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使用基于双引物寡核苷酸系统的多重PCR检测法快速检测和鉴定12种呼吸道病毒。

Rapid detection and identification of 12 respiratory viruses using a dual priming oligonucleotide system-based multiplex PCR assay.

作者信息

Kim Suk Ran, Ki Chang-Seok, Lee Nam Yong

机构信息

Department of Laboratory Medicine and Genetics, Samsung Medical Center, Sungkyunkwan University School of Medicine, Seoul, Republic of Korea.

出版信息

J Virol Methods. 2009 Mar;156(1-2):111-6. doi: 10.1016/j.jviromet.2008.11.007. Epub 2008 Dec 24.

Abstract

Acute viral respiratory infections are among the most common causes of human disease. Rapid and accurate diagnosis of viral respiratory infections is important for providing timely therapeutic interventions. This study evaluated a new multiplex PCR assay (Seegene Inc., Seoul, Korea) for simultaneous detection and identification of 12 respiratory viruses using two primer mixes. The viruses included parainfluenza viruses 1, 2, and 3, human metapneumovirus, human coronavirus 229E/NL63 and OC43, adenovirus, influenza viruses A and B, human respiratory syncytial viruses A and B, and human rhinovirus A. The analytical sensitivity of the assay was 10-100 copies per reaction for each type of virus. There was no cross-reactivity with common bacterial or viral pathogens. A comparison with conventional viral culture and immunofluorescence was carried out using 101 respiratory specimens from 92 patients. Using viral culture, 57 specimens (56.4%) were positive without co-infection. The same viruses were identified in all 57 specimens using the multiplex PCR. Seven of the 57 specimens (12.3%) were found to be co-infected with other respiratory viruses, and 19 of 44 (43.2%) specimens which were negative by culture were positive by the multiplex PCR. The Seeplex Respiratory Virus Detection assay represents a significant improvement over the conventional methods for the detection of a broad spectrum of respiratory viruses.

摘要

急性病毒性呼吸道感染是人类疾病最常见的病因之一。对病毒性呼吸道感染进行快速准确的诊断对于及时提供治疗干预措施至关重要。本研究评估了一种新的多重PCR检测方法(韩国首尔Seegene公司),该方法使用两种引物混合物同时检测和鉴定12种呼吸道病毒。这些病毒包括1型、2型和3型副流感病毒、人偏肺病毒、人冠状病毒229E/NL63和OC43、腺病毒、甲型和乙型流感病毒、人呼吸道合胞病毒A和B以及人鼻病毒A。该检测方法对每种病毒的分析灵敏度为每个反应10 - 100个拷贝。与常见的细菌或病毒病原体无交叉反应。使用来自92例患者的101份呼吸道标本与传统病毒培养和免疫荧光法进行了比较。采用病毒培养法,57份标本(56.4%)呈阳性,无合并感染。使用多重PCR在所有57份标本中鉴定出相同病毒。57份标本中有7份(12.3%)被发现与其他呼吸道病毒合并感染,44份培养阴性的标本中有19份(43.2%)经多重PCR检测呈阳性。Seeplex呼吸道病毒检测法在检测多种呼吸道病毒方面比传统方法有显著改进。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c889/7112863/57e8fbf5f8d2/gr1.jpg

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