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Revision as of 13:11, 12 July 2012

PCR using Phusion DNA polymerase:

If this reaction is to be done from scratch, add the reagents in the order they are listed in the table. When multiple PCR experiments need to be run concurrently, everything that is not experiment specific (primers and template DNA) can be made up ahead of time as a master mix. In this case the master mix should be kept on ice as it contains enzymes. The primers and template DNA should be added to a PCR tube and the master mix added just before the sample is put in just before PCR begins.

Reagent	50 µl reaction	20 µl reaction	Final Concentration
H2O	Add to make 50 µl	Add to make 20 µl
5x Phusion buffer	10 µl	4 µl	1x
10 mM dNTPs	1 µl	0.4 µl	200 µM
Primer 1	x µl	x µl	0.5 µM
Primer 2	x µl	x µl	0.5 µM
Template DNA	x µl	x µl
Phusion DNA polymerase	0.5 µl	0.2 µl	0.02 u/ µl

N.B. The volume of primer that needs to be added will vary in accordance with the concentration of DNA in the initial sample

PCR machine settings:

		Temperature (oc)	Time (s)
Hold 1		95	360
Cycle (30x)	Denaturing	98	10
	Annealing	60	30
	Elongation	72	120

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