I have problems getting very weak fluorescence signal from my probe-based RT-qPCR assay. The Ct is not bad (less than 30, and I see a clear although weak band on gel), but the signal intensity is low and probably therefore the curves are not nice and clean but sort of shaky. This is a standard probe-based assay with CY3-BHQ2 probe, using the Strategene MX3005P instrument, and the default fast 2-step protocol, annealing/extension at 60C.
I have had similar problems with another CY3-based probe previously with this instrument, so I'm slightly suspecting that there might be something wrong with the detection. I have set the CY3 signal amplification to the maximum in the software but it's still quite weak.
Alternatively, I guess it might be about the probe binding. I have little experience in optimizing this type of assays, so I would welcome any suggestions here. Increasing probe concentration? Lowering the annealing/extension temp? Trying a 3-step protocol perhaps?