I am trying to define a standard curve for the primers that I have designed for qPCR and I ordered to sythetize the correpondent oligo for test the primers in different concentrations, but I don't know how much pure oligo I should use in the dilutions and I can't find some work that explain this issue. Somebody can help me?
I usually use 2500ng for the first dilution and 0,25ng for the last one in 50ul per reaction, but I have used total RNA