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多形汉逊酵母中复制质粒的染色体靶向

Chromosomal targeting of replicating plasmids in the yeast Hansenula polymorpha.

作者信息

Faber K N, Swaving G J, Faber F, Ab G, Harder W, Veenhuis M, Haima P

机构信息

Department of Microbiology, University of Groningen, Haren, The Netherlands.

出版信息

J Gen Microbiol. 1992 Nov;138(11):2405-16. doi: 10.1099/00221287-138-11-2405.

Abstract

Using an optimized transformation protocol we have studied the possible interactions between transforming plasmid DNA and the Hansenula polymorpha genome. Plasmids consisting only of a pBR322 replicon, an antibiotic resistance marker for Escherichia coli and the Saccharomyces cerevisiae LEU2 gene were shown to replicate autonomously in the yeast at an approximate copy number of 6 (copies per genome equivalent). This autonomous behaviour is probably due to an H. polymorpha replicon-like sequence present on the S. cerevisiae LEU2 gene fragment. Plasmids replicated as multimers consisting of monomers connected in a head-to-tail configuration. Two out of nine transformants analysed appeared to contain plasmid multimers in which one of the monomers contained a deletion. Plasmids containing internal or flanking regions of the genomic alcohol oxidase gene were shown to integrate by homologous single or double cross-over recombination. Both single- and multi-copy (two or three) tandem integrations were observed. Targeted integration occurred in 1-22% of the cases and was only observed with plasmids linearized within the genomic sequences, indicating that homologous linear ends are recombinogenic in H. polymorpha. In the cases in which no targeted integration occurred, double-strand breaks were efficiently repaired in a homology-independent way. Repair of double-strand breaks was precise in 50-68% of the cases. Linearization within homologous as well as nonhomologous plasmid regions stimulated transformation frequencies up to 15-fold.

摘要

我们使用优化的转化方案研究了转化质粒DNA与多形汉逊酵母基因组之间可能的相互作用。仅由pBR322复制子、大肠杆菌抗生素抗性标记和酿酒酵母LEU2基因组成的质粒在酵母中能够自主复制,拷贝数约为6(每基因组当量的拷贝数)。这种自主行为可能归因于酿酒酵母LEU2基因片段上存在的类似多形汉逊酵母复制子的序列。质粒以多聚体形式复制,由头对尾连接的单体组成。在分析的9个转化子中,有2个似乎含有质粒多聚体,其中一个单体存在缺失。含有基因组醇氧化酶基因内部或侧翼区域的质粒通过同源单交换或双交换重组进行整合。观察到单拷贝和多拷贝(两到三个)串联整合。靶向整合发生在1%至22%的情况中,且仅在基因组序列内线性化的质粒中观察到,这表明同源线性末端在多形汉逊酵母中具有重组活性。在未发生靶向整合的情况下,双链断裂以与同源性无关的方式有效修复。在50%至68%的情况中,双链断裂的修复是精确的。在同源以及非同源质粒区域内的线性化将转化频率提高了15倍。

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