No PCR product is obtained despite correct thermal cycling and component concentrations. Investigation reveals potential primer-related issues including design flaws or contamination.
Common Causes
1Primers designed or synthesized incorrectly; sequence not complementary to template
2Primers contain repetitive sequences, high self-complementarity, or regions that amplify pseudogenes
3Primer Tm calculated incorrectly due to wrong salt concentration or primer concentration assumptions
4Primers contain impurities or contaminants that inhibit PCR
5Target sequence too long for current PCR conditions and component concentrations
Solutions
1Verify primers have correct sequence and are complementary to template; resynthesize if needed
2Use primer design program to avoid repetitive sequences and high complementarity; perform BLAST search to avoid pseudogene amplification
3Calculate primer Tm using oligocalc tool with default salt concentration and 0.2–1 µM primer concentration; use lowest Tm for annealing temperature calculation
4Use desalted or more highly purified primers; test dilution to determine inhibitory effects (maintain >0.02 µM minimum)
5For long targets, reoptimize protocol and increase extension step duration; consider nested PCR approach