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Highly multiplexed oligonucleotide probe-ligation testing enables efficient extraction-free SARS-CoV-2 detection and viral genotyping

机译:高度复用寡核苷酸探针连接测试能够有效的无萃取SARS-COV-2检测和病毒基因分型

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There is an urgent and unprecedented need for sensitive and high-throughput molecular diagnostic tests to combat the SARS-CoV-2 pandemic. Here we present a generalized version of the RNA-mediated oligonucleotide Annealing Selection and Ligation with next generation DNA sequencing (RASL-seq) assay, called "capture RASL-seq" (cRASL-seq), which enables highly sensitive (down to ~1-100 pfu/ml or cfu/ml) and highly multiplexed (up to ~10,000 target sequences) detection of pathogens. Importantly, cRASL-seq analysis of COVID-19 patient nasopharyngeal (NP) swab specimens does not involve nucleic acid purification or reverse transcription, steps that have introduced supply bottlenecks into standard assay workflows. Our simplified protocol additionally enables the direct and efficient genotyping of selected, informative SARS-CoV-2 polymorphisms across the entire genome, which can be used for enhanced characterization of transmission chains at population scale and detection of viral clades with higher or lower virulence. Given its extremely low per-sample cost, simple and automatable protocol and analytics, probe panel modularity, and massive scalability, we propose that cRASL-seq testing is a powerful new technology with the potential to help mitigate the current pandemic and prevent similar public health crises.
机译:对抗SARS-COV-2流行的敏感和高通量的分子诊断测试急需和前所未有的需求。在这里,我们介绍了RNA介导的寡核苷酸退火选择和用下一代DNA测序(RASL-SEQ)测定的连接,称为“捕获RASL-SEQ”(CRASL-SEQ),这使得能够高度敏感(下降至〜1 -100 pfu / ml或cfu / ml)和高度复用(高达约10,000个靶序列)检测病原体。重要的是,Covid-19患者鼻咽(NP)棉签(NP)棉签样本的Crasl-SEQ分析不涉及核酸纯化或逆转录,将供应瓶颈引入标准测定工作流程的步骤。我们的简化方案另外,在整个基因组上还可以直接和有效的基因分型,其在整个基因组上,可用于增强人口规模的传输链的表征,并检测具有更高或更低的毒力的病毒型湿度。鉴于其单样本极低,简单可自动的协议和分析,探头面板模块化和巨大可扩展性,我们提出了克拉斯赛-SEQ测试是一种强大的新技术,有可能帮助减轻目前大流行并防止类似的公共卫生危机。

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