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机构地区:[1]北京农业大学,中国农业科学院哈尔滨兽医研究所兽医生物技术国家重点实验室
出 处:《畜牧兽医学报》1996年第1期76-81,共6页ACTA VETERINARIA ET ZOOTECHNICA SINICA
摘 要:本研究以质粒pGEM-7Zf(+)为载体,对我国北方和南方疫区伊氏锥虫动基体株的kDNA小环进行了克隆,并以其中之pTK011-C_1为探针对不同地理区的动基体株和无动基体株的不同DNA进行杂交,结果表明,我国北、南两大疫区动基体株的kDNA小环大小均约为1kb,且均属A型,pTK011·C_1只与动基体株的kDNA及tDNA杂交,不与其nDNA杂交,也不与无动基体株的任何DNA及黄牛白细胞DNA杂交。说明具有特异性,可以用于诊断。tDNA的杂交信号与kDNA相当,诊断中可以代替kNDA作为检测对象。The kDNA minicircles of kinetoplatic strains of Trypanosoma evansi from the camelin Xinjiang Uygar Autonomous Region, Northwest China, and the horse in HubeiProvince, South China, were cloned in plasmid pGEM-7Zf(+),and one of tlie clonedkDNA minicircle pTKO11-C_1 from the camel was used to probe kDNAs,nDNAs andtDNAs of kinetoplastic and dyskinetoplastic strains from different geographical regions. The kDNA minicircles obtained from strains in Northwest and South China were allabout 1kb in size and belonged to type A according to the restriction endonucleaseanalysis.The probe pTK011-C_1 hybridized with kDNAs and tDNAs of kinetoplasticstrains,but not with their nDNAs,and also not with any kinds of DNAs fromdyskinetoplastic strains as well as bovine leucocyte DNA by Southern and Dot blothybridizations.This indicated that pTK011-C_1 was species specific and could be usedto diagnose animal T. evansi infection in China. The hybirdization strength of tDNA wasalmost the same to that of kDNA,thus,it could be used as testing target instead ofkDNA in diagnostic hybridization.
分 类 号:S852.7[农业科学—基础兽医学]
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