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Detection of 12 respiratory viruses by duplex real time PCR assays in respiratory samples

机译:通过双重实时PCR检测呼吸道样品中的12种呼吸道病毒

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Different viruses can be responsible for similar clinical manifestations of respiratory infections. Thus, the etiological diagnosis of respiratory viral diseases requires the detection of a large number of viruses. In this study, 6 duplex real-time PCR assays, using EvaGreen intercalating dye, were developed to detect 12 major viruses responsible for respiratory diseases: influenza A and B viruses, enteroviruses (including enterovirus spp, and rhinovirus spp), respiratory syncytial virus, human metapneumovirus, coronaviruses group I (of which CoV 229E and CoV NL63 are part) and II (including Coy OC43 and CoV HKU1), parainfluenza viruses type 1, 2, 3 and 4, human adenoviruses and human bocaviruses. The 2 target viruses of each duplex reaction were distinguishable by the melting temperatures of their amplicons. The 6 duplex real time PCR assays were applied for diagnostic purpose on 202 respiratory samples from 157 patients. One hundred fifty-seven samples were throat swabs and 45 were bronchoalveolar lavages. The results of the duplex PCR assays were confirmed by comparison with a commercial, validated, assay; in addition, the positive results were confirmed by sequencing. The analytical sensitivity of the duplex PCR assays varied from 10(3) copies/ml to 10(4) copies/ml. For parainfluenza virus 2 only it was 10(5) copies/ml. Seventy clinical samples (35%) from 55 patients (30 children and 25 adults) were positive for 1 or more viruses. In adult patients, influenza A virus was the most frequently detected respiratory virus followed by rhinoviruses. In contrast, respiratory syncytial virus was the most common virus in children, followed by enteroviruses, influenza A virus and coronavirus NL63. The small number of samples/patients does not allow us to draw any epidemiological conclusion. Altogether, the results of this study indicate that the 6 duplex PCR assays described in this study are sensitive, specific and cost-effective. Thus, this assay could be particularly useful to identify the main respiratory viruses directly from clinical samples, after nucleic acid extraction, and, also, to screen a large number of patients for epidemiological studies. (C) 2015 Elsevier Ltd. All rights reserved.
机译:不同的病毒可能导致呼吸道感染的相似临床表现。因此,呼吸道病毒性疾病的病因学诊断需要检测大量病毒。在这项研究中,使用EvaGreen嵌入染料开发了6种双工实时PCR检测方法,以检测与呼吸道疾病有关的12种主要病毒:甲型和乙型流感病毒,肠病毒(包括肠病毒和鼻病毒),呼吸道合胞病毒,人偏肺病毒,I型冠状病毒(其中CoV 229E和CoV NL63是一部分)和II型(包括Coy OC43和CoV HKU1),1型,2型,3型和4型副流感病毒,人腺病毒和人博卡病毒。每个双链反应的2种靶病毒可以通过其扩增子的解链温度来区分。对来自157位患者的202份呼吸道样品进行了6次双工实时PCR分析,以用于诊断。 157份样品为咽拭子,45份为支气管肺泡灌洗液。通过与商业验证过的测定法进行比较,证实了双重PCR测定法的结果。此外,通过测序证实了阳性结果。双重PCR检测的分析灵敏度从10(3)拷贝/ ml到10(4)拷贝/ ml不等。仅对于副流感病毒2,它是10(5)拷贝/ ml。 55名患者(30名儿童和25名成人)的70份临床样本(35%)对一种或多种病毒呈阳性反应。在成年患者中,甲型流感病毒是最常见的呼吸道病毒,其次是鼻病毒。相反,呼吸道合胞病毒是儿童中最常见的病毒,其次是肠病毒,甲型流感病毒和冠状病毒NL63。少量的样本/患者不允许我们得出任何流行病学结论。总体而言,这项研究的结果表明,该研究中描述的6种双链PCR检测方法灵敏,特异且具有成本效益。因此,该试验在核酸提取后直接从临床样品中鉴定出主要的呼吸道病毒以及筛选大量的患者进行流行病学研究特别有用。 (C)2015 Elsevier Ltd.保留所有权利。

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