For validation by qPCR of several microRNAs, is it necessary to measure normalization miRNAs in each plate in addition to the miRNAs under study? Or can you make plates of microRNAs and then extrapolate the value we got from one of the normalization microRNAs?
Saurabh Mandal
As long as you gather your Cq values at a valid threshold on a per target basis, If you have same cDNA and same master mix, your comparisons will be valid. However, to avoid interplate variability, it is best practice to pipette all samples for a given target, and reference genes on a single plate.
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