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A Method for Gene Disruption That Allows Repeated Use of USR3 Selection in the Construction of Multiply Disrupted Yeast Strains

机译:一种基因破坏的方法允许在多重分裂的酵母菌株的构建中重复使用USR3选择。

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摘要

In this paper, we describe a 3.8-kb molecular construct that we have used to disrupt yeast genes. The construct consists of a functional yeast URA3 gene flanked by 1.1-kb direct repeats of a bacterial sequence. It is straightforward to insert the 3.8-kb segment into a cloned target gene of interest and then introduce the resulting disruption into the yeast genome by integrative transformation. An appropriate DNA fragment containing the disruption plus flanking homology can be obtained by restriction enzyme digestion. After introducing such fragments into yeast by transformation, stable integrants can be isolated by selection for Ura+. The important feature of this construct that makes it especially useful is that recombination between the flanking direct repeats occurs at a high frequency (10-4) in vegetatively grown cultures. After excision, only one copy of the repeat sequence remains behind. Thus in the resulting strain, the Ura+ selection can be used again, either to disrupt a second gene in similar fashion or for another purpose.
机译:在本文中,我们描述了一个用于破坏酵母基因的3.8kb分子构建体。该构建体由一个功能性酵母URA3基因组成,该基因的两侧是细菌序列的1.1 kb直接重复序列。将3.8kb的片段插入克隆的目标基因中,然后通过整合转化将产生的破坏作用引入酵母基因组中,这很简单。可以通过限制性内切酶消化获得包含破坏和侧翼同源性的合适的DNA片段。通过转化将此类片段引入酵母后,可以通过选择Ura + 分离稳定的整合子。该构建体使其特别有用的重要特征是,在营养生长的培养物中,侧翼直接重复之间的重组发生频率很高(10 -4 )。切除后,仅保留重复序列的一个副本。因此,在所得菌株中,可以再次使用Ura + 选择,以类似的方式或出于其他目的破坏第二个基因。

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