I am working on a gene expression experiment using SYBR green RT-PCR. I see perfect single peak melting curves for reference gene in my control samples but curves are erratic for treatment sample groups.I tried multiple reference gene primers,the results are the same. I am planning to spike equal amount of RNA to my extracted RNA samples for the expression study. Any one has faced similar problem? have any experience with spiking RNA for real-time RT-PCR? need your comments and suggestion. Thanks.