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从鼻咽拭子中富集严重急性呼吸综合征冠状病毒2(SARS-CoV-2)序列,同时鉴定鼻腔微生物群。

Enrichment of SARS-CoV-2 sequence from nasopharyngeal swabs whilst identifying the nasal microbiome.

作者信息

Alrezaihi Abdulrahman, Penrice-Randal Rebekah, Dong Xiaofeng, Prince Tessa, Randle Nadine, Semple Malcolm G, Openshaw Peter J M, MacGill Tracy, Myers Todd, Orr Robert, Zakotnik Samo, Suljič Alen, Avšič-Županc Tatjana, Petrovec Miroslav, Korva Miša, AlJabr Waleed, Hiscox Julian A

机构信息

University of Liverpool, Liverpool, UK; King Saud University, Riyadh, Saudi Arabia.

University of Liverpool, Liverpool, UK.

出版信息

J Clin Virol. 2024 Apr;171:105620. doi: 10.1016/j.jcv.2023.105620. Epub 2023 Nov 25.

Abstract

Simultaneously characterising the genomic information of coronaviruses and the underlying nasal microbiome from a single clinical sample would help characterise infection and disease. Metatranscriptomic approaches can be used to sequence SARS-CoV-2 (and other coronaviruses) and identify mRNAs associated with active transcription in the nasal microbiome. However, given the large sequence background, unenriched metatranscriptomic approaches often do not sequence SARS-CoV-2 to sufficient read and coverage depth to obtain a consensus genome, especially with moderate and low viral loads from clinical samples. In this study, various enrichment methods were assessed to detect SARS-CoV-2, identify lineages and define the nasal microbiome. The methods were underpinned by Oxford Nanopore long-read sequencing and variations of sequence independent single primer amplification (SISPA). The utility of the method(s) was also validated on samples from patients infected seasonal coronaviruses. The feasibility of profiling the nasal microbiome using these enrichment methods was explored. The findings shed light on the performance of different enrichment strategies and their applicability in characterising the composition of the nasal microbiome.

摘要

同时对来自单个临床样本的冠状病毒基因组信息和潜在的鼻腔微生物群进行表征,将有助于对感染和疾病进行表征。宏转录组学方法可用于对严重急性呼吸综合征冠状病毒2(SARS-CoV-2)(以及其他冠状病毒)进行测序,并识别与鼻腔微生物群中活跃转录相关的信使核糖核酸(mRNA)。然而,鉴于庞大的序列背景,未富集的宏转录组学方法通常无法对SARS-CoV-2进行足够的读数和覆盖深度测序以获得一致基因组,尤其是对于临床样本中病毒载量中等和较低的情况。在本研究中,评估了各种富集方法以检测SARS-CoV-2、识别谱系并定义鼻腔微生物群。这些方法以牛津纳米孔长读长测序和序列独立单引物扩增(SISPA)的变体为基础。该方法的实用性也在感染季节性冠状病毒患者的样本上得到了验证。探索了使用这些富集方法对鼻腔微生物群进行分析的可行性。这些发现揭示了不同富集策略的性能及其在表征鼻腔微生物群组成方面的适用性。

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