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Construction and Identification of mntA Deletion Mutant of Bacillus anthracis AP422

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ã€Authorã€‘ DIAO Li-Peng;WANG Yan-Chun;WAN Xiu-Kun;TAO Hao-Xia;YUAN Sheng-Ling;YANG Bai-Liang;LIU Chun-Jie;College of Animal Science and Veternary Medicine,Tianjian Agriculture University;Beijing Institute of Biotechnology,State Key Laboratory of Pathogen and Biosafety;

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ã€Abstractã€‘ Objective: To construct mntA gene deletion mutant of attenuated Bacillus anthracis AP422 strain.Methods: The upstream and downstream homologous arms of mntA gene were amplified by PCR, then they werelinked to the thermosensitive plasmid to construct the targeting vector, which was transformed to the attenuated B. anthracis AP422. Under the pressure of antibiotics and temperature, mntA gene of AP422 was knocked out by ho-mologous recombination, and then the resistance selection marker was deleted using Cre-LoxP system. The recombi-nant strain was identified by PCR and Western blotting and its biological character was also analyzed. Results: The mntA gene was successfully knocked out and the resistance selection marker was also deleted. Compared tothe AP422 strain, the fitness of the mutant strain decreased significantly. Conclusion: The mntA gene deletion mu-tant strain is more attenuated and can potentially serve as an live attenuated vaccine candidate.æ›´å¤š è¿˜åŽŸ

ã€å…³é”®è¯ã€‘ ç‚ç–½èŠ½èƒžæ†èŒï¼› mntAåŸºå› ï¼› æ¸©æ•è´¨ç²’ï¼› åŒæºé‡ç»„ï¼› Cre-LoxPç³»ç»Ÿï¼›
ã€Key wordsã€‘ Bacillus anthracisï¼› mntA geneï¼› thermosensitive plasmidï¼› homologous recombinationï¼› Cre-LoxP systemï¼›

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Construction and Identification of mntA Deletion Mutant of Bacillus anthracis AP422

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