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Use of rpsL for dominance selection and gene replacement in Streptomyces roseosporus.

机译:rpsL在玫瑰链霉菌中的优势选择和基因替换中的应用。

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摘要

We developed a gene replacement system using the rpsL gene of Streptomyces roseosporus and demonstrated its utility by constructing a deletion in the S. roseosporus glnA gene. A 1.3-kb BamHI fragment that hybridized to the Mycobacterium smegmatis rpsL gene was subcloned from an S. roseosporus cosmid library and sequenced. Plasmid pRHB514 containing the rpsL gene conferred streptomycin sensitivity (Sm(S)) to the Sm(r) S. roseosporus TH149. The temperature-sensitive plasmid pRHB543 containing rpsL and the S. roseosporus glnA gene disrupted with a hygromycin resistance (Hm(r)) gene was introduced into S. roseosporus TH149, and recombinants containing single and double crossovers were obtained after a temperature increase. Southern hybridization analysis revealed that single crossovers occurred in the glnA or rpsL genes and that double crossovers resulted in replacement of the chromosomal glnA gene with the disrupted glnA. Glutamine synthetase activity was undetectable in the recombinant containing the disrupted glnA gene.
机译:我们开发了一种使用玫瑰链霉菌的rpsL基因的基因替代系统,并通过在玫瑰孢菌glnA基因中构建缺失来证明其实用性。将与耻垢分枝杆菌rpsL基因杂交的1.3-kb BamHI片段从玫瑰孢霉黏粒文库中亚克隆并测序。含有rpsL基因的质粒pRHB514赋予了链霉素对玫瑰迷链球菌TH149的敏感性(Sm(S))。将含有rpsL和被潮霉素抗性(Hm(r))基因破坏的玫瑰孢链球菌glnA基因的温度敏感性质粒pRHB543引入玫瑰孢菌TH149,并在温度升高后获得包含单双交换的重组体。 Southern杂交分析表明,在glnA或rpsL基因中发生了单次交换,并且两次交换导致了被破坏的glnA取代了染色体glnA基因。在含有被破坏的glnA基因的重组体中谷氨酰胺合成酶活性是不可检测的。

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