通过酵母体内同时重组和质粒洗牌构建缺乏线性化单一切割位点的大型质粒。
Construction of a large plasmid lacking linearizing single restriction sites by simultaneous in vivo recombination and plasmid shuffling in yeast.
作者信息
Miletti K E, Leibowitz M J
机构信息
Department of Molecular Genetics and Microbiology, University of Medicine and Dentistry of New Jersey-Robert Wood Johnson Medical School, Piscataway, NJ 08854-5635, USA.
出版信息
Yeast. 2000 Dec;16(16):1527-34. doi: 10.1002/1097-0061(200012)16:16<1527::AID-YEA643>3.0.CO;2-8.
Creation of large ( approximately 15 kb) recombinant plasmids can be done in a single step by co-transformation of yeast cells with a partial restriction digest of a plasmid vector and a linear insert whose ends overlap one of the vector restriction sites. This method is used to generate a plasmid expressing the Saccharomyces cerevisiae rRNA genes containing the Ca.LSU group I intron ribozyme from Candida albicans. This plasmid expresses functional rRNA and ribozyme.
通过将酵母细胞与质粒载体的部分限制性消化产物和线性插入片段(其末端与载体的一个限制性位点重叠)共转化,可以一步创建大型(约15 kb)重组质粒。该方法用于生成表达含有白色念珠菌Ca.LSU I组内含子核酶的酿酒酵母rRNA基因的质粒。该质粒表达功能性rRNA和核酶。
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