Home Failure Case Library Insufficient Amplification from Polymerase Issues
PCR (Invitrogen Guide) severe

Insufficient Amplification from Polymerase Issues

Symptom
Weak or absent PCR product. Primers are degraded or show primer-dimer formation at the bottom of gel.
Common Causes
  1. 1 Proofreading polymerase 3′→5′ exonuclease activity degrading primers at room temperature
  2. 2 Insufficient DNA polymerase quantity for reaction requirements
  3. 3 Low Mg2+ concentration inadequate for polymerase activity
  4. 4 Excess PCR additives (DMSO, formamide) requiring more enzyme
Solutions
  1. 1 Use hot-start DNA polymerases to prevent primer degradation; alternatively set up PCR on ice or add polymerase last
  2. 2 Increase DNA polymerase amount per manufacturer recommendations, especially with high additive concentrations
  3. 3 Optimize Mg2+ concentration for maximum yield; increase if EDTA or high dNTPs present
  4. 4 Check polymerase preference for MgSO4 vs MgCl2 (e.g., Pfu works better with MgSO4)
  5. 5 Use lowest possible concentration of additives; adjust annealing temperature accordingly
Related Video (2)
Addgene ★ 82
Polymerase Chain Reaction (PCR) Protocol
"Core PCR protocol demonstration showing standard polymerase setup and execution steps where polymerase selection and primer handling directly impact success."
YouTube (Curated Tutorials) ★ 78
Primer Design: Important Considerations and Tips for Good Primer Design
"Dedicated primer design tutorial addressing primer quality and design considerations, directly relevant to understanding how degraded/poorly designed primers cause amplification failure."
Source: thermofisher.com ↗
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