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PCR / RT-PCR Amplification Problems moderate

Excessive DNA Smearing on Gel

Symptom
Amplified DNA appears as broad smear rather than discrete bands, indicating degradation or over-amplification artifacts.
Common Causes
  1. 1 Excessive template concentration in reaction
  2. 2 Too many PCR cycles performed (>35 cycles)
  3. 3 Thermal cycling conditions not optimized for specific thermal cycler
  4. 4 Annealing temperature too low enabling promiscuous priming
  5. 5 Primer concentration too high
  6. 6 Extension time too long for target amplicon
  7. 7 Poor DNA template quality or degradation
  8. 8 Excessive DNA loaded on gel for electrophoresis
Solutions
  1. 1 Titrate template amount to optimal concentration for your system
  2. 2 Reduce number of cycles to below 35
  3. 3 Optimize cycling conditions based on thermal cycler manufacturer recommendations
  4. 4 When using Ready-To-Go Beads, re-optimize annealing temperature; increase by 2°C to 5°C increments
  5. 5 Titrate primer concentration to optimal level
  6. 6 Decrease extension time in small increments
  7. 7 Use freshly prepared DNA or isolate template by alternative purification method
  8. 8 Re-run gel electrophoresis with reduced sample loading volume
Related Video (3)
Addgene ★ 85
Polymerase Chain Reaction (PCR) Protocol
"Direct PCR protocol walkthrough showing proper template preparation and reaction setup to avoid excessive concentration issues"
Bilibili (China-Accessible Mirrors) ★ 82
First-person PCR and gel electrophoresis demonstration
"Hands-on PCR workflow with gel electrophoresis visualization demonstrates how smearing artifacts appear and proper band patterns"
Bilibili (China-Accessible Mirrors) ★ 78
PCR protocol fundamentals—hands-on operation guide
"Structured PCR protocol fundamentals with operational guidance covers reaction parameter control critical for preventing over-amplification"
Source: sigmaaldrich.com ↗
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