Abstract
赵秋敏,曹务春,李建民,张泮河,陈山虎,曹克新,高东旗,杨红,张习坦.粒细胞埃立克体444-Epank基因的检测与序列分析[J].Chinese journal of Epidemiology,2002,23(4):286-287
粒细胞埃立克体444-Epank基因的检测与序列分析
Detection and sequencial analysis of Granulocytic ehrlichia 444-Epank gene
Received:August 20, 2001  Revised:June 08, 2012
DOI:
KeyWord: 粒细胞埃立克体  Epank基因  序列分析
English Key Word: Granulocytic ehrlichia Epank gene Sequence determination
FundProject:国家自然科学基金资助项目 (39970655 )
Author NameAffiliation
Zhao Qiumin Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
Cao Wuchun Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
Li Jianmin Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
Zhang Panhe Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
Chen Shanhu 内蒙古大兴安岭林业中心卫生防疫站 
Cao Kexin 内蒙古大兴安岭林业中心卫生防疫站 
Gao Dongqi Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
Yang Hong Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
Zhang Xitan Department of Epidemiology,Institute of Microbiology and Epidemiology of Acadmy of Military Medical Science, Beijing 100071, China 
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Abstract:
      目的 进一步证实中国大陆粒细胞埃立克体感染的病原学证据。方法 从粒细胞埃立克体结构蛋白基因序列高变区构建特异引物 ,对蜱标本、动物标本、人血标本进行聚合酶链反应(PCR)检测 ;收集全沟硬蜱特异PCR产物 ,进行克隆和序列测定 ,与GenBank中注册的序列进行同源性比较。结果 从黑龙江省采集的全沟硬蜱 (62组 ,310只 ) 2组中扩增出 44 4bp的特异DNA片段 ,而从内蒙古的动物脏器标本 (8份 )没有扩增出该片段 ,从内蒙古林业局人员血标本 (129份 )中扩增出1份该片段。对该片段的克隆和序列测定结果显示其DNA序列与美国人粒细胞埃立克体分离株(AF04 7897)对应位置相差 23个核苷酸 ,同源性为 94 .9% ,推测的氨基酸同源性为 88.44 %。结论通过粒细胞埃立克体 44 4 Epank基因的检测与分析进一步证实中国大陆存在粒细胞埃立克体的感染
English Abstract:
      Objective To provide further pathogenic evidence of Granulocytic ehrlichia infection in China. Methods Specific primers derived from 444 Epank gene were used to amplify Granulocytic ehrlichia DNA from specimens of ticks, animals and human blood. PCR products of ticks were cloned and sequenced. Results 444 bp specific DNA fragements were amplified from 2 of 62 pools of Ixodes persulcatus collected from Heilongjiang province and 1 of 129 blood specimens from forest workers in Inner Mongolia. Eight animal specimens were negative. PCR products from ticks were then cloned and squenced. It differed at 23 positions in comparison to American strain (AF047897) with 94.9 % homology. The homology of deduced ammonia was 88.44 %. Conclusion Our findings further confirmed that Granulocytic ehrlichia infection did exist in China.
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