Bio-Rad DCode™ Universal Mutation Detection System User Manual

Polyacrylamide gels are described by reference to two characteristics:

1) The total monomer concentration (%T)
2) The crosslinking monomer concentration (%C)

%T =

gm acrylamide + gm bis-acrylamide

x 100

Total Volume

%C =

gm bis-acrylamide

x 100

gm acrylamide + gm bis-acrylamide

50x TAE Buffer
Reagent

Amount Final

Concentration

Tris base

242.0 g

2 M

Acetic acid, glacial

57.1 ml

1 M

0.5 M EDTA, pH 8.0

100.0 ml

50 mM

dH

2

O

to 1,000.0 ml

Mix. Autoclave for 20–30 minutes. Store at room temperature.

The table below provides the percentage acrylamide/bis needed for a particular size range.

Gel Percentage

Base Pair Separation

6%

300–1000 bp

8%

200–400 bp

10%

100–300 bp

0% Denaturing Solution

6% Gel

8% Gel

10% Gel

12% Gel
40% Acrylamide/Bis

15 ml

20 ml

25 ml

30 ml

50x TAE buffer

2 ml

2 ml

2 ml

2 ml

dH

2

O

83 ml

78 ml

73 ml

68 ml

Total volume

100 ml

100 ml

100 ml

100 ml

Degas for 10–15 minutes. Filter through a 0.45 µ filter. Store at 4°C in a brown bottle for
approximately 1 month.

100% Denaturing Solution

6% Gel

8% Gel

10% Gel

12% Gel

40% Acrylamide/Bis

15 ml

20 ml

25 ml

30 ml

50x TAE buffer

2 ml

2 ml

2 ml

2 ml

Formamide (deionized)

40 ml

40 ml

40 ml

40 ml

Urea

42 g

42 g

42 g

42 g

dH

2

O

to 100 ml

to 100 ml

to 100 ml

to 100 ml

Degas for 10–15 minutes. Filter through a 0.45 µ filter. Store at 4°C in a brown bottle for
approximately 1 month. A 100% denaturant solution requires re-dissolving after storage. Place
the bottle in a warm bath and stir for faster results.

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