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My RNAseq data and qPCR showed that there is an up-regulation of one lincRNA in the treated cells but when I want to amplify the full length of this lincRNA (1600bp) by RT-PCR, I have no band. Do...
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I diluted siRNA and RNAiMAX in opti-MEM and added to the cells which they were in the growth medium. Is it a right way? or should I culture cells in the opti-MEM medium for a while and not in...
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I am trying to clone a pGreenPuro vector (size 8kb) into stbl3 cells but eventually there is no colony on the plates. I plate them 37 ’C overnight on the LB-agar plates. Any solution?
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