优化呼吸道病毒全基因组测序快速抗原检测的核酸回收率

IF 4 3区 医学 Q2 VIROLOGY Journal of Clinical Virology Pub Date : 2024-07-15 DOI:10.1016/j.jcv.2024.105714
G Butel-Simoes , E Steinig , I Savic , M Zhanduisenov , G Papadakis , T Tran , J Moselen , L Caly , DA Williamson , CK Lim
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引用次数: 0

摘要

背景对来自快速抗原检测(RAT-WGS)的呼吸道病毒进行全基因组测序(WGS)是扩大呼吸道感染基因组监测的一种新方法。但迄今为止,有关这些病毒在 RAT 上的基因组稳定性的数据还很有限。在本研究中,我们研究了储存条件和核酸防腐剂对增强稳定性和提高从 RAT 身上回收呼吸道病毒基因组的能力的影响。方法在不同的环境温度(4°C、20°C 和 36°C)下,用两种防腐试剂(RNALater 和 DNA/RNA 屏蔽)将常见呼吸道病毒的混合物接种到大鼠体内,在两个不同的时间点(72 小时和 7 天)从大鼠体内提取核酸,并进行实时多重呼吸道 PCR 检测一系列呼吸道病毒。利用 TWIST 综合病毒研究小组的目标富集技术进行 WGS 检测。结果核酸降解(以 PCR 周期阈值的相对变化和基于 WGS 的指标表示)在 20 °C 和 36 °C 时最为显著。在所有温度条件下,在 RNALater 或 DNA / RNA 屏蔽层中储存都能提高呼吸道病毒的基因组恢复能力,但在 RNALater 中最为明显。结论在模拟条件下,RAT-WGS 证明:(i) 病毒基因组在 4°C 的 72 小时和 1 周内基本稳定;(ii) 与 DNA/RNA 屏蔽相比,RNALater 能更有效地保存核酸;(iii) 在 RNALater 中,每个样本的测序深度为 500,000 个读数,在所有呼吸道病毒和条件下都能实现基因组恢复。
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Optimising nucleic acid recovery from rapid antigen tests for whole genome sequencing of respiratory viruses

Background

Whole genome sequencing (WGS) of respiratory viruses from rapid antigen tests (RAT-WGS) is a novel approach to expanding genomic surveillance of respiratory infections. To date however, there are limited data on the genomic stability of these viruses on RATs. In this study, we investigated the effect of storage conditions and nucleic acid preservatives on the ability to enhance stability and improve recovery of respiratory virus genomes from RATs.

Methods

A mixture of common respiratory viruses was used to inoculate RATs at different environmental temperatures (4°C, 20°C and 36°C), with two preservative reagents (RNALater and DNA/RNA shield) Nucleic acid was extracted from RATs at two different timepoints (72 h and seven days) and subject to real-time multiplex respiratory PCR to detect a range of respiratory viruses. WGS was performed using target-enrichment with the TWIST Comprehensive Viral Research Panel. Defined metrics from an automated in-house bioinformatic pipeline were used to assess and compare viral genome recovery under different conditions.

Results

Nucleic acid degradation (indicated by relative change in PCR cycle threshold and WGS-based metrics) was most notable at 20 °C and 36 °C. Storage in either RNALater or DNA / RNA shield improved genome recovery for respiratory viruses across all temperature conditions, although this was most pronounced for RNALater. Subtyping of Influenza viruses demonstrated the applicability of RAT-WGS in downstream genomic epidemiological surveillance.

Conclusions

Under simulated conditions, RAT-WGS demonstrated that (i) viral genomes were generally stable at 4°C at 72 h and 1 week, (ii) RNALater has a more significant preservation of nucleic acids compared to DNA/RNA Shield and (iii) genome recovery can be achieved using a sequencing depth of 500,000 reads per sample in RNALater, across all respiratory viruses and conditions.

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来源期刊
Journal of Clinical Virology
Journal of Clinical Virology 医学-病毒学
CiteScore
22.70
自引率
1.10%
发文量
149
审稿时长
24 days
期刊介绍: The Journal of Clinical Virology, an esteemed international publication, serves as the official journal for both the Pan American Society for Clinical Virology and The European Society for Clinical Virology. Dedicated to advancing the understanding of human virology in clinical settings, the Journal of Clinical Virology focuses on disseminating research papers and reviews pertaining to the clinical aspects of virology. Its scope encompasses articles discussing diagnostic methodologies and virus-induced clinical conditions, with an emphasis on practicality and relevance to clinical practice. The journal publishes on topics that include: • new diagnostic technologies • nucleic acid amplification and serologic testing • targeted and metagenomic next-generation sequencing • emerging pandemic viral threats • respiratory viruses • transplant viruses • chronic viral infections • cancer-associated viruses • gastrointestinal viruses • central nervous system viruses • one health (excludes animal health)
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