Hello,
In qPCR having a set of primers and a Taqman probe, how to determine the size of the amplicon (to be) without running a gel from the PCR product? Would the presence/position of a hydrolysis probe affects the amplicon size and hence the Ct values of the amplified products between different assays developers for the same target?
Ahmed Elsadek Fakhr
If you know the primer sequence of your primers you can know the length of products through blast analysis.
Hydrolysis probe should not affect the product size as the probe is hydrolyzed not the amplicon.
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Sven Reister
probe binds between the primers, wouldn't work in another way with Taqman assays. so the primers drive the amplicon size
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