construction of a recombinant vector for site-directed mutagenesis in salmonella typhimurium

نویسندگان

ania ahani azari

taghi zahraei salehi

bahar nayeri fasaei

omid madadgar

masoud alebouyeh

چکیده

background: among all common techniques in sitedirectedmutagenesis, λ red recombinase system has beenwidely used to knock out chromosomal genes in bacteria. in thismethod, there is always the risk of dna linear digestion byhost's restriction enzymes that leads to the low frequency ofrecombination. objectives:to overcome this, we constructeda recombinant vector to disrupt phop gene in salmonellatyphimurium. methods: the soeing pcr method andrestriction enzymes were used to construct the vector. results:the resulting plasmid, ptaaz92, contains a kanamycincassette with two long homologous arms flanking of the phopgene. conclusions: after electrotransformation of theptaaz92 into the salmonella typhimurium , the phop gene isreplaced by the kanamycin cassette through homologousrecombination. according to the high homology of the phopgene in many of salmonella species the ptaaz92 can be used todisrupt the phop gene in most of these species.

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عنوان ژورنال:
iranian journal of veterinary medicine

ناشر: دانشگاه تهران

ISSN 2251-8894

دوره 8

شماره 3 2014

میزبانی شده توسط پلتفرم ابری doprax.com

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