比较4种通过实时聚合酶链反应(PCR)对实验感染和自然感染马匹鼻分泌物中的马疱疹病毒1型(EHV-1)进行定量的方法。在攻毒当天及此后13天,每天从4匹实验感染的马采集鼻分泌物。另外从30匹有符合自然EHV-1感染临床症状的马采集鼻拭子。使用EHV-1和马甘油醛-3-磷酸脱氢酶的标准曲线以及DNA产量对EHV-1靶分子进行绝对定量,并表示为每百万有核鼻细胞中的EHV-1糖蛋白B(gB)基因拷贝数、每个完整拭子中的EHV-1 gB基因拷贝数、每1微升纯化DNA中的EHV-1 gB基因拷贝数以及每1纳克模板DNA中的EHV-1 gB基因拷贝数。研究结果表明,所有4种计算方法在实验感染和自然感染的马匹之间产生了可比的结果,并且不同方法之间具有显著的相关性。报告从感染马匹采集的鼻拭子中EHV-1病毒载量的定量结果在研究和诊断领域都是一项重要进展,能够确定受感染马匹的感染风险、疾病阶段或对抗病毒治疗的反应。然而,与计算整个拭子的载量、纳入管家基因或使用恒定数量的提取DNA的方案相比,将PCR结果相对于预先选定体积的DNA或鼻分泌物进行标准化的方案可能更容易出现变化。

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