Bio-Rad DCode™ Universal Mutation Detection System User Manual

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Fig. 4.15. Constant denaturing gel. Amplified mutant and wild-type alleles of exon 8 from the p53 gene.
Separation by CDGE run at 130 V for 2.5 hours on a 10% acrylamide gel in 51% denaturant at 56 °C. Lane 1, mutant
allele; lane 2, wild-type allele; lane 3, mutant and wild-type allele.

Reagent Preparation

The concentration of denaturant is determined from a perpendicular or parallel DGGE

gel. The concentration of acrylamide may vary, depending on the size of the fragment that is
being analyzed. Both 0% and 100% denaturant should be made as stock solutions. A 100%
denaturant is a mixture of 7 M urea and 40% deionized formamide. Reagents for casting and
running CDGE gels are included in the DCode electrophoresis reagent kit for DGGE/CDGE,
catalog number 170-9032.

For different percent crosslinking, use the equation below to determine the amount of Bis

to add. The example stock solution below is for an acrylamide/bis ratio of 37.5:1.

40% Acrylamide/Bis (37.5:1)
Reagent

Amount

Acrylamide

38.93 g

Bis-acrylamide

1.07 g

dH

2

O

to 100.0 ml

Filter through a 0.45 µ filter and store at 4°C.

For different percent crosslinking, use the equation below to determine the amount of Bis

to add. The example stock solution is for an acrylamide/bis ratio of 37.5:1.

Polyacrylamide gels are described by reference to two characteristics:

1) Total monomer concentration (%T)
2) Crosslinking monomer concentration (%C)

%T =

gm acrylamide + g bis-acrylamide

x 100

total volume

%C =

gm bis-acrylamide

x 100

gm acrylamide + g bis-acrylamide

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