I used from High Fidelity PCR

Enzyme Mix (thermo scientific:product number k0191) for PCR performing.

My PCR product is 3131bp from HEK-293 cell line DNA.

On the first day, I performed a PCR test but reached a weak specific band. There does not exist any extra band or primer dimer.

Cycling protocol for PCR product:

Initial Denaturation: 95˚C for 3 min

Denaturation: 95˚C -30 s

Annealing: 55˚C for 30 s

Extension 72 ˚C for 3.30 min.

Final Extension 72 ˚C for12 min

Number of cycle: 30

Component of any reaction:

10X High Fidelity PCR buffer with 15 mM MgCl2…….5ul

dNTP Mix (10mM)……………………………….……..1 ul

Forward primer (10pm)……………………..…….…...2.5 ul

Revers primer (10pm)…………………………...……..2.5 ul

Template DNA (46ngr/1ul)……………………………….3 ul (138 ngr/50ul reaction)

High Fidelity PCR Enzyme Mix……………………..…0.6 ul

Water, nuclease-free……………………………….….35.4 ul

On the second day, I performed PCR with the same cycling protocol but I used from 7ul (322 ngr/50ul reaction) of Template DNA in this reaction (insted of 3ul) to obtain a stronger band. No Bands Were Observed.

Can you help me?

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