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首页> 外文期刊>Infection, Genetics and Evolution: Journal of Molecular Epidemiology and Evolutionary Genetics in Infectious Diseases >Molecular analysis of several in-house rRT-PCR protocols for SARS-CoV-2 detection in the context of genetic variability of the virus in Colombia
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Molecular analysis of several in-house rRT-PCR protocols for SARS-CoV-2 detection in the context of genetic variability of the virus in Colombia

机译:在哥伦比亚病毒遗传变异性范围内SARS-COV-2检测的几个内部RRT-PCR方案的分子分析

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摘要

The COVID-19 pandemic caused by SARS-CoV-2 is a public health problem unprecedented in the recent history of humanity. Different in-house real-time RT-PCR (rRT-PCR) methods for SARS-CoV-2 diagnosis and the appearance of genomes with mutations in primer regions have been reported. Hence, whole-genome data from locally-circulating SARS-CoV-2 strains contribute to the knowledge of its global variability and the development and fine tuning of diagnostic protocols. To describe the genetic variability of Colombian SARS-CoV-2 genomes in hybridization regions of oligonucleotides of the main in-house methods for SARS-CoV-2 detection, RNA samples with confirmed SARS-CoV-2 molecular diagnosis were processed through next-generation sequencing. Primers/probes sequences from 13 target regions for SARS-CoV-2 detection suggested by 7 institutions and consolidated by WHO during the early stage of the pandemic were aligned with Muscle tool to assess the genetic variability potentially affecting their performance. Finally, the corresponding codon positions at the 3' end of each primer, the open reading frame inspection was identified for each gene/protein product. Complete SARS-CoV-2 genomes were obtained from 30 COVID-19 cases, representative of the current epidemiology in the country. Mismatches between at least one Colombian sequence and five oligonucleotides targeting the RdRP and N genes were observed. The 3' end of 4 primers aligned to the third codon position, showed high risk of nucleotide substitution and potential mismatches at this critical position. Genetic variability was detected in Colombian SARS-CoV-2 sequences in some of the primer/probe regions for in-house rRT-PCR diagnostic tests available at WHO COVID-19 technical guidelines; its impact on the performance and rates of false-negative results should be experimentally evaluated. The genomic surveillance of SARS-CoV-2 is highly recommended for the early identification of mutations in critical regions and to issue recommendations on specific diagnostic tests to ensure the coverage of locally-circulating genetic variants.
机译:Covid-19由SARS-COV-2引起的大流行是在最近的人类历史中前所未有的公共卫生问题。已经报道了不同的​​内部实时RT-PCR(RRT-PCR)方法,用于SARS-COV-2诊断和具有引物区中突变的基因组的外观。因此,来自局部循环SARS-COV-2菌株的全基因组数据有助于了解其全球变异性和诊断方案的开发和微调的知识。为了描述SARS-COV-2检测的主要内部方法的寡核苷酸的寡核苷酸杂交区域中蛋白酶SARS-COV-2基因组的遗传变异,通过下一代处理具有证实SARS-COV-2分子诊断的RNA样品测序。来自7个机构的13个目标区域的引物/探针序列,由7个机构建议,并在大流行早期的世卫组织巩固的是,用肌肉工具对齐,以评估潜在影响其性能的遗传变异性。最后,对每个引物的3'末端的相应密码子位置,针对每个基因/蛋白质产品鉴定开放阅读帧检查。完整的SARS-COV-2基因组是从30个Covid-19案例获得的基因组,代表该国目前流行病学。观察到至少一种蛋白酶序列和靶向RDRP和N基因的五个寡核苷酸之间的不匹配。 4个引物的3'末端与第三密码子位置对齐,显示出高风险的核苷酸取代和在该关键位置处的潜在不匹配。在Covid-19技术指南的IN-HEAT RRT-PCR诊断测试中,在一些引物/探针区域中检测到植物变异性在植物/探针区的一些底漆/探针区域中检测到。应通过实验评估其对假阴性结果的性能和率的影响。强烈建议在关键区域中早期识别突变的基因组监测,并对特定诊断试验发出建议以确保局部循环遗传变异的突变。

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