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丝状真菌链格孢中高效的基因靶向

Efficient gene targeting in the filamentous fungus Alternaria alternata.

作者信息

Shiotani H, Tsuge T

机构信息

School of Agricultural Sciences, Nagoya University, Japan.

出版信息

Mol Gen Genet. 1995 Jul 28;248(2):142-50. doi: 10.1007/BF02190795.

DOI:10.1007/BF02190795
PMID:7651337
Abstract

To characterize homologous recombination of transforming DNA in the filamentous fungus Alternaria alternata, we have compared the frequencies of gene targeting by circular and linear DNA fragments in the fungus. The A. alternata BRM1 gene, which is an essential gene for melanin biosynthesis, was selected as a target locus. BRM1 targeting events are easily identified because loss of function leads to a change in mycelial color from black to light brown. We constructed targeting vectors by inserting 0.6 to 3.1 kb internal BRM1 segments into a plasmid containing the hygromycin B phosphotransferase gene. When circular plasmids were used, melanin-deficient (Mel-) transformants accounted for 30 to 80% of hygromycin B-resistant (HyR) transformants, correlating closely with the size of the BRM1 segment in the transforming DNA. Restriction enzyme digestion within the BRM1 region greatly enhanced the frequency of gene targeting: integration of the linear plasmids was almost completely attributable to homologous recombination, regardless of the size of the BRM1 segments. Plasmids carrying both BRM1 segments and rDNA segments were transformed into the fungus to examine the effect of the number of target copies on homologous recombination. Using the circular plasmids, Mel- transformants accounted for only 5% of HyR transformants. In contrast, when the linear plasmid produced by restriction enzyme digestion within the BRM1 segment was used, almost all transformants were Mel-. These results indicate that homologous integration of circular molecules in A. alternata is sensitive to the length of homology and the number of targets, and that double-strand breaks in transforming DNA greatly enhance homologous recombination.

摘要

为了表征丝状真菌链格孢中转化DNA的同源重组,我们比较了该真菌中环状和线性DNA片段的基因靶向频率。选择了黑色素生物合成必需基因链格孢BRM1基因作为靶位点。由于功能丧失会导致菌丝体颜色从黑色变为浅棕色,因此很容易识别BRM1靶向事件。我们通过将0.6至3.1 kb的BRM1内部片段插入含有潮霉素B磷酸转移酶基因的质粒中来构建靶向载体。当使用环状质粒时,黑色素缺陷型(Mel-)转化体占潮霉素B抗性(HyR)转化体的30%至80%,这与转化DNA中BRM1片段的大小密切相关。BRM1区域内的限制性酶切大大提高了基因靶向频率:线性质粒的整合几乎完全归因于同源重组,而与BRM1片段的大小无关。将携带BRM1片段和rDNA片段的质粒转化到该真菌中,以检查靶拷贝数对同源重组的影响。使用环状质粒时,Mel-转化体仅占HyR转化体的5%。相反,当使用在BRM1片段内通过限制性酶切产生的线性质粒时,几乎所有转化体都是Mel-。这些结果表明,链格孢中环状分子的同源整合对同源长度和靶标数量敏感,并且转化DNA中的双链断裂极大地增强了同源重组。

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本文引用的文献

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