Development and evaluation of a quadruple real-time fluorescence-based quantitative reverse transcription polymerase chain reaction assay for detecting Langya, Mojiang, Nipah, and Cedar viruses

IF 3.5 Q1 PUBLIC, ENVIRONMENTAL & OCCUPATIONAL HEALTH
Wenjun He , Tian Ma , Yalan Wang , Weifang Han , Jun Liu , Wenwen Lei , Le Zhang , Guizhen Wu
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引用次数: 0

Abstract

The emerging viruses within the genus Henipavirus in the family Paramyxoviridae pose a great threat to public biosafety. To develop a quadruple real-time fluorescence-based quantitative reverse transcription polymerase chain reaction (qRT-PCR) assay is pivotal for the early warning of the potential of zoonotic infectious diseases. Specific primers and probes were designed for the relatively conserved regions based on whole genome sequences of Langya virus (LayV), Mojiang virus (MojV), Nipah virus (NiV), and Cedar virus (CedV), followed by the establishment of a quadruple real-time fluorescence-based qRT-PCR detection method. No cross-reactivity was observed with other viral nucleic acids. The optimal linear detection range for LayV, MojV, NiV, and CedV was 101-108 copies/μL, and the lower limit of detection was 10 copies/μL. Three different DNA concentrations of LayV, MojV, NiV, and CedV (104, 105, and 106 copies/μL) were tested 14 times, achieving good repeatability. The standard deviation of the cycle threshold values for each concentration was <0.5 and the coefficient of variation was <3 %. Furthermore, the amplification efficiency of quadruple real-time fluorescence-based qRT-PCR was >90 %, and the correlation coefficient was >0.99. The established quadruple real-time fluorescence-based qRT-PCR assay for the detection of LayV, MojV, NiV, and CedV exhibits good sensitivity, specificity, and repeatability. Therefore, it can be used to detect Henipavirus and other related clinical specimens.

开发和评估用于检测琅琊、墨江、尼帕和雪松病毒的四重实时荧光定量反转录聚合酶链反应测定法
副粘病毒科 Henipavirus 属中新出现的病毒对公共生物安全构成了巨大威胁。开发一种基于四重实时荧光定量反转录聚合酶链反应(qRT-PCR)的检测方法,对于早期预警潜在的人畜共患传染病至关重要。根据琅琊病毒(LayV)、墨江病毒(MojV)、尼帕病毒(NiV)和雪松病毒(CedV)的全基因组序列,针对相对保守的区域设计了特异性引物和探针,随后建立了基于四重实时荧光的 qRT-PCR 检测方法。没有观察到与其他病毒核酸的交叉反应。LayV、MojV、NiV和CedV的最佳线性检测范围为101-108拷贝/μL,检测下限为10拷贝/μL。对三种不同浓度的 LayV、MojV、NiV 和 CedV(104、105 和 106 拷贝/μL)DNA 进行了 14 次测试,重复性良好。每个浓度的周期阈值的标准偏差为 0.5,变异系数为 3%。此外,基于四重实时荧光的 qRT-PCR 扩增效率为 90%,相关系数为 0.99。所建立的基于四重实时荧光的 qRT-PCR 检测 LayV、MojV、NiV 和 CedV 的方法具有良好的灵敏度、特异性和重复性。因此,该方法可用于检测亨氏病毒及其他相关临床标本。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Biosafety and Health
Biosafety and Health Medicine-Infectious Diseases
CiteScore
7.60
自引率
0.00%
发文量
116
审稿时长
66 days
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