Guys, I REALLY NEED HELP

At the end of the last year I optimized every parameter of my RAPD-PCR, and as a result I did obtain great products multiple times. Then, I went home for my vacation (I wish I didn't) and now I'm back at the lab, and guess what? I CAN'T MAKE IT WORK AGAIN.

I already: changed PCR Buffer, dNTP, water, magnesium solution, changed the primer, re-patterned my DNA samples, autoclaved every tip and tube again, tried a different thermocycler...

DOES ANYONE HAVE ANY IDEA OF WHAT'S GOING ON?

I'll let all my conditions and a picture of my previus PCR results below:

Final concentrations in the mixer (13 uL) = 2,5 mM MgCl2, 1x PCR Buffer, 800 mM primer, 30ng DNA (total), 0,2 mM dNTP, 1U Taq.

PCR run:

Hot Start at 96°C for 3'

45 cycles of 92 °C for 1', 38 °C for 1', 72 °C for 2'. (already tried with 40 cycles)

Final extension at 72 °C for 5'.

Primers I'm currently using: OPC-05 (GATGACCGCC)

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