Hi there,

First of all, your PCR experiment is giving very low intensity bands (except the last 2 obviously but as it is overexposed I can't tell...) so there might be some issue there. There are also some controls lacking : colony PCR on a plasmidless clone and colony PCR on a clone containing the empty plasmid to see what kind of background is expected in the cell context. Intuitively I would say the last 2 reactions are true positives (if there are true bands with the expected size there...) and I think the rest you get is non target specific amplification.

Thank you dear Dominique. About controls I have done Colony PCR for them before; Colon containing pcDNA3.1+ whithot insert and no transfected DH5-alpha alone. PCR were negative for bout of them. In last step, TA coloning, I had the same, you called "non-target specific amplification" bands. About the size of bands, they are my actual desired size, 476bps. Ladder is 100bp but badly opened. Middle ladde's band is 500bps where my band is below it. I want to continue my work and transfet cell line, but I do not know take this results as possitive or no. What would you do?

Sincerely

Hi again,

As your colony PCR is not working great I would go for systematic plasmid extraction, digest and sequencing for those exhibiting the right profile of digestion.

I completely agree with Dominique. Use empty pcDNA3.1 vector as negative control and to check whether sites from the vector backbone gets amplified by your primers. Use the TA cloned plasmid as positive control to check the amplicon of your desired size. After you get positive result, digest your clones with the restriction enzymes you used for cloning, load them beside your colony PCR products and see whether they align according to your expected size. Moreover, if you have isolated plasmid and then set PCR, your bands (with insert) should be more intense. That is what I get after 29 cycles. 

Hope it helps!