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一种基于序列无关、单引物扩增(SISPA)和纳米孔测序的方法,用于检测和鉴定蜱传病毒病原体。

Utility of a Sequence-Independent, Single-Primer-Amplification (SISPA) and Nanopore Sequencing Approach for Detection and Characterization of Tick-Borne Viral Pathogens.

机构信息

Center for Biological Threats and Special Pathogens 1 (ZBS-1), Robert Koch Institute, 13353 Berlin, Germany.

Department of Virology, Faculty of Veterinary Medicine, Dokuz Eylül University, İzmir 35890, Turkey.

出版信息

Viruses. 2021 Jan 29;13(2):203. doi: 10.3390/v13020203.

Abstract

Currently, next generation sequencing (NGS) is the mainly used approach for identification and monitorization of viruses with a potential public health threat in clinical and environmental samples. To facilitate detection in NGS, the sequence-independent, single-primer-amplification (SISPA) is an effective tool for enriching virus sequences. We performed a preliminary assessment of SISPA-nanopore sequencing as a potential approach for screening tick-borne viruses in six specimens with detectable Crimean-Congo hemorrhagic fever virus (CCHFV) and Jingmen tick virus (JMTV) sequences. A comparison of unbiased NGS and SISPA followed by nanopore sequencing was carried out in 4 specimens with single and pooled ticks. The approach was further used for genome sequencing in culture-grown viruses. Overall, total/virus-specific read counts were significantly elevated in cell culture supernatants in comparison to single or pooled ticks. Virus genomes could be successfully characterized by SISPA with identities over 99%. Genome coverage varied according to the segment and total read count. Base calling errors were mainly observed in tick specimens and more frequent in lower viral loads. Culture-grown viruses were phylogenetically-related to previously-reported local viruses. In conclusion, the SISPA + nanopore sequencing was successful in generating data comparable to NGS and will provide an effective tool for broad-range virus detection in ticks.

摘要

目前,下一代测序(NGS)是在临床和环境样本中鉴定和监测具有潜在公共卫生威胁的病毒的主要方法。为了便于在 NGS 中检测,无序列依赖性、单引物扩增(SISPA)是富集病毒序列的有效工具。我们初步评估了 SISPA-纳米孔测序作为一种潜在的方法,用于筛查六种具有可检测克里米亚-刚果出血热病毒(CCHFV)和荆门 tick 病毒(JMTV)序列的标本中的 tick 传播病毒。在 4 份具有单 tick 和 pooled tick 的标本中,进行了无偏 NGS 和 SISPA 后纳米孔测序的比较。该方法进一步用于培养病毒的基因组测序。总体而言,与单个或 pooled tick 相比,细胞培养上清液中的总/病毒特异性读数显著升高。通过 SISPA 可以成功地对病毒基因组进行特征分析,其身份超过 99%。根据片段和总读数,基因组覆盖率有所不同。碱基调用错误主要发生在 tick 标本中,并且在较低病毒载量时更频繁。培养的病毒与之前报道的本地病毒在系统发育上相关。总之,SISPA +纳米孔测序成功地生成了与 NGS 相当的数据,将为 tick 中的广谱病毒检测提供有效的工具。

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