I ran an array based q PCR and obtained data for fold change in genes. I followed this up by running end pint PCR followed by a gel. But the fold change in my end point PCR is not the same as as in my RT PCR. The primer sets are different and conditions were different as the RT PCR was a profiler array from Qiagen. Does this usually happen or should the fold change in RT PCR and end pint PCR be the same?
Thank you