Design, development, and validation of a strand-specific RT-qPCR assay to differentiate replicating versus nonreplicating Rabies virus

IF 2.2 4区 医学 Q3 BIOCHEMICAL RESEARCH METHODS
Hong Xiang, Chao Hong, Yuan Tian, Yu Gao, Yina Cun, Hongling Zhao, Guilan Li, Yu Chen, Jian Zhou
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引用次数: 0

Abstract

The Rabies virus, a single-strand RNA virus with a negative-sense polarity, is responsible for causing encephalitis and is a zoonotic disease. If not promptly treated after infection, it has a close to 100 % fatality rate. Similar to other negative-sense polarity single-strand RNA viruses, the Rabies virus requires the creation of a positive-strand RNA intermediate for replication. One approach to identify this replication activity is to detect the complementary strand of the viral RNA genome in suspected infected cells or tissues. The reported Rabies virus RT-qPCR detection methods are designed to detect total viral load in samples without distinguishing between positive- and negative-strand for RNA viruses. As such, in this study, a sensitive Taqman-based strand-specific RT-qPCR assay has been developed to quantitatively detect both the positive- and negative-strand of the Rabies virus. This method demonstrates good reproducibility across a wide dynamic range and exhibits linearity of 8 logs with a lower limit of detection of 103 copies/μL for the positive-strand and 9 logs with a lower limit of detection of 102 copies/μL for the negative-strand. Notably, it can accurately detect a specific viral RNA strand even in the presence of high levels of the opposite strand, confirming the method’s specificity. In summary, a reliable strand-specific RT-qPCR assay has been developed and validated to differentiate replicating from non-replicating Rabies virus.
设计、开发和验证用于区分复制与非复制狂犬病病毒的链特异性 RT-qPCR 检测方法。
狂犬病病毒是一种具有负义极性的单链 RNA 病毒,可引起脑炎,是一种人畜共患病。如果感染后不及时治疗,死亡率接近 100%。与其他负义极性单链 RNA 病毒类似,狂犬病病毒的复制也需要产生正链 RNA 中间体。确定这种复制活动的一种方法是检测可疑感染细胞或组织中病毒 RNA 基因组的互补链。已报道的狂犬病病毒 RT-qPCR 检测方法旨在检测样本中的总病毒载量,而不区分 RNA 病毒的正链和负链。因此,本研究开发了一种灵敏的基于 Taqman 的特异性链 RT-qPCR 检测方法,可定量检测狂犬病病毒的阳性链和阴性链。该方法在宽动态范围内具有良好的重现性,阳性链的线性度为 8 logs,检测下限为 103 copies/μL;阴性链的线性度为 9 logs,检测下限为 102 copies/μL。值得注意的是,即使存在高水平的反向链,它也能准确检测出特定的病毒 RNA 链,从而证实了该方法的特异性。总之,我们开发并验证了一种可靠的特异性链 RT-qPCR 检测方法,可用于区分复制与非复制狂犬病病毒。
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来源期刊
CiteScore
5.80
自引率
0.00%
发文量
209
审稿时长
41 days
期刊介绍: The Journal of Virological Methods focuses on original, high quality research papers that describe novel and comprehensively tested methods which enhance human, animal, plant, bacterial or environmental virology and prions research and discovery. The methods may include, but not limited to, the study of: Viral components and morphology- Virus isolation, propagation and development of viral vectors- Viral pathogenesis, oncogenesis, vaccines and antivirals- Virus replication, host-pathogen interactions and responses- Virus transmission, prevention, control and treatment- Viral metagenomics and virome- Virus ecology, adaption and evolution- Applied virology such as nanotechnology- Viral diagnosis with novelty and comprehensive evaluation. We seek articles, systematic reviews, meta-analyses and laboratory protocols that include comprehensive technical details with statistical confirmations that provide validations against current best practice, international standards or quality assurance programs and which advance knowledge in virology leading to improved medical, veterinary or agricultural practices and management.
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