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用于将DNA位点特异性插入棒状杆菌染色体的基于噬菌体的载体。

Bacteriophage-based vectors for site-specific insertion of DNA in the chromosome of Corynebacteria.

作者信息

Oram Mark, Woolston Joelle E, Jacobson Andrew D, Holmes Randall K, Oram Diana M

机构信息

Department of Biomedical Sciences, University of Maryland Baltimore, Baltimore, MD 21201, USA.

出版信息

Gene. 2007 Apr 15;391(1-2):53-62. doi: 10.1016/j.gene.2006.12.003. Epub 2006 Dec 14.

Abstract

In Corynebacterium diphtheriae, diphtheria toxin is encoded by the tox gene of some temperate corynephages such as beta. beta-like corynephages are capable of inserting into the C. diphtheriae chromosome at two specific sites, attB1 and attB2. Transcription of the phage-encoded tox gene, and many chromosomally encoded genes, is regulated by the DtxR protein in response to Fe(2+) levels. Characterizing DtxR-dependent gene regulation is pivotal in understanding diphtheria pathogenesis and mechanisms of iron-dependent gene expression; although this has been hampered by a lack of molecular genetic tools in C. diphtheriae and related Coryneform species. To expand the systems for genetic manipulation of C. diphtheriae, we constructed plasmid vectors capable of integrating into the chromosome. These plasmids contain the beta-encoded attP site and the DIP0182 integrase gene of C. diphtheriae NCTC13129. When these vectors were delivered to the cytoplasm of non-lysogenic C. diphtheriae, they integrated into either the attB1 or attB2 sites with comparable frequency. Lysogens were also transformed with these vectors, by virtue of the second attB site. An integrated vector carrying an intact dtxR gene complemented the mutant phenotypes of a C. diphtheriae DeltadtxR strain. Additionally, strains of beta-susceptible C. ulcerans, and C. glutamicum, a species non-permissive for beta, were each transformed with these vectors. This work significantly extends the tools available for targeted transformation of both pathogenic and non-pathogenic Corynebacterium species.

摘要

在白喉棒状杆菌中,白喉毒素由某些温和棒状噬菌体(如β噬菌体)的tox基因编码。β样棒状噬菌体能够在两个特定位点attB1和attB2插入白喉棒状杆菌染色体。噬菌体编码的tox基因以及许多染色体编码基因的转录受DtxR蛋白调控,以响应Fe(2+)水平。表征DtxR依赖性基因调控对于理解白喉发病机制和铁依赖性基因表达机制至关重要;尽管这受到白喉棒状杆菌及相关棒状杆菌属物种缺乏分子遗传工具的阻碍。为了扩展白喉棒状杆菌的基因操作体系,我们构建了能够整合到染色体中的质粒载体。这些质粒包含β噬菌体编码的attP位点和白喉棒状杆菌NCTC13129的DIP0182整合酶基因。当这些载体导入非溶原性白喉棒状杆菌的细胞质中时,它们以相当的频率整合到attB1或attB2位点。溶原菌也通过第二个attB位点用这些载体进行转化。携带完整dtxR基因的整合载体补充了白喉棒状杆菌DeltadtxR菌株的突变表型。此外,β敏感的溃疡棒状杆菌菌株和对β噬菌体不敏感的谷氨酸棒状杆菌菌株都用这些载体进行了转化。这项工作显著扩展了可用于致病和非致病棒状杆菌物种靶向转化的工具。

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