Wittrup: PCR: Difference between revisions

From OpenWetWare
Jump to navigationJump to search
No edit summary
No edit summary
 
(3 intermediate revisions by the same user not shown)
Line 1: Line 1:
'''Materials'''
'''Materials'''


Taq polymerase (usually 5 U per L) and 10X buffer
Taq polymerase (usually 5 U per 0.001 mL) and 10X buffer


MgCl2
MgCl2
Line 19: Line 19:
DMSO (optional)
DMSO (optional)


'''Mix the components of each 50 L reaction on ice:'''


reagent final concentration
'''Mix the components of each 0.050 mL reaction on ice:'''
10X buffer 1X
 
MgCl2 final concentration 1.5 to 2.5 mM
The final concentration of each of the reagents are as follows:
forward primer 0.5 uM
 
reverse primer 0.5 uM
10X buffer---------------1X
dNTP 10 mM each of dATP, dGTP, dTTP, dCTP
 
DNA template typically 10 ng
MgCl2--------------------final concentration 1.5 to 2.5 mM
water x L to 49 L final volume
 
Taq Polymerase 2.5 to 5 Unit
forward primer----------0.5 uM
 
reverse primer----------0.5 uM
 
dNTP---------------------10 mM each of dATP, dGTP, dTTP, dCTP
 
DNA template------------typically 10 ng
 
water----------------------add water to 0.049 mL volume
 
Taq Polymerase---------2.5 to 5 Unit (usually 0.001 mL)
 
 
The use of DMSO and betaine usually improve specificity of the annealing reaction. If the use of DMSO and betaine are desired, the final concentration of DMSO and betaine should be 3% (v/v) and 1 M.


DMSO and betaine tend to improve specificity of the annealing reaction. If the use of DMSO and betaine are desired, the final concentration of DMSO and betaine should be 3% (v/v) and 1 M.


Proceed with thermal cycling conditions outlined below:
Proceed with thermal cycling conditions outlined below:
Denature 1 min at 94 C
 
Anneal 1 min at the proper annealing temperature (depend on the primers)
Denature-------1 min at 94 degree Celsius
Extend 1 min for each 1 kb at 72 C
 
Anneal----------1 min at the proper annealing temperature (depend on the primers)
 
Extend----------1 min for each 1 kb at 72 degree Celsius
 
Repeat for 30 cycles (typical amplification)
Repeat for 30 cycles (typical amplification)
Final extension for 5 to 10 min at 72 C.
 
Final extension for 5 to 10 min at 72 degree Celsius.

Latest revision as of 13:41, 24 September 2006

Materials

Taq polymerase (usually 5 U per 0.001 mL) and 10X buffer

MgCl2

forward primer

reverse primer

DNA template

PCR grade water

dNTP mix or each of dATP, dCTP, dGTP, dTTP

2.5 M betaine (optional)

DMSO (optional)


Mix the components of each 0.050 mL reaction on ice:

The final concentration of each of the reagents are as follows:

10X buffer---------------1X

MgCl2--------------------final concentration 1.5 to 2.5 mM

forward primer----------0.5 uM

reverse primer----------0.5 uM

dNTP---------------------10 mM each of dATP, dGTP, dTTP, dCTP

DNA template------------typically 10 ng

water----------------------add water to 0.049 mL volume

Taq Polymerase---------2.5 to 5 Unit (usually 0.001 mL)


The use of DMSO and betaine usually improve specificity of the annealing reaction. If the use of DMSO and betaine are desired, the final concentration of DMSO and betaine should be 3% (v/v) and 1 M.


Proceed with thermal cycling conditions outlined below:

Denature-------1 min at 94 degree Celsius

Anneal----------1 min at the proper annealing temperature (depend on the primers)

Extend----------1 min for each 1 kb at 72 degree Celsius

Repeat for 30 cycles (typical amplification)

Final extension for 5 to 10 min at 72 degree Celsius.

Retrieved from "https://openwetware.org/mediawiki/index.php?title=Wittrup:_PCR&oldid=73249"