通过消除DNA转移的三个障碍,开发一种用于吸水链霉菌应城亚种(三种有用抗真菌化合物的产生菌)的基因克隆系统。
Development of a gene cloning system for Streptomyces hygroscopicus subsp. yingchengensis, a producer of three useful antifungal compounds, by elimination of three barriers to DNA transfer.
作者信息
Qin Z, Peng K, Zhou X, Liang R, Zhou Q, Chen H, Hopwood D A, Kieser T, Deng Z
机构信息
Department of Soil Sciences and Agrochemistry, Huazhong Agricultural University, Wuhan, Hubei, People's Republic of China.
出版信息
J Bacteriol. 1994 Apr;176(7):2090-5. doi: 10.1128/jb.176.7.2090-2095.1994.
Abstract
Streptomyces hygroscopicus 10-22 could not be transformed with any of the commonly used Streptomyces plasmid vectors and was resistant to plaque formation by the Streptomyces phages phi C31 and R4. Repeated selection resulted in the isolation of derivatives of S. hygroscopicus 10-22 that could be transformed with pIJ101- and pJV1-derived cloning vectors and of restriction-deficient derivatives that could accept DNA propagated in Streptomyces lividans 66. These new strains, which include three that still produce the original antibiotics, can be used as hosts for gene cloning. Insertion of nonreplicating vectors by homologous recombination and transposition of Tn4560 were demonstrated in S. hygroscopicus 10-22.
摘要
吸水链霉菌10-22不能被任何常用的链霉菌质粒载体转化,并且对链霉菌噬菌体φC31和R4形成噬菌斑具有抗性。经过反复筛选,获得了吸水链霉菌10-22的衍生物,它们可以被pIJ101和pJV1衍生的克隆载体转化,还获得了限制缺陷型衍生物,这些衍生物可以接受在变铅青链霉菌66中繁殖的DNA。这些新菌株,包括三种仍能产生原始抗生素的菌株,可作为基因克隆的宿主。在吸水链霉菌10-22中证明了通过同源重组插入非复制型载体以及Tn4560的转座。
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