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dsRNA-Seq: Identification of Viral Infection by Purifying and Sequencing dsRNA

机译:dsRNA-Seq:通过纯化和测序dsRNA鉴定病毒感染

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摘要

RNA viruses are a major source of emerging and re-emerging infectious diseases around the world. We developed a method to identify RNA viruses that is based on the fact that RNA viruses produce double-stranded RNA (dsRNA) while replicating. Purifying and sequencing dsRNA from the total RNA isolated from infected tissue allowed us to recover dsRNA virus sequences and replicated sequences from single-stranded RNA (ssRNA) viruses. We refer to this approach as dsRNA-Seq. By assembling dsRNA sequences into contigs we identified full length or partial RNA viral genomes of varying genome types infecting mammalian culture samples, identified a known viral disease agent in laboratory infected mice, and successfully detected naturally occurring RNA viral infections in reptiles. Here, we show that dsRNA-Seq is a preferable method for identifying viruses in organisms that don’t have sequenced genomes and/or commercially available rRNA depletion reagents. In addition, a significant advantage of this method is the ability to identify replicated viral sequences of ssRNA viruses, which is useful for distinguishing infectious viral agents from potential noninfectious viral particles or contaminants.
机译:RNA病毒是世界范围内新出现和重新出现的传染病的主要来源。我们基于RNA病毒在复制时会产生双链RNA(dsRNA)的事实,开发了一种识别RNA病毒的方法。从感染组织分离的总RNA中纯化dsRNA并对其进行测序,使我们能够从单链RNA(ssRNA)病毒中回收dsRNA病毒序列和复制序列。我们将此方法称为dsRNA-Seq。通过将dsRNA序列组装到重叠群中,我们鉴定了感染哺乳动物培养物样本的各种基因组类型的全长或部分RNA病毒基因组,在实验室感染的小鼠中鉴定了已知的病毒病原体,并成功地检测了爬行动物中自然发生的RNA病毒感染。在这里,我们证明了dsRNA-Seq是在没有测序基因组和/或市售rRNA耗竭剂的生物中鉴定病毒的首选方法。另外,该方法的显着优势是能够鉴定ssRNA病毒的复制病毒序列,这对于将传染性病毒制剂与潜在的非传染性病毒颗粒或污染物区分开很有用。

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