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内源性绵羊肺腺瘤病毒全基因组序列测定与序列分析 被引量:3

Cloning and sequence analysis of endogenous jaagsiekte sheep retrovirus
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摘要 参照内源性绵羊肺腺瘤病毒株enJSRV-20全基因组序列设计合成3对引物,应用PCR技术扩增内源性绵羊肺腺瘤病毒基因片段分别连接pMD-18T载体并测序,完成了内源性绵羊反转录病毒基因组序列测定。分析结果显示,测定序列全长7 519bp,与内源性绵羊肺腺瘤病毒代表株enJSRV-20核苷酸同源性为99.4%,与外源性绵羊肺腺瘤病毒代表株AF357971.1的核苷酸同源性为90.4%。基于全基因组序列核苷酸的系统进化发生树分析结果显示,扩增序列与enJSRV-20的亲缘关系最近。 Three pair of primers were designed according to the sequence of enJSRV-20 strain. Sequence of enJSRV was amplified by PCR technology and the PCR product was cloned into pMD18-T vector and then sequenced. So complete sequence of enjSRV was analyzed. Analysis results show that the sequences of enJSRV-20 strain had 99. 4% similarity with enJSRV sequenced, the similarity with AF357971. 1 strain was 90. 4%. Phylogenetic analysis based complete sequence showed that the sequence had the closest linkage to enJSRV-20. It will be useful in the study of infectivity clone and the function of enJSRV.
出处 《中国兽医学报》 CAS CSCD 北大核心 2012年第7期962-966,共5页 Chinese Journal of Veterinary Science
基金 国家自然科学基金资助项目(31060332)
关键词 内源性绵羊肺腺瘤病毒 PCR扩增 全基因序列 enJSRV PCR amplification ful-length genome sequence
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同被引文献33

  • 1刘淑英,马学恩,齐景伟,王宇.绵羊肺腺瘤病毒NM株前病毒基因组的克隆与全序列分析[J].中国病毒学,2006,21(5):443-448. 被引量:16
  • 2王宇,刘淑英,韩敏,李建云.内源性绵羊肺腺瘤病毒NM株gag基因的克隆、序列分析及蛋白结构预测[J].中国预防兽医学报,2007,29(4):272-276. 被引量:8
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