南方医科大学学报

南方医科大学学报 ›› 2015, Vol. 35 ›› Issue (11): 1546-.

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肠出血型大肠埃希菌O157:H7 espF 基因缺失株和回补株的构建

华颖,孙琦,王湘雨,杜艳丽,邵娜,张其威,赵卫,万成松   

  • 出版日期:2015-11-20 发布日期:2015-11-20

Construction of enterohemorrhagic Escherichia coli O157:H7 strains with espF gene
deletion and complementation

  • Online:2015-11-20 Published:2015-11-20

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摘要: 目的利用Red同源重组系统敲除肠出血型大肠埃希菌的espF基因及其核苷酸片段;建立以pBAD 33质粒为载体的espF
基因回补实验平台。方法设计1 对同源臂引物扩增卡那霉素抗性打靶片段,将抗性打靶片段电转入含有PKD46 质粒的
EDL933w,在PKD 46介导的重组系统帮助下,打靶片段和菌体espF基因发生同源重组,PCR和测序验证;PCR扩增espF及其核
苷酸片段的整个ORF区序列,将其克隆入pBAD33质粒,分别将重组质粒转入相应的缺失株,以构建出相应的回补突变株。采
用RT-PCR的方法验证在相应的回补突变株中espF及其核苷酸片段是否转录。结果构建了espF基因及其核苷酸片段缺失的
EHEC O157:H7 EDL933w突变菌株和相应的回补株,且espF基因及其核苷酸片段在回补株中均发生转录。结论本研究运用
Red重组系统构建了肠出血型大肠埃希菌O157:H7 espF基因缺失株,并建立以pBAD33质粒为载体的EHEC O157:H7基因回
补方法,为进一步研究肠出血型大肠埃希菌中espF基因的调控机制奠定了基础。

Abstract: Objective To construct enterohemorrhagic Escherichia coli (EHEC) O157:H7 strains with delection espF gene and its
nucleotide fragment and with espF gene complementation. Methods A pair of homologous arm primers was designed to
amplify the gene fragment of kanamycin resistance, which was transformed into EHEC O157:H7 EDL933w strain via the
PKD46 plasmid by electroporation. The replacement of the espF gene by kanamycin resistance gene through the
PKD46-mediated red recombination system was confirmed by PCR and sequencing. The entire coding region of espF along
with its nucleotide fragment was amplified by PCR and cloned into pBAD33 plasmid, which was transformed into a mutant
strain to construct the strain with espF complementation. RT-PCR was used to verify the transcription of espF and its nucleotide
fragment in the complemented mutant strain. Results and Conclusion We established EHEC O157:H7 EDL933w strains with
espF gene deletion and with espF gene complementation. Both espF and its nucleotide fragment were transcribed in the
complemented mutant strain. The two strains provide a basis for further study of the regulatory mechanism of espF.