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利用酵母转化系统进行寡脱氧核苷酸定向诱变

Oligodeoxynucleotide-directed mutagenesis using the yeast transformation system.

作者信息

Walder R Y, Walder J A

出版信息

Gene. 1986;42(2):133-9. doi: 10.1016/0378-1119(86)90289-1.

Abstract

In this report we describe a highly efficient method for site-specific mutagenesis using the yeast transformation system. The method is based on the observation that Saccharomyces cerevisiae can be transformed at high frequency with single-stranded circular DNA vectors [Singh et al., Gene 20 (1982) 441-449]. The model system studied was the TRP1 gene of S. cerevisiae cloned into a derivative of the phage M13mp9 vector containing the yeast URA3 gene. ARS1, located adjacent to the TRP1 gene, allows the plasmid to replicate autonomously in yeast. Synthetic 5'P-oligodeoxynucleotides, 19 and 35 nucleotides (nt) in length, designed to produce an A----T transversion mutation within the TRP1 gene, were annealed to ss DNA of the M13 vector at a molar ratio of 30:1 and directly transformed into yeast. The intended single nt mutation was obtained at frequencies of 24 and 43%, respectively. The latter approaches the theoretical limit of 50%. In the absence of the 5'-terminal phosphate, both the transformation frequency and the efficiency of mutagenesis by the synthetic oligodeoxynucleotide (oligo) were decreased by 2-4 fold. This procedure completely obviates the need for any enzymatic manipulations in vitro after forming the heteroduplex with the oligo primer containing the desired mutation. For yeast genes, direct phenotypic selection is possible in the recipient strain.

摘要

在本报告中,我们描述了一种利用酵母转化系统进行位点特异性诱变的高效方法。该方法基于这样的观察结果:酿酒酵母能够被单链环状DNA载体高频转化[辛格等人,《基因》20(1982)441 - 449]。所研究的模型系统是克隆到含有酵母URA3基因的噬菌体M13mp9载体衍生物中的酿酒酵母TRP1基因。位于TRP1基因附近的ARS1使质粒能够在酵母中自主复制。设计用于在TRP1基因内产生A→T颠换突变的长度为19和35个核苷酸(nt)的合成5'P - 寡脱氧核苷酸,以30:1的摩尔比与M13载体的单链DNA退火,并直接转化到酵母中。预期的单核苷酸突变分别以24%和43%的频率获得。后者接近50%的理论极限。在没有5'-末端磷酸的情况下,合成寡核苷酸(oligo)的转化频率和诱变效率均降低了2 - 4倍。在用含有所需突变的oligo引物形成异源双链体后,该程序完全消除了体外任何酶促操作的必要性。对于酵母基因,可以在受体菌株中进行直接表型选择。

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