18 February 2015 3 7K Report

If I'm doing a qPCR experiment where I need to determine the relative decrease in gene expression from RNAi lines that were generated by T-DNA insertion do I need to run my reference primers on each independent line? Or can I use the wild-type sample for all normalization? For example I will have 30 independent lines of tomato that each potentially have a different T-DNA insertion for our gene of interest and I will be comparing their expression to a pooled sample of wild-type tomato.

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