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作 者:刘芳 常子丽 李建云 王建军 王浩珲 胡艳红 武正华 马志东 范龙兴 张忠兵
机构地区:[1] 内蒙古地方病防治研究中心,呼和浩特010031 [2] 内蒙古满洲里市疾病预防控制中心地方病防治科
出 处:《中华地方病学杂志》2015年第5期322-325,共4页Chinese Journal of Endemiology
摘 要:目的 确定内蒙古鼠疫自然疫源地8种啮齿类动物细胞色素C氧化酶亚基Ⅰ (CO Ⅰ)基因扩增的最佳引物.方法 在内蒙古锡林郭勒盟和乌兰察布市,采集8个鼠种的动物,提取基因组DNA,选择6对已报道的扩增鼠CO Ⅰ基因的引物(F1/R1、F2/R2、F3/R3、F4/R4、VF/VR、F6/R6),PCR扩增8个鼠种的CO Ⅰ基因,对扩增的产物进行测序,并对测序结果进行生物信息学分析和比较.结果 达乌尔黄鼠扩增CO Ⅰ基因的最佳引物为F3/R3,达乌尔鼠兔和蒙古兔尾鼠均为鸡尾酒引物VF/VR,大沙鼠、蒙古毛足鼠和布氏田鼠均为F6/R6,五趾跳鼠为F2/R2,子午沙鼠为F1/R1.8种啮齿动物的CO Ⅰ序列进行比对后,发现所有DNA条码都是物种所独有,每个物种都有各自的鉴别位点.结论 不同鼠种在扩增CO Ⅰ基因时需要相应种属特异性引物;扩增多种鼠种时,优先选择F6/R6引物或鸡尾酒引物,针对特殊鼠种可选择该鼠种特异引物进行扩增.Objective To determine the optimal primers of cytochrome C oxidase subunit Ⅰ (CO Ⅰ) gene for 8 kinds of rodents in natural epidemic focus of plague in Inner Mongolia.Methods In Xilingol League and Wulanchabu City of Inner Mongolia,eight kinds of rodents were collected and DNA was extracted;six pairs of targeted primers (F1/R1,F2/R2,F3/R3,F4/R4,VFNR,F6/R6) were used to amplify the CO Ⅰ gene of the 8 species by PCR;PCR products were send to biotechnology company for sequencing,and bioinformatics analysis of the sequencing results was conducted.Results F3/R3 was the optimal CO Ⅰ gene primer for Spermophilus dauricus;cocktail primer (VFNR) was the optimal CO Ⅰ gene primer for Ochotona daurica and Lagurus przewalskii;F6/R6 was the optimal CO Ⅰ gene primer for Rhombomys opimus,Phodopus campbelli and Microtus brandti;F2/R2 was the optimal CO Ⅰ gene primer for Allactaga sibirica,and F1/R1 was the optimal CO Ⅰ gene primer for Meriones meridianus.CO Ⅰ gene sequences of the 8 kinds of rodents were compared;DNA barcoding was unique in each rodent and every rodent had differential point.Conclusions Different rodent needs its own species-specific primers for CO Ⅰ gene amplification.Upon amplification of different rodent,cocktail or F6/R6 primers are the first choices,and choose the species-specific primers for particular species to amplify.
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