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5.9 years ago
AP
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Hello everyone,
I am trying to validate my RNAseq data by doing qpcr for which I am looking at the fold change of few genes across various timepoints of treatment conditions. I am getting huge amount of variation (in thousand folds ) in my biological replicates. I thought may be it is due to genomic DNA contamination so thats why I repeated all my experiment and did DNase treatment twice but still I am having such variations. I am using two reference genes EF and GAPDH and I also have variations in the Ct values of reference genes across various timepoints. I will really appreciate it if you could suggest me with possible problems and solutions.
Thank you,
Ambika
It sounds like you have variable degradation of your samples.
i already checked the degradation by running gel on my RNA samples before and after DNAse treatment. They look fine.
As this is purely wet-lab, I may redirect you to Stackexchange to ask this question.