Hi,
I am currently working on a project designing a primer template for detecting any pathogenic species of leptospira in a serum sample, but I seem to have hit a roadblock. While the ncbi primer design tool has proven exceedingly useful, I am unable to figure out how to extract a conserved primer (both forward and reverse) that can be used for two different strains of borgpetersenii and three different strains of interoganns. I used mauve to get a comparative genomics profile of the five different strains, and then ran a highly conserved region through the ncbi pcr design tool. While it gives me results, these results are good for the particular species that I used. So how could I go about designing a primer that can be used for all these strains, if that is at all possible ? Any help or clarity would be greatly appreciated.
Thanks in advance
You can use ProSig (http://public.lanl.gov/jgans/prosig/prosig-1.1.tar.gz) to automatically design PCR primers that target conserved regions of multiple bacterial genomes. The basic idea is to first enumerate a large number of valid PCR primer pairs and then throw away all of the pairs that don't produce an amplicon in all of your target genomes. This approach does not require a multiple sequence alignment. See http://www.ncbi.nlm.nih.gov/pubmed/22434885 for a description of the algorithm.
The link to ProSig no longer works. The publication has only been cited 8 times since 2012.