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Comparative Analysis of Molecular Methods for Detection of Influenza Viruses

机译:甲型流感病毒检测分子方法的比较分析

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Aims:?Influenza is a serious threat to human population worldwide therefore continuous surveillance is required to update influenza seasonal vaccines. A rapid, sensitive, specific and cost effective diagnostic method will be much helpful for patient management in the present scenario. Present study is conceptualized for detection of influenza viruses by molecular methods and compare with ‘gold standard’ virus isolation.???Study Design:?Standard strains of Influenza virus were used to standardize the molecular diagnostic assays and results were then compared with virus isolation.Place and Duration of Study:?Centre for Biotechnology, Maharshi Dayanand University, Rohtak, Haryana, India, between December 2015 and April 2016.Methodology:?Standard strains of Influenza A and B virus were used for influenza virus isolation using virus culturing in MDCK (Madin-Darby Canine Kidney) cell line by following standard tissue culture procedure. Isolated viruses were detected by Hemagglutination assay (HA) and typed by Hemagglutination inhibition assay (HI). Conventional one step RT-PCR, Taqman real time RT-PCR and RT-LAMP (Reverse transcription loop mediated isothermal amplification) were standardized on RNA extracted from standard strains. Sensitivity and specificity of these molecular methods were compared with each other as well as with virus culture (gold standard).Results:?Both influenza A and B virus strains were cultured in MDCK cells and produced cytopathic effect during virus culture. Conventional RT-PCR and real time RT-PCR detected both type of Influenza viruses. RT-LAMP also successfully detected and typed influenza viruses. RT-LAMP proved to be more rapid than other two molecular assays.??Conclusion:?Molecular diagnostic methods are useful in detection and typing of Influenza viruses and these methods provide results in short period of time when compared with traditional virus culture methods. RT-LAMP is rapid, sensitive, specific and cost effective method for influenza virus detection and subtyping.
机译:目的:?流感对全世界的人口严重威胁,因此需要连续监测来更新流感季节性疫苗。快速,敏感,特异性和成本效益的诊断方法对本场景中的患者管理有很大的帮助。目前的研究是通过分子方法检测流感病毒的概念化,并与“黄金标准”病毒隔离进行比较。??Sutudy设计:?使用甲型病毒的标准菌株标准化分子诊断测定和结果与病毒分离进行比较.Place和持续时间:?生物技术中心,Maharshi Dayanand大学,Rohtak,印度,2015年12月至2016年12月间。方法:?使用病毒培养的病毒分离用于流感病毒分离的标准菌株MDCK(Madin-Darby Canine肾脏)细胞系通过以下标准组织培养程序。通过血凝测定(HA)检测分离的病毒,并通过血凝集抑制测定法(HI)键入。常规的一步RT-PCR,Taqman实时RT-PCR和RT灯(逆转录环介导的等温扩增)在标准菌株中提取的RNA上标准化。将这些分子方法的敏感性和特异性彼此进行比较,以及病毒培养(金标准)。结果:α和B病毒株在MDCK细胞中培养,并在病毒培养过程中产生了细胞病变作用。常规RT-PCR和实时RT-PCR检测到两种类型的流感病毒。 RT-LAMP还成功地检测到和类型的流感病毒。 RT-LAMP被证明比其他两个分子测定更快。结论:多分子诊断方法可用于检测和键入流感病毒,与传统病毒培养方法相比,这些方法在短时间内提供结果。 RT-LAMP是流感病毒检测和亚型的快速,敏感,具体和成本效益的方法。

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