EMSA using ds Oligonucleotides【Harvard University】
互联网
Cepko/Tabin Lab ,Harvard University http://axon.med.harvard.edu/~cepko/protocol/mike/E1.html Cepko/Tabin Lab ,Harvard University http://axon.med.harvard.edu/~cepko/protocol/mike/E1.html Solutions
10X Annealing Buffer
200 mM Tris 8.0 200 ml 1M Tris pH 8.0 ml .5M EDTA pH 8.0 ml 5M NaCl ml Q store at room temperature
10X Klenow Buffer
500 mM Tris 7.5 500
100 mM MgCl2
ml 1M Tris pH 7.5 2 100 ml 1M MgCl2
10 mM DTT 20
0.5
330
ml 0.5 M DTT m g/ ml BSA 50 ml 10 mg/ml BSA (NEB)ml Q store at -80℃ in 50 ml aliq.
2X Binding Buffer (ref: Gutman et al.GENE 110,1992 pg 197)
20% glycerol 400
20 mM Tris 7.5 20
100 mM KCl 100
1 mM DTT 2
478
ml 50% glycerol ml 1M Tris pH 7.5 ml 1M KCl ml 0.5 M DTT ml Q make fresh as needed
Poly dI/dC
Make a 1
Procedure
• Design complementary oligonucleotides with compatible half sites on the ends (I use BamHI and BglII).Dry down 300 ng of the two purified oligos together and resuspend in 9
• Mix the following and incubate at room temperature for 30 min:
1
5
25
dGTP)
5
14
1
Bring up to 200 microliters with TE,phenol/chloroform extract and ethanol precipitate with 0.1 volume of 3 M NaOAc pH 5.2 as well as tRNA .Dry and resuspend in 100
• Generate a table of binding reaction parameters and competitor concentrations.Prepare the gel and running buffer.
EMSA Gel:
8 ml 30% acrylamide (0.8% BIS)
6 ml 50% glycerol
6 ml 10X TBE
40 ml Q
180
Cool to 4℃ along with the appropriate amount of 1X TBE.
• Mix the binding reagents in the following order:
i)10
ii)3
iii)Q to 20
iv)competitor at 10-20X excess
