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Next-generation sequencing of dsRNA is greatly improved by treatment with the inexpensive denaturing reagent DMSO

机译:通过使用廉价的变性试剂DMSO处理极大地改善了dsRNA的下一代测序

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摘要

dsRNA is the genetic material of important viruses and a key component of RNA interference-based immunity in eukaryotes. Previous studies have noted difficulties in determining the sequence of dsRNA molecules that have affected studies of immune function and estimates of viral diversity in nature. DMSO has been used to denature dsRNA prior to the reverse-transcription stage to improve reverse transcriptase PCR and Sanger sequencing. We systematically tested the utility of DMSO to improve the sequencing yield of a dsRNA virus (Φ6) in a short-read next-generation sequencing platform. DMSO treatment improved sequencing read recovery by over two orders of magnitude, even when RNA and cDNA concentrations were below the limit of detection. We also tested the effects of DMSO on a mock eukaryotic viral community and found that dsRNA virus reads increased with DMSO treatment. Furthermore, we provide evidence that DMSO treatment does not adversely affect recovery of reads from a ssRNA viral genome (influenza A/California/07/2009). We suggest that up to 50 % DMSO treatment be used prior to cDNA synthesis when samples of interest are composed of or may contain dsRNA.
机译:dsRNA是重要病毒的遗传物质,是真核生物中基于RNA干扰的免疫力的关键组成部分。先前的研究已经指出,很难确定影响自然免疫功能和估计病毒多样性的dsRNA分子的序列。 DMSO已用于在逆转录阶段之前使dsRNA变性,以改善逆转录酶PCR和Sanger测序。我们系统地测试了DMSO在短读下一代测序平台中提高dsRNA病毒(Φ6)测序产量的效用。即使RNA和cDNA浓度低于检测极限,DMSO处理也可将测序读取恢复提高两个数量级以上。我们还测试了DMSO对模拟真核病毒群落的影响,并发现DMSO处理后dsRNA病毒读数增加。此外,我们提供了证据,即DMSO处理不会对从ssRNA病毒基因组读取的数据产生不利影响(甲型流感/加利福尼亚州2009年7月)。我们建议,当目标样品由dsRNA组成或可能包含dsRNA时,在cDNA合成之前应使用高达50%的DMSO处理。

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