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The minimal duplex DNA sequence required for site-specific recombination promoted by the FLP protein of yeast in vitro

机译:酵母的FLP蛋白在体外促进位点特异性重组所需的最小双链DNA序列

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摘要

The 2–micron piiraid of tho yeast Saccharomyces cerevisiae codes for a site-specific reconbinase (‘FLP') that efficiently catalyses recombination across the plasmid's two 599 bp repeats both in vivo and in vitro. We have used the partially purified FLP protein to define the minimal duplex DNA sequence required for intra- and intermolecular recombination in vitro. Previous DNase footprinting experiments had shown that FLP protected 50 bp of DNA around the recombination site. We made BAL31 deletions and synthetic FLP sites to show that the minimal length of the site that was able to reconbine with a wild-type site was 22 bp. The site consists of two 7 bp inverted repeats surrounding an 8 bp core region. We also showed that the deleted sites recombined with themselves and that one of three 13 bp repeated elements within the FLP target sequence was not necessary for efficient recombination in vitro. Mutants lacking this redundant 13 bp element required a lower amount of FLP recombinase to achieve naxinal yield of recombination than the wild type site. Finally, we discuss the structure of the FLP site in relation to the proposed function of FLP recombination in copy number amplification of the 2–micron plasmid in vivo.
机译:酵母酿酒酵母的2微米piiraid编码一种位点特异性重组酶('FLP'),可在体内和体外有效地催化质粒两个599 bp重复序列之间的重组。我们已经使用了部分纯化的FLP蛋白来定义体外和分子间重组所需的最小双链DNA序列。先前的DNase足迹实验表明FLP保护了重组位点周围50 bp的DNA。我们进行了BAL31缺失和合成FLP位点的研究,以表明能够与野生型位点重新结合的位点的最小长度为22 bp。该位点由围绕一个8 bp核心区域的两个7 bp反向重复序列组成。我们还显示了缺失的位点与它们自身重组,并且在FLP目标序列中三个13 bp重复元件之一对于体外有效重组不是必需的。与野生型位点相比,缺少这种冗余的13 bp元件的突变体需要较少量的FLP重组酶才能达到重组的naxinal产量。最后,我们讨论了与FLP重组在体内2微米质粒的拷贝数扩增中所提出的功能有关的FLP位点结构。

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