I extracted RNA using a plant RNA extraction kit and then converted it to cDNA using another kit. I used GFP-tagged plant gene primers to amplify those genes with a 50 µl total reaction mixture. I followed the Tm of the primers for annealing temperatures, but each time, the bands did not appear in their proper locations. what is the possible reason or what should be done to solve the issue?
Paul Rutland
often primers do not anneal well at their Tm.Try a pcr at 5c lower than the lowest Tm of the 2 primers
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