Gel Smearing & Faint Band Troubleshooter

Pain point

PCR products or ladders smear; bands are faint or absent; gels don't resolve expected sizes.

Repro/diagnostic steps

1. Run a ladder-only lane and a known-good sample to isolate gel system vs sample problems.
2. Confirm buffer type/concentration and gel % match target fragment size range.
3. Check loading amount and sample salt/contamination.

Root causes (common)

• Overloading DNA or high salt in samples.
• Degraded DNA or protein contamination.
• Wrong gel percentage or overheating during run.
• Old/mis-prepared buffer or staining artifacts.

Fix workflow

1. Make fresh buffer; verify correct dilution and polarity.
2. Reduce load, desalt/cleanup samples if necessary.
3. Adjust gel % and run voltage/time to reduce heat.
4. Validate with ladder-only run before committing critical samples.

Expected result

• Ladder resolves cleanly; samples show discrete bands at expected sizes.

References

• https://www.thermofisher.com/us/en/home/life-science/cloning/cloning-learning-center/invitrogen-school-of-molecular-biology/na-electrophoresis-education/na-electrophoresis-troubleshooting.html
• https://www.thermofisher.com/cl/en/home/technical-resources/technical-reference-library/nucleic-acid-purification-analysis-support-center/nucleic-acid-stains-ladders-markers-support/nucleic-acid-stains-ladders-markers-support-troubleshooting.html
• https://www.researchgate.net/post/What_troubleshooting_can_be_done_for_smeared_PCR_bands_in_gel_electrophoresis