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A new multiplex RT-qPCR method for the simultaneous detection and discrimination of Zika and chikungunya viruses

机译:一种新的多重RT-QPCR方法,用于同时检测和歧视Zika和Chikungunya病毒

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摘要

Objective The re-emergence and spread of tropical viruses to new areas has raised a wave of concern worldwide. In order to treat patients at an early stage and prevent the diffusion of an outbreak, early diagnosis, and therefore fast and adequate detection, is needed. To this end, a multiplex reverse transcription real-time polymerase chain reaction TaqMan method was designed to detect Zika (ZIKV) and chikungunya (CHIKV) viruses simultaneously. Methods Two methods targeting different genome segments were selected from the literature for each virus. These were adapted for high genome coverage and combined in a four-plex assay that was thoroughly validated in-house. The SCREENED tool was used to evaluate the sequence coverage of the method. Results The full validation approach showed that the new four-plex method allows the specific and sensitive identification and discrimination of ZIKV and CHIKV in routine samples. The combination of two targets per virus allowing almost 100% coverage of about 500 genomes is shown for the first time. Conclusions PCR is a reliable user-friendly technique that can be applied in remote areas. Such multiplex methods enable early and efficient diagnosis, leading to rapid treatment and effective confinement in outbreak cases. They may also serve as an aid for surveillance, and the full validation permits easy method-transfer allowing worldwide harmonization.
机译:客观热带病毒对新地区的重新出现和传播在全球范围内提出了一股关注的浪潮。为了在早期治疗患者并防止爆发的扩散,需要早期诊断,因此快速和足够的检测。为此,多重逆转录实时聚合酶链反应Taqman方法旨在同时检测Zika(Zikv)和Chikungunya(Chikv)病毒。方法选自各种病毒的文献中靶向不同基因组段的两种方法。这些适用于高基因组覆盖率,并结合在内部彻底验证的四个plex测定中。筛选的工具用于评估该方法的序列覆盖范围。结果全面验证方法表明,新的四个PLEX方法允许在常规样本中进行特定和敏感的ZIKV和CHIKV的鉴定和辨别。每种病毒的两个靶标的组合是第一次显示几乎100%基因组的覆盖率。结论PCR是一种可靠的用户友好技术,可应用于偏远地区。这种多重方法使得早期和高效诊断,导致爆发案件的快速治疗和有效的禁闭。它们也可以作为监视的援助,完整的验证允许允许全球协调的简单方法转移。

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