| 西藏地区儿童急性呼吸道感染中呼吸道合胞病毒的初步研究 |
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| 引用本文: | Deng J,Zhu RN,Qian Y,Sun Y,Zhao LQ,Wang F,Wu H,Shan MN,Deji MD. 西藏地区儿童急性呼吸道感染中呼吸道合胞病毒的初步研究[J]. 病毒学报, 2012, 28(2): 97-102 |
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| 作者姓名: | Deng J Zhu RN Qian Y Sun Y Zhao LQ Wang F Wu H Shan MN Deji MD |
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| 作者单位: | 首都儿科研究所病毒研究室北京市感染与免疫中心实验室;西藏自治区人民医院儿科 |
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| 基金项目: | 国家自然基金项目(30872153) |
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| 摘 要: | 本研究为了解西藏地区儿童急性呼吸道感染中呼吸道合胞病毒(Respiratory syncytial virus,RSV)及基因型别。首先采用直接免疫荧光法检测2011年4~7月西藏自治区人民医院儿科病房因急性呼吸道感染住院患儿的鼻咽分泌物标本中7种常见的呼吸道病毒及人类偏肺病毒(Human metapneumovirus,hMPV)的抗原。然后对RSV抗原阳性的标本分别提取RNA,用逆转录-巢式聚合酶链反应法(Nest-PCR)确定RSV型别,同时用实时荧光PCR(Real-Time PCR)方法进行验证。再通过对G蛋白基因PCR扩增产物序列测定确定RSV的基因型。通过与GenBank中不同地区RSV分离株的G蛋白基因序列比对,了解西藏地区RSV G蛋白的结构特点及变异情况。结果表明,从167例标本中检测出呼吸道病毒抗原阳性的为65例,总阳性率为38.9%(65/167),其中RSV 45例,占阳性标本的69.2%(45/65),对其中42例RSV阳性标本进行了PCR分型,其中40例为A亚型,2例为B亚型。对7株A亚型RSV G蛋白基因PCR产物测序结果显示,全部为GA2基因型。西藏RSV与RSV原型株A2株核苷酸的同源性为90.7%~91.8%,氨基酸的同源性只有86.5%~87.2%。氨基酸的变异主要集中在胞外区一个高度保守序列的两端。7株西藏A亚型RSV G蛋白的核苷酸序列与GenBank中不同的RSV分离株相比同源性为90.7%~91.8%。西藏地区2011年春季小儿急性呼吸道感染的病毒病原主要为呼吸道合胞病毒,A亚型是2011年西藏地区的流行优势型别,其G蛋白胞外区基因具有较高的变异性。
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| 关 键 词: | 西藏地区 儿童 急性呼吸道感染 呼吸道合胞病毒 基因型 |
Preliminary analysis on respiratory syncytial virus identified in children with acute respiratory infections in Tibet Autonomous Region, China |
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| Deng Jie,Zhu Ru-Nan,Qian Yuan,Sun Yu,Zhao Lin-Qing,Wang Fang,Wu Hong,Shan Min-Na,Deji Mei-Duo. Preliminary analysis on respiratory syncytial virus identified in children with acute respiratory infections in Tibet Autonomous Region, China[J]. Chinese journal of virology, 2012, 28(2): 97-102 |
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| Authors: | Deng Jie Zhu Ru-Nan Qian Yuan Sun Yu Zhao Lin-Qing Wang Fang Wu Hong Shan Min-Na Deji Mei-Duo |
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| Affiliation: | Laboratory of Virology, Beijing Municipal Laboratory of Infection and Immunity, Capital Institute of Pediatrics, Beijing 100020, China. jie_deng@sina.com |
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| Abstract: | To understand the role of respiratory syncytial virus (RSV) in children with acute respiratory infections (ARI) in Tibet Autonomous Region and the contribution of two major groups of RSV, nasopharyngeal aspirates (NPA) were collected from hospitalized children with ARI in Department of Pediatrics, Tibet People's Hospital in Lasa, Tibet from April to July in 2011 and tested for seven common respiratory viruses and human metapneumovirus (hMPV) by direct immunofluorescence assay (DFA). Total RNAs were extracted from RSV positive samples by DFA and reverse transcripted to cDNA. Nested-PCR was employed to determine the genogroups of RSV, which were confirmed by real time-PCR and sequence analysis for G protein encoding gene. The Characteristics and variations of G genes from RSV in this project were identified by sequence comparison with those G genes in GenBank. Out of 167 samples, 65 were positive for respiratory viruses with a total positive rate of 38.9%, including 45 (69.2%, 45/65)positive samples for RSV. Among 42 samples that were positive for RSV and genotyped, 40 were identified as group A and 2 as group B. Sequence analysis of full-length G genes for 7 RSV of group A indicated that all of these belonged to subgroup GA2. The nucleotide identities between RSVs from Tibet and prototype A2 strain were 90.7%-91.8%, with 86.5%-87.2% identities of amino acid. The mutations of amino acids were mainly located in both ends of a highly conserved region in the ectodomain of the G proteins. The data indicated that RSV was the most important viral etiologic agent of ARI in spring of 2011 in Tibet and group A of RSV was predominant during the study period. High divergence existed in the ectodomain of G proteins of RSVs from Tibet. |
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| Keywords: | Respiratory syncytial virus Acute respiratory infection Tibet Children Genotype |
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