I have total RNA extracted from samples which are rather precious. I am trying to perform cDNA synthesis then qPCR. The RNA appears to be intact and reasonably pure, but I only have between 20 and 100 ng per samples. The reverse transcription kit claims that it can work with as little as 100 pg of RNA. However I have always done qPCR with at least 250 ng RNA, and usually 1000 ng.
Has anyone actually performed RT and qPCR starting with so little material? Would starting with a low amount of RNA potentially skew the results of the eventual qPCR?
Thanks in advance.