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动物冠状病毒通用PCR方法的建立及基因序列分析 被引量:3

Establishment of universal PCR and sequence analyse of polymerase genes of animal coronaviruses
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摘要 参考GenBank中公布的冠状病毒相关序列,根据动物冠状病毒聚合酶基因的保守区段设计一对通用引物。用这对引物对犬冠状病毒、猫冠状病毒等8种动物冠状病毒的cDNA模板进行通用PCR扩增和通用PCR反应条件的优化,结果均得到与试验设计相符的449 bp条带;特异性试验结果表明犬冠状病毒、猫冠状病毒等均扩增出449 bp目的条带,而阴性对照没有。敏感性试验结果表明,其敏感程度与常规PCR方法相同。将扩增的聚合酶基因与冠状病毒的参考毒株进行同源性比对,同源率在56.69%~99.55%之间。进化树分析结果与文献中对冠状病毒根据血清学与基因学角度分类报道相一致。 A pair of universal primers were designed according to conservative regions of RNA polymemse genes of animal coronavirues published at GenBank, and used to amplify DNA fragment from cDNA of canine comnavirus (CCV), feline coronavirus and other 6 coronaviruses. The PCR conditions were optimized and a specific 449 bp gene segment was amplified from CCV and other coronaviruses. Sequence of PCR fragments of RNA polymerase genes were compared with those of reference strains, which showed nucleotide homology of 56.69 % to 99.55 %. The results also showed a phylogenetic tree that was identical to the published results.
作者 吕彩云 王权 张建武 陈燕军 胡永浩
机构地区 甘肃农业大学动物医学院 中国农业科学院上海家畜寄生虫病研究所重点实验室
出处 《中国预防兽医学报》 CAS CSCD 北大核心 2007年第6期461-466,共6页 Chinese Journal of Preventive Veterinary Medicine
基金 "十五""863"国家重大科技攻关专项"功能基因组和生物芯片"(2003AA2Z2060)
关键词 动物冠状病毒 聚合酶基因 通用聚合酶链反应 animal coronavirus polymerase gene universal PCR
分类号 S852.659.6 [农业科学—基础兽医学] S852.44 [农业科学—兽医学]
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参考文献14

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二级参考文献59

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共引文献13

同被引文献31

引证文献3

二级引证文献17

中国预防兽医学报
2007年 第6期

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