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| 利用单基因组扩增法对马传染性贫血病毒疫苗株异质性的分析 | |
| 引用本文: | 韦华冕,王雪峰,王珊珊,杜承,刘海芳,刘强,周建华. 利用单基因组扩增法对马传染性贫血病毒疫苗株异质性的分析[J]. 病毒学报, 2012, 28(4): 431-438 |
| 作者姓名: | 韦华冕 王雪峰 王珊珊 杜承 刘海芳 刘强 周建华 |
| 作者单位: | 中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001;中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001;中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001;中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001;中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001;中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001;中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室,哈尔滨,150001 |
| 基金项目: | 国家自然科学基金面上项目(31070809);“十二五”科技重大专项(2012ZX10001-008) |
| 摘 要: | 前期研究发现,马传染性贫血病毒(Equine infectious anemia virus EIAV)中国弱毒疫苗株并非单一病毒,而是由多种准种(quasispecies)组成的种群。阐明该疫苗株的具体构成,对于确定优势疫苗株和分析其在体内的进化具有重要意义。本研究比较了传统RNA病毒测序法(即bulk PCR)和单基因组扩增法(Single-genome Amplification, SGA)在扩增EIAV疫苗株囊膜表面蛋白gp90基因 V3~V5区序列上的差异。结果发现,利用SGA法和bulk PCR法获得的序列在组内差异率分别为1.84%和1.88%。进一步序列比较发现,SGA法扩增的序列中除了含有与bulk PCR法中同源性较高的序列外,还存在bulk PCR法未检出的含强毒株LN40特异性位点,以及单个氨基酸缺失的序列。上述序列的存在为该疫苗株“多克隆构成”假说提供了佐证。此外,在对抽样偏差分析中发现,由于疫苗株中各种病毒准种在量上的差异,使得传统bulk PCR法不能有效的扩增组成比例较低的病毒准种,而导致测得的序列组成不能完全代表实际情况。SGA法通过对单基因组分的扩增和测序,可避免bulk PCR法的以上缺陷,在分析以准种形式存在的RNA病毒序列方面具有独特的优势。 |
| 关 键 词: | 单基因组扩增 Bulk PCR 马传染性贫血病毒 多样性 |
The Application of Single-genome Amplification and Sequencing in Genomic Analysis of An Attenuated EIAV Vaccine |
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| WEI Hua-mian,WANG Xue-feng,WANG Shan-shan,DU Cheng, LIU Hai-fang,LIU Qiang,ZHOU Jian-hua. The Application of Single-genome Amplification and Sequencing in Genomic Analysis of An Attenuated EIAV Vaccine[J]. Chinese journal of virology, 2012, 28(4): 431-438 | |
| Authors: | WEI Hua-mian WANG Xue-feng WANG Shan-shan DU Cheng LIU Hai-fang LIU Qiang ZHOU Jian-hua |
| Affiliation: | (State Key Laboratory of Veterinary Biotechnology,Harbin Veterinary Research Institute,Chinese Academy of Agricultural Sciences,Harbin 150001,China) |
| Abstract: | Our previous studies found that the Chinese attenuated EIAV vaccine was composed of a pool of quasispecies,which showed a complicated diversity called "multi-species".Further determining the viral composition of these species in the vaccine should improve the identification of predominant viruses in the vaccine and facilitate the analysis of in vivo evolution of EIAV and the vaccine.In this study,the comparison of fidelities in amplifying and sequencing the V3 to V5 fragment of EIAV envelope gp90 gene by either a single-genome amplification(SGA) approach or the traditional RT-PCR(bulk PCR) was performed.Results revealed that the diversities were 1.84% and 1.88% for SGA-and bulk PCR-derived sequences,respectively.Futher analysis revealed that beside the sequences highly homologous to those derived by the bulk PCR,nine of 73 sequences derived by SGA contained a deduced amino acid domain that was identical to the corresponding domain in the virulent strain LN40.In addition,sequences with deletion of one predicted amino acid residual was detected by using SGA The presence of these less populated sequences provided additional evidence for the "multi-species" hypothesis for the action mechanism of the EIAV vaccine.Furthermore,based on the analysis of sampling bias,Our results that the difference in copy number of each viral specie in the pool of quasispecies resulted in the inefficiency to amplify viral sequences that were in low population by bulk PCR.Therefore,the sequences amplified by bulk PCR could not correctly represent the composition of quasispecies.As an approach based on the amplification and sequencing single isolated genome,SGA significantly improved the weakness of bulk PCR and appeared its advantage in analysis of EIAV genome composition with high variety. |
| Keywords: | Single-genome amplification Bulk PCR Equine infectious anemia virus Diversity |
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