Bio-Rad DCode™ Universal Mutation Detection System User Manual

DNA leaks between wells

1. Acrylamide not polymerized. Add more

TEMED and ammonium persulfate to
final concentration of 0.1%.

2. Degas acrylamide solution before

casting gel.

3. Let gel polymerize for at least 60 minutes.
4. Do not overload sample well. Reduce

sample volume.

Skewed or distorted bands,

1. Impurities in acrylamide. Filter before

use. or DNA spikes in gel

Check shelf life date of acrylamide.

2. Carefully load DNA into wells. Do not

pierce or puncture wells.

Heteroduplex Analysis

Normal and mutant

1. Optimize concentration of DEM.

DNA unresolved

2. Add 15% urea to gel.
3. Adjust voltage or run time so that

samples travel at least 15 cm from well.

Air bubbles in gel

Clean glass plates

Fuzzy DNA bands

1. Clean wells before use. Check for

matching comb and spacer thickness.

2. Let gel polymerize for at least 60 minutes.

Bands did not migrate far

1. Increase run time.

enough into gel

2. Decrease acrylamide concentration.
3. Increase voltage.

DNA leaks between wells

1. Acrylamide not polymerized. Add more

TEMED and ammonium persulfate to
final concentration of 0.1%.

2. Degas acrylamide solution before casting

gel.

3. Let gel polymerize for at least 60 minutes.
4. Do not overload sample well. Reduce

sample volume.

Skewed or distorted bands,

1. Impurities in acrylamide. Filter before

or DNA spikes in gel

use. Check shelf life date of
acrylamide.

2. Carefully load DNA in wells. Do not

pierce or puncture the wells.

SSCP

Normal and mutant

1. Optimize running temperature.

DNA unresolved

2. Add 5–10% glycerol to gel.
3. Reduce crosslinking of acrylamide and

bis.

4. Use different concentration of buffer.

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