Natalya Panova, Nina P Allan, Noelle C Rubas, Rosa H Lee, Braden P Kunihiro, Lesley Umeda, Rafael Peres, Ruben Juarez, Alika K Maunakea
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Stool samples were collected from patients at varying timepoints post-convalescence, and viral DNA was isolated and sequenced using the QIAamp Viral RNA Mini Kit (Qiagen Inc.) and Ion Ampliseq<sup>™</sup> Library Kit Plus (Life Technologies Corporation). Capacity of neutralizing antibodies in patient plasma was tested using a Luminex panel (Coronavirus Ig Total Human 11-Plex ProcartaPlex<sup>™</sup> Panel, ThermoFisher). Of 64 samples obtained from post-acute patients, 21 (32.8%) yielded sufficient material for whole-genome sequencing. This allowed us to identify widely divergent phylogenetic relativity of the SARS-CoV-2 genome from post-acute patients living in the same households and infected around the same time. Additionally, we observed that individuals who recovered from infection expressed varying degrees of antibodies against SARS-CoV-2 structural proteins that corresponded to distinct variants. 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引用次数: 0
摘要
全基因组SARS-CoV-2测序工具对于追踪COVID-19大流行至关重要。然而,目前的技术需要在COVID-19检测后对活跃感染患者进行采样,以从鼻咽通道中恢复足够的SARS-CoV-2 RNA,这些RNA在感染的最初几周内迅速清除。对来自康复的非传染性患者的病毒基因组进行前瞻性评估将极大地促进流行病学追踪。因此,我们制定了一项方案,在症状出现后10-120天的时间点,从急性后SARS-CoV-2患者的粪便样本中分离出SARS-CoV-2基因组并进行测序。在康复后的不同时间点收集患者的粪便样本,使用QIAamp病毒RNA迷你试剂盒(Qiagen Inc.)和Ion Ampliseq™Library Kit Plus (Life Technologies Corporation)分离病毒DNA并进行测序。使用Luminex面板(ThermoFisher公司的冠状病毒Ig Total Human 11-Plex ProcartaPlex™面板)检测患者血浆中中和抗体的能力。从急性后患者获得的64份样本中,21份(32.8%)获得了足够的全基因组测序材料。这使我们能够从生活在同一家庭并在同一时间感染的急性后患者中识别出广泛不同的SARS-CoV-2基因组的系统发育相关性。此外,我们观察到,从感染中恢复的个体表达了不同程度的针对SARS-CoV-2结构蛋白的抗体,这些抗体对应于不同的变体。有趣的是,我们在病毒基因组中发现了一种新的点突变,在这种突变中,与感染野生型病毒的患者相比,受感染患者在体外表达的抗体中和病毒的能力显著降低。总之,我们展示了一种方案,可以成功地从感染后4个月的患者粪便样本中对SARS-CoV-2基因组进行测序,这可以应用于评估大流行期间SARS-CoV-2基因组的临时和安全监测的变异与免疫反应之间的关系的研究。
Sequencing the SARS-CoV-2 Genome from Stool Samples of Post-acute Cases Implicates a Novel Mutation Associated with Reduced Antibody Neutralization.
Whole-genome SARS-CoV-2 sequencing tools are crucial for tracking the COVID-19 pandemic. However, current techniques require sampling of actively infectious patients following COVID-19 testing to recover enough SARS-CoV-2 RNA from the nasopharyngeal passage, which rapidly clears during the first few weeks of infection. A prospective assessment of the viral genome sourced from recovered non-infectious patients would greatly facilitate epidemiological tracking. Thus, we developed a protocol to isolate and sequence the genome of SARS-CoV-2 from stool samples of post-acute SARS-CoV-2 patients, at timepoints ranging from 10-120 days after onset of symptoms. Stool samples were collected from patients at varying timepoints post-convalescence, and viral DNA was isolated and sequenced using the QIAamp Viral RNA Mini Kit (Qiagen Inc.) and Ion Ampliseq™ Library Kit Plus (Life Technologies Corporation). Capacity of neutralizing antibodies in patient plasma was tested using a Luminex panel (Coronavirus Ig Total Human 11-Plex ProcartaPlex™ Panel, ThermoFisher). Of 64 samples obtained from post-acute patients, 21 (32.8%) yielded sufficient material for whole-genome sequencing. This allowed us to identify widely divergent phylogenetic relativity of the SARS-CoV-2 genome from post-acute patients living in the same households and infected around the same time. Additionally, we observed that individuals who recovered from infection expressed varying degrees of antibodies against SARS-CoV-2 structural proteins that corresponded to distinct variants. Interestingly, we identified a novel point mutation in the viral genome where infected patients expressed antibodies with a significantly reduced capacity to neutralize the virus in vitro relative to that of those infected with the wild-type strain. Altogether, we demonstrate a protocol to successfully sequence the SARS-CoV-2 genome from stool samples from patients up to 4 months post-infection, which can be applied to studies that assess the relationship between variants and immune response post-hoc and safe monitoring of the SARS-CoV-2 genome during the pandemic.
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