Hi all,

I am a Microbiologist, and I'm very new to using any bioinformatics tool and still struggling in understanding the very basic concepts of bioinformatics in general....I hope you would bear up with my very naive questions, as I'm really really lost..

I want to design a primer for my bacterial enzyme, so from what I know is that I have to make multiple alignment for the DNA sequences I have first.. .

I am using CLC genome workbench as I find it user friendly. I add about 8 different sequences of this enzyme from 8 different bacterial strains and then made the alignment, but doing this I found that there is almost no similarity and the percentage of conserved parts is very little. I understand this would be a hindrance to design a good primer, right?

So what shall I do now...should I choose other organisms than those and start all over or what?

Highly variable sequences are hard nuts to crack, but I would try PrimerDesign-M software published recently in Bioinformatics (see the paper). This tool designs primers based on multiple-alignment of highly variable genomic sequences.

You need to specify your aim from this designing. Are you going to do clone for expression, in this case, you need from the starting methionine to the last stop codon. Or, if you want to only isolate the conserved region(s). Also, you should mention if you aligned DNA/mRNA or Protein seq. I got the feeling that you might doing something wrong. Mostly aligning similar sequences will give you conserved region all over the seq. Also, remember that mRNA or CDS seq will not help you if you wish to clone for expression, you need to find where is the DNA/mRNA seq that correspond to the starting aa. The same for the last stop codon. Another hint is to check if you use CLC GW properly or not, is by copying and pasting one seq and use it in your alignment.