Two integration methods are widely used: single and double crossover. Before I chose which one to use, I want to make sure the advantages and disadvantages of them.
Single crossovers result either in double-stranded breaks (when you use a linearized vector) or insertion ( in case of circular constructs), double cross overs result in replacement. Could you please provide some details on your work?
And by the way both of these phenomena may occur simultaneously within the host cell, and there is not much you can do to control the process. You may however, select for the single or double crossover clones, afterwards. Note that single crossovers resulting in double-stranded breaks would most likely cause cell death.
When you wanna do this in bacteria, there are two possibilitys. The plasmid you use can itegrate in your gene of interest by a singgle crossover. You interrupt the ORF by this integration. The best way to delete a gene is by double crossover, replacing the gene by an antibiotic cassette.
Thomas, I agree with you. Because single corssover just disrupt the target gene and might still leave partial function of the gene, and sometimes the insert is looped out. The double crossover can completely remove the whole gene.