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[2003年至2008年北京地区急性呼吸道感染患儿腺病毒的鉴定与分型]

[Identification and typing of adenoviruses from pediatric patients with acute respiratory infections in Beijing from 2003 to 2008].

作者信息

Deng Jie, Qian Yuan, Zhao Lin-qing, Zhu Ru-nan, Wang Fang, Sun Yu, Liao Bin, Huang Rong-yan, Yuan Yi, Qu Dong, Ren Xiao-xu

机构信息

Laboratory of Virology, Beijing Municipal Laboratory of Infection and Immunity, Capital Institute of Pediatrics, Beijing, 100020, China.

出版信息

Zhonghua Er Ke Za Zhi. 2010 Oct;48(10):739-43.

PMID:21176480
Abstract

OBJECTIVE

Adenovirus (ADV) is one of the most common causes of acute respiratory infections in infants and children. The objective of this study was to investigate the prevalence of adenovirus infection among pediatric patients with acute respiratory infections in Beijing and the types of the adenoviruses circulating in Beijing on the molecular bases.

METHOD

Clinical specimens including throat swabs from outpatients and nasopharyngeal aspirates from hospitalized patients were collected from patients with acute respiratory infections in a consecutive period of 6 years from Jan 2003 to Dec 2008. Adenoviruses were identified from the collected clinical specimens by tissue culture and/or immunofluorescence assay and typed by nested-PCR based on the sequence of the encoding gene of hexon. Primers were designed for PCR amplification using hexon gene of adenovirus as target. One primer pair was designed as universal primers for amplifying a 1278 bp gene fragment located at the hexon gene of adenovirus types 3, 7, 11 and 21. Four primer pairs with the sequences located within the region of this 1278 bp fragment were designed specifically for amplifying adenoviruses types 3, 7, 11 or 21, respectively, which were used for a multiplex nest-PCR in a single tube. The products from this multiplex nest-PCR were 502 bp (for type 3), 311 bp (for type 7), 880 bp (for type 11) and 237 bp (for type 21), respectively, and the type of the adenovirus tested can be determined after agarose electrophoresis analysis of the PCR products. For those strains which could not be typed by the multiplex nest-PCR, the gene fragment was amplified by a universal primer pair for all adenovirus types from group A to F and the PCR products were sequenced directly.

RESULT

Out of 17 941 clinical specimens collected, including 4378 throat swabs from outpatients and 13 563 nasopharyngeal aspirates from hospitalized patients, 304 were adenovirus positive by tissue culture and/or immunofluorescence assay, the overall positive rate was 1.69% (304/179 41). Among these 304 adenovirus positive specimens, 184 were by virus isolation and 184 by immunofluorescence assay, among which 64 were positive by both methods. The types of the adenoviruses were tested for 285 patients including 174 viral isolates and 111 clinical specimens. By using the multiplex nest-PCR, 272 were typable, including 174 (61.1%, 174/285) for ADV3, 92 (32.3%, 92/285) for ADV7, 6 for ADV11 (2.1%, 6/285) and no adenovirus type 21 was detected. Sequence analysis for those 13 nontypable specimens by the multiplex nest-PCR showed that 9 were ADV2 (3.2%, 9/285), 2 were ADV6 (0.7%, 2/285), 1 was ADV1 (0.4%, 1/285) and 1 was ADV5 (0.4%, 1/285). Most of the patients positive for adenovirus were under 5 years of age and 64.4% were from patients with lower respiratory infections, such as bronchiolitis and pneumonia. All the 5 cases of severe pneumonia with pulmonary failure were caused by ADV7 infection.

CONCLUSION

Adenovirus is still an important pathogen for acute respiratory infection in infants and young children and most of the adenoviruses associated with acute respiratory infections in children in Beijing from 2003 to 2008 were ADV3 and ADV7. ADV7 could cause severe lower respiratory infections.

摘要

目的

腺病毒(ADV)是婴幼儿急性呼吸道感染最常见的病因之一。本研究旨在调查北京地区急性呼吸道感染儿科患者中腺病毒感染的流行情况以及北京地区流行的腺病毒分子类型。

方法

收集2003年1月至2008年12月连续6年期间急性呼吸道感染患者的临床标本,包括门诊患者的咽拭子和住院患者的鼻咽抽吸物。通过组织培养和/或免疫荧光法从收集的临床标本中鉴定腺病毒,并根据六邻体编码基因序列通过巢式PCR进行分型。以腺病毒六邻体基因作为靶标设计引物进行PCR扩增。设计一对通用引物用于扩增位于3、7、11和21型腺病毒六邻体基因的1278 bp基因片段。另外设计四对引物,其序列位于该1278 bp片段区域内,分别用于特异性扩增3、7、11或21型腺病毒,用于单管多重巢式PCR。该多重巢式PCR产物分别为502 bp(3型)、311 bp(7型)、880 bp(11型)和237 bp(21型),对PCR产物进行琼脂糖电泳分析后可确定所检测腺病毒的类型。对于那些不能通过多重巢式PCR分型的菌株,用一对针对A至F组所有腺病毒类型的通用引物扩增基因片段,并对PCR产物直接测序。

结果

在收集的17941份临床标本中,包括4378份门诊患者咽拭子和13563份住院患者鼻咽抽吸物,通过组织培养和/或免疫荧光法检测出304份腺病毒阳性,总体阳性率为1.69%(304/17941)。在这304份腺病毒阳性标本中,病毒分离阳性184份,免疫荧光法阳性184份,其中两种方法均阳性64份。对285例患者的腺病毒进行分型检测,包括174份病毒分离株和111份临床标本。采用多重巢式PCR,272份可分型,其中3型腺病毒174份(61.1%,174/285),7型腺病毒92份(32.3%,92/285),11型腺病毒6份(2.1%,6/285),未检测到21型腺病毒。对多重巢式PCR不能分型的13份标本进行序列分析,结果显示9份为2型腺病毒(3.2%,9/285),2份为6型腺病毒(0.7%,2/285),1份为1型腺病毒(0.4%,1/285),1份为5型腺病毒(0.4%,1/285)。大多数腺病毒阳性患者年龄在5岁以下,64.4%来自下呼吸道感染患者,如细支气管炎和肺炎。所有5例伴有呼吸衰竭的重症肺炎均由7型腺病毒感染引起。

结论

腺病毒仍是婴幼儿急性呼吸道感染的重要病原体,2003年至2008年北京地区儿童急性呼吸道感染相关的腺病毒大多为3型和7型。7型腺病毒可引起严重的下呼吸道感染。

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