Hi everybody,

I carried out a qPCR in order to quantify expression level of two genes under different conditions. I used three pairs of primers, one for the endogenous control and two for the GOI, I did not design but they have already been used by a colleague before.

I added NTC samples and -RT (RNA after DNase treatment).

I got amplification in both, NTC and -RT samples. The peaks of these samples showed by the melt curve matches exactly the peaks of the unknown samples and even Ct value is not that high but almost the same of a few unknown samples.

I would suppose a primer dimer formation because of the amplification in NTC rather than DNA contamination but I'm just at the beginning with qPCR and I would love to hear from anyone else using it opinion, advice and suggestion.

Similar questions and discussions