I am trying to optimize a primers extension assay with 2-3 kb RNA fragments to study RNA modifications (methylation and pseudouridylation).
I was wondering if anyone has an idea about the minimum length of primers that can be used without compromising the annealing and the specificity.
Secondly is there a minimum distance that should be kept from the annealing site to the site to be analyzed.( this could also be considered as a minimal length that the RT enzyme would extend from the site of annealing)