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作 者:马莹[1] 胡孝素[1] 王雅静[1] 王子龙[1]
机构地区:[1]四川大学华西基础医学和法医学院寄生虫学教研室,成都610044
出 处:《中国寄生虫学与寄生虫病杂志》2002年第4期197-200,共4页Chinese Journal of Parasitology and Parasitic Diseases
基 金:国家自然科学基金资助项目 (No.39970 667)~~
摘 要:目的 测定我国平原疫区和荒漠疫区杜氏利什曼原虫分离株活性蛋白激酶 C受体同源物 (L ACK)基因序列 ,并与山丘疫区分离株及国外利什曼原虫分离株进行比较。 方法 应用 RT- PCR扩增 L ACK基因 ,将其克隆入p UC18载体后用双脱氧链末端终止法测序 ,并与 Gen Bank中相关数据进行比较。 结果 用 RT- PCR成功扩增出约95 0 bp的 L ACK基因片段 ,测序结果表明其片段大小均为 94 2 bp,与 Gen Bank中多种利什曼原虫 L ACK基因的核苷酸序列一致性达 97%以上。我国山丘、平原和荒漠 3个不同疫区杜氏利什曼原虫分离株的 L ACK基因序列的一致性达95 %以上。 结论 获得了我国平原和荒漠疫区杜氏利什曼原虫 L ACK基因序列。我国 3个不同疫区杜氏利什曼原虫分离株的 L ACK基因具有高度同源性。Objective To determine the nucleotide sequence of the LACK (Leishmania homologue of receptors for activated protein kinase C) gene of Leishmania donovani isolates from plain foci (L.d SD1) and desert foci (L.d XJ771) of China, and to find out the difference of the sequence of LACK gene with other Leishimania spp. and also the isolate from hill foci of China.. Methods. The LACK genes of L.d SD1 and L.d XJ771 were amplified by RT-PCR and cloned into pUC18 vector respectively, sequenced by the dideoxy chain termination method, then analyzed and compared with that of other isolates.. Results . The LACK genes of the two isolates were successfully cloned. Both of the 2 fragments were 942 bp in length. Comparison of the two nucleotide sequences with that of other Leishmania spp. in GenBank showed that the identities were more than 97%, and the identities of the nucleotide sequences of LACK genes of the three L.d isolates from plain, desert and hill foci of China were more than 95%.. Conclusion . High identities exist among the nucleotide sequences of LACK genes of the three L.d isolates from the three foci of China.
关 键 词:杜氏利什曼原虫 荒漠疫区 基因克隆 序列分析 平原疫区 活性蛋白激酶C受体同源物 对比分析
分 类 号:R382.22[医药卫生—医学寄生虫学]
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