Bio-Rad DCode™ Universal Mutation Detection System User Manual

Buffer temperature does not

1. Use 50% ethylene glycol as chiller

coolant.reach set temperature

2. Insure that DCode temperature

controller is set at desired buffer
temperature.

3. Check that chiller is set to –20°C.

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 or power.

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 in wells. Do not

pierce or puncture wells.

PTT

“Smile effect”–band pattern curves

Decrease power setting, or fill lower chamber
upward at both sides of gelwith buffer up
to the "Max" setting on tank

Air bubbles in gel

Clean glass plates

Fuzzy DNA bands

1. Clean wells before use. Check for

matching comb thickness 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. Running buffer too concentrated.

Check buffer protocol.

4. Increase voltage or power.

Skewed or distorted bands

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.

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