14 June 2017 3 262 Report

To get a gene's full sequence, I design some primers according to the RNAseq result and cDNA-RACE. it should be note that RNAseq result is consistent with cDNA-RACE result. i try to make the primer F and R target to the fore and aft ends (ATG and TAG), respectively. however, those primers either could not result any stripe or the stripes turn out to be irrelevant sequence.

what's wrong with my PCR?

it drive me nuts.

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