Home Failure Case Library Sequence Errors at PCR Product Termini
PCR (Invitrogen Guide) moderate

Sequence Errors at PCR Product Termini

Symptom
Sequencing shows errors, truncations, or unexpected sequences specifically at the 5′ or 3′ ends of amplified products.
Common Causes
  1. 1 Primer design with direct repeats causing sequence misalignment at product ends
  2. 2 Low primer quality with non-full-length oligos truncated at 5′ ends
  3. 3 Contaminating nucleases or exonucleases degrading product termini
  4. 4 UV damage from gel visualization
Solutions
  1. 1 Avoid direct repeats within primer sequences to prevent misalignment at PCR product ends
  2. 2 Order PCR primers with purification to remove truncated non-full-length oligos
  3. 3 Use molecular-grade, nuclease-free reagents; set up reactions on ice to minimize exonuclease activity
  4. 4 Use long-wavelength UV (360 nm) with limited exposure or longer-wavelength excitation dyes
  5. 5 Sequence both DNA strands with duplicate samples to confirm reliability
Related Video (2)
YouTube (Curated Tutorials) ★ 92
Primer Design: Important Considerations and Tips for Good Primer Design
"Directly addresses primer design considerations and tips, which is the root cause of the failure case involving primer-induced sequence errors at product termini"
Addgene ★ 85
How to Design Primers for PCR
"Teaches primer design fundamentals for PCR, enabling researchers to recognize and avoid direct repeats and misalignment issues that cause terminal sequence errors"
Source: thermofisher.com ↗
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