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Characterisation of a newly identified human rhinovirus, HRV-QPM, discovered in infants with bronchiolitis.在患有细支气管炎的婴儿中发现的一种新鉴定的人鼻病毒HRV-QPM的特征描述。
J Clin Virol. 2007 Jun;39(2):67-75. doi: 10.1016/j.jcv.2007.03.012. Epub 2007 May 7.
2
Comparison of results of detection of rhinovirus by PCR and viral culture in human nasal wash specimens from subjects with and without clinical symptoms of respiratory illness.对有和没有呼吸道疾病临床症状的受试者的人鼻腔冲洗液标本中,采用聚合酶链反应(PCR)和病毒培养法检测鼻病毒的结果进行比较。
J Clin Microbiol. 2007 Jul;45(7):2126-9. doi: 10.1128/JCM.02553-06. Epub 2007 May 2.
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Rhinovirus-associated hospitalizations in young children.幼儿中与鼻病毒相关的住院情况。
J Infect Dis. 2007 Mar 15;195(6):773-81. doi: 10.1086/511821. Epub 2007 Feb 2.
4
Prevalence of viral respiratory tract infections in children with asthma.哮喘患儿中病毒性呼吸道感染的患病率。
J Allergy Clin Immunol. 2007 Feb;119(2):314-21. doi: 10.1016/j.jaci.2006.08.041. Epub 2006 Nov 30.
5
MassTag polymerase-chain-reaction detection of respiratory pathogens, including a new rhinovirus genotype, that caused influenza-like illness in New York State during 2004-2005.2004 - 2005年期间在纽约州引起流感样疾病的呼吸道病原体(包括一种新型鼻病毒基因型)的MassTag聚合酶链反应检测
J Infect Dis. 2006 Nov 15;194(10):1398-402. doi: 10.1086/508551. Epub 2006 Oct 6.
6
Chronic rhinoviral infection in lung transplant recipients.肺移植受者的慢性鼻病毒感染
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Two outbreaks of severe respiratory disease in nursing homes associated with rhinovirus.养老院中两起与鼻病毒相关的严重呼吸道疾病暴发。
J Am Geriatr Soc. 2006 Feb;54(2):284-9. doi: 10.1111/j.1532-5415.2005.00529.x.
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Detection of rhinoviruses by tissue culture and two independent amplification techniques, nucleic acid sequence-based amplification and reverse transcription-PCR, in children with acute respiratory infections during a winter season.在一个冬季,采用组织培养以及两种独立的扩增技术——基于核酸序列的扩增技术和逆转录-聚合酶链反应,对患有急性呼吸道感染的儿童进行鼻病毒检测。
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10
The role of rhinovirus in asthma exacerbations.鼻病毒在哮喘急性加重中的作用。
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用于全面检测人鼻病毒的实时逆转录-聚合酶链反应检测法

Real-time reverse transcription-PCR assay for comprehensive detection of human rhinoviruses.

作者信息

Lu Xiaoyan, Holloway Brian, Dare Ryan K, Kuypers Jane, Yagi Shigeo, Williams John V, Hall Caroline B, Erdman Dean D

机构信息

Gastroenteritis and Respiratory Virus Laboratory Branch, Division of Viral Diseases, Centers for Disease Control and Prevention, Atlanta, Georgia, USA.

出版信息

J Clin Microbiol. 2008 Feb;46(2):533-9. doi: 10.1128/JCM.01739-07. Epub 2007 Dec 5.

DOI:10.1128/JCM.01739-07
PMID:18057136
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2238069/
Abstract

Human rhinoviruses (HRVs) are important contributors to respiratory disease, but their healthcare burden remains unclear, primarily because of the lack of sensitive, accurate, and convenient means of determining their causal role. To address this, we developed and clinically validated the sensitivity and specificity of a real-time reverse transcription-PCR (RT-PCR) assay targeting the viral 5' noncoding region defined by sequences obtained from all 100 currently recognized HRV prototype strains and 85 recently circulating field isolates. The assay successfully amplified all HRVs tested and could reproducibly detect 50 HRV RNA transcript copies, with a dynamic range of over 7 logs. In contrast, a quantified RNA transcript of human enterovirus 68 (HEV68) that showed the greatest sequence homology to the HRV primers and probe set was not detected below a concentration of 5 x 10(5) copies per reaction. Nucleic acid extracts of 111 coded respiratory specimens that were culture positive for HRV or HEV were tested with the HRV real-time RT-PCR assay and by two independent laboratories that used different in-house HRV/HEV RT-PCR assays. Eighty-seven HRV-culture-positive specimens were correctly identified by the real-time RT-PCR assay, and 4 of the 24 HEV-positive samples were positive for HRV. HRV-specific sequences subsequently were identified in these four specimens, suggesting HRV/HEV coinfection in these patients. The assay was successfully applied in an investigation of a coincidental outbreak of HRV respiratory illness among laboratory staff.

摘要

人鼻病毒(HRV)是导致呼吸道疾病的重要因素,但其对医疗保健的负担仍不明确,主要原因是缺乏灵敏、准确且便捷的手段来确定其致病作用。为解决这一问题,我们开发并在临床上验证了一种针对病毒5'非编码区的实时逆转录聚合酶链反应(RT-PCR)检测方法的敏感性和特异性,该区域由从目前所有100种公认的HRV原型株以及85种近期流行的现场分离株获得的序列所定义。该检测方法成功扩增了所有测试的HRV,并且能够重复检测到50个HRV RNA转录本拷贝,动态范围超过7个对数。相比之下,与HRV引物和探针组序列同源性最高的人肠道病毒68型(HEV68)的定量RNA转录本,在每个反应低于5×10⁵拷贝的浓度时未被检测到。对111份编码的呼吸道标本的核酸提取物进行了检测,这些标本经培养为HRV或HEV阳性,采用HRV实时RT-PCR检测方法,并由两个独立实验室使用不同的内部HRV/HEV RT-PCR检测方法进行检测。实时RT-PCR检测方法正确鉴定出87份HRV培养阳性标本,24份HEV阳性样本中有4份为HRV阳性。随后在这4份标本中鉴定出HRV特异性序列,提示这些患者存在HRV/HEV合并感染。该检测方法成功应用于对实验室工作人员中HRV呼吸道疾病同时爆发的调查。