定制多重实时逆转录聚合酶链反应与快速诊断呼吸道21种病原体检测试剂盒在检测多种呼吸道病毒方面的比较评估。
Evaluation of custom multiplex real - time RT - PCR in comparison to fast - track diagnostics respiratory 21 pathogens kit for detection of multiple respiratory viruses.
作者信息
Malhotra Bharti, Swamy M Anjaneya, Reddy P V Janardhan, Kumar Neeraj, Tiwari Jitendra Kumar
机构信息
Department of Microbiology & Immunology, Advanced Basic Sciences & Clinical Research Laboratory, (ICMR Grade - I Viral Diagnostics & Research Laboratory), Sawai Man Singh Medical College, Jawahar Lal Nehru Marg, Jaipur, 302 004, India.
出版信息
Virol J. 2016 Jun 6;13:91. doi: 10.1186/s12985-016-0549-8.
BACKGROUND
Severe acute respiratory infections in children can be fatal, rapid identification of the causative agent and timely treatment can be life saving. Multiplex real time RT-PCR helps in simultaneous detection of multiple viruses saving cost, time and labour. Commercially available multiplex real time RT-PCR kits are very expensive. Therefore the aim of the present study was to develop a cost effective multiplex real time RT-PCR for the detection of 18 respiratory viruses and compare it with an in-vitro diagnostics approved Fast Track Diagnostic Respiratory Pathogens 21 Kit (FTD).
METHODS
Nasopharyngeal aspirates and throat swabs were collected and processed for extraction of nucleic acid using an automated extraction system and multiplex real time RT-PCR was performed using the FTD kit and a custom assay on 356 samples.
RESULTS
Custom and FTD assays detected one or more respiratory viruses in 268 (75.29 %) and 262 (73.60 %) samples respectively. The concordance between the custom assay and the FTD assay was 100 % for HCoV OC43, HCoV 229E, HPIV-1, HPIV-2, HBoV, HPeV, Flu A, and Influenza A(H1N1)pdm09 and 94.66 - 99.71 % for the remaining viruses; Flu B (99.71 %), HRV (99.71 %), HPIV-3 (98.87 %), HPIV-4 (99.43 %), HCoV NL63 (99.71 %), HMPV A/B (99.71 %), RSV A/B (94.66 %), EV (98.31 %), HCoV HKU1 (99.71 %), HAdV (99.71 %). Major discrepancy was observed for RSV A/B, which was over detected in 18 samples by the custom assay as compared to the FTD assay. The custom assay was much cheaper than the FTD assay and the time taken was only 29 min more.
CONCLUSION
The custom primer and probe mix was found to be comparable to the FTD assay with good concordance but was much cheaper and the time taken for reporting was only 29 min more. The low cost custom multiplex RT-PCR can be a useful alternative to the costly FTD kit for rapid identification of viral aetiology in resource limited settings.
背景
儿童严重急性呼吸道感染可能致命,快速识别病原体并及时治疗可挽救生命。多重实时逆转录聚合酶链反应(RT-PCR)有助于同时检测多种病毒,节省成本、时间和人力。市售的多重实时RT-PCR试剂盒非常昂贵。因此,本研究的目的是开发一种经济高效的多重实时RT-PCR方法,用于检测18种呼吸道病毒,并将其与体外诊断批准的快速通道诊断呼吸道病原体21试剂盒(FTD)进行比较。
方法
收集鼻咽抽吸物和咽拭子,使用自动提取系统进行核酸提取,并使用FTD试剂盒和定制检测方法对356份样本进行多重实时RT-PCR。
结果
定制检测方法和FTD检测方法分别在268份(75.29%)和262份(73.60%)样本中检测到一种或多种呼吸道病毒。对于人冠状病毒OC43、人冠状病毒229E、人副流感病毒1型、人副流感病毒2型、人博卡病毒、人细小病毒、甲型流感病毒和甲型H1N1流感大流行病毒,定制检测方法与FTD检测方法的一致性为100%,对于其余病毒,一致性为94.66% - 99.71%;乙型流感病毒(99.71%)、人鼻病毒(99.71%)、人副流感病毒3型(98.87%)、人副流感病毒4型(99.43%)、人冠状病毒NL63(99.71%)、人偏肺病毒A/B(99.71%)呼吸道合胞病毒A/B(94.66%)、肠道病毒(98.31%)、人冠状病毒HKU1(99.71%)、人腺病毒(99.71%)。观察到呼吸道合胞病毒A/B存在主要差异,与FTD检测方法相比,定制检测方法在18份样本中检测到的该病毒数量过多。定制检测方法比FTD检测方法便宜得多,且报告时间仅多29分钟。
结论
发现定制引物和探针混合物与FTD检测方法具有可比性,一致性良好,但成本低得多,报告时间仅多29分钟。低成本的定制多重RT-PCR可为资源有限环境中快速鉴定病毒病因的昂贵FTD试剂盒提供有用的替代方案。
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