SOE PCR (Splicing by Overlap-Extension)

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Revision as of 13:21, 10 August 2023 by EricMiller (talk | contribs) (Created page with "Eventually, a 50ul PCR. * 5x GC buffer (or whichever PCR buffer used): 10ul * Templates: Up to 100ng of largest fragment ** Equivalent molarity for all other fragments * dNTPs: 1ul * Water:To 47.5ul * Phusion: 0.5ul * PCR for 15 cycles "using the annealing temperature of the homologous regions". * Extension time: use the length of the (n-1) longest fragments, where n is the total number of fragments * Immediately after these 15 cycles: ** Add 1ul each of outside prime...")

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Eventually, a 50ul PCR.

5x GC buffer (or whichever PCR buffer used): 10ul
Templates: Up to 100ng of largest fragment
- Equivalent molarity for all other fragments
dNTPs: 1ul
Water:To 47.5ul
Phusion: 0.5ul

PCR for 15 cycles "using the annealing temperature of the homologous regions".
Extension time: use the length of the (n-1) longest fragments, where n is the total number of fragments

Immediately after these 15 cycles:
- Add 1ul each of outside primers direct to the PCR tube
- PCR for 30 cycles, using annealing temperature matching your flanking primers; extension time: use the total length of the construct

Run 2ul on a gel. Gel purify ending result if needed.
- Your product will probably be a minority in a mix of DNA!

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