New method for generating deletions and gene replacements in Escherichia coli.

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J Bacteriol. 1989 September; 171(9): 4617-4622

research-article

New method for generating deletions and gene replacements in Escherichia coli.

C M Hamilton, M Aldea, B K Washburn, P Babitzke and S R Kushner

Department of Genetics, University of Georgia, Athens 30602.

ABSTRACT

We describe a method for generating gene replacements and deletionsin Escherichia coli. The technique is simple and rapid and canbe applied to most genes, even those that are essential. Whatmakes this method unique and particularly effective is the useof a temperature-sensitive pSC101 replicon to facilitate thegene replacement. The method proceeds by homologous recombinationbetween a gene on the chromosome and homologous sequences carriedon a plasmid temperature sensitive for DNA replication. Thus,after transformation of the plasmid into an appropriate host,it is possible to select for integration of the plasmid intothe chromosome at 44 degrees C. Subsequent growth of these cointegratesat 30 degrees C leads to a second recombination event, resultingin their resolution. Depending on where the second recombinationevent takes place, the chromosome will either have undergonea gene replacement or retain the original copy of the gene.The procedure can also be used to effect the transfer of anallele from a plasmid to the chromosome or to rescue a chromosomalallele onto a plasmid. Since the resolved plasmid can be maintainedby selection, this technique can be used to generate deletionsof essential genes.

J Bacteriol. 1989 September; 171(9): 4617-4622

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