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灰盖鬼伞中的插入诱变:利用显性选择标记产生带标签的、孢子形成缺陷型突变体。

Insertional mutagenesis in Coprinus cinereus: use of a dominant selectable marker to generate tagged, sporulation-defective mutants.

作者信息

Cummings W J, Celerin M, Crodian J, Brunick L K, Zolan M E

机构信息

Department of Biology, Indiana University, Bloomington 47405, USA.

出版信息

Curr Genet. 1999 Dec;36(6):371-82. doi: 10.1007/s002940050512.

DOI:10.1007/s002940050512
PMID:10654091
Abstract

We have constructed a dominant selectable marker, PHT1, for transformation of the basidiomycete Coprinus cinereus. PHT1 consists of a bacterial hygromycin B resistance gene fused to the promoter and terminator regions of the C. cinereus beta-tubulin gene. We found in transformation experiments that PHT1 confers hygromycin B resistance to all strains of C. cinereus tested, that it integrates without apparent bias into the genome, and that it is stable through meiotic crosses. We used a plasmid containing this marker, pPHT1, for restriction enzyme-mediated integration (REMI) and found that this technique could increase transformation efficiencies more than seven-fold. In REMI experiments using KpnI, the integrated DNA was flanked by intact KpnI sites in 53% of the cases examined, single-copy insertions represented 60% of the integration events, and most multicopy insertions were oriented head-to-tail. A screen of REMI-generated transformants yielded sporulation-defective mutants at a frequency of 1.2%. Genetic analysis showed that in six of nine mutants examined, the defect in spore formation is most likely a direct result of the pPHT1 insertion, and in three of these mutants a single pPHT1 locus was shown to cosegregate with the sporulation defect. We used semi-random PCR to isolate the genomic DNA adjacent to one pPHT1 insertion in a sporulation-defective mutant and found that we had disrupted the C. cinereus spo11 gene. Thus, REMI, in combination with pPHT1, is a powerful tool for the dissection of the meiotic process in C. cinereus.

摘要

我们构建了一个显性选择标记PHT1,用于担子菌灰盖鬼伞的转化。PHT1由一个细菌潮霉素B抗性基因与灰盖鬼伞β-微管蛋白基因的启动子和终止子区域融合而成。我们在转化实验中发现,PHT1赋予所有测试的灰盖鬼伞菌株潮霉素B抗性,它能无明显偏向地整合到基因组中,并且在减数分裂杂交中是稳定 的。我们使用含有这个标记的质粒pPHT1进行限制性内切酶介导的整合(REMI),发现该技术可使转化效率提高7倍以上。在使用KpnI的REMI实验中,在所检测的53%的案例中,整合的DNA两侧是完整的KpnI位点,单拷贝插入占整合事件的60%,并且大多数多拷贝插入是头对头排列的。对REMI产生的转化体进行筛选,得到产孢缺陷突变体的频率为1.2%。遗传分析表明,在所检测的9个突变体中的6个中,孢子形成缺陷很可能是pPHT1插入的直接结果,并且在其中3个突变体中,单个pPHT1位点与产孢缺陷共分离。我们使用半随机PCR分离产孢缺陷突变体中一个pPHT1插入位点附近的基因组DNA,发现我们破坏了灰盖鬼伞的spo11基因。因此,REMI与pPHT1相结合,是剖析灰盖鬼伞减数分裂过程的有力工具。

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