Gel electrophoresis reveals multiple bands, smearing, or bands at incorrect sizes in addition to or instead of the expected product, indicating lack of amplification specificity.
Common Causes
1Premature replication at low temperatures before denaturation due to non-hot-start polymerase
2Annealing temperature too low allowing non-specific primer binding
4Poor primer design with self-complementarity, primer-dimers, or GC-rich 3' ends
5Excessive primer concentration (>1 µM) promoting non-specific amplification
6Contamination with exogenous DNA from aerosols or previous reactions
7Incorrect template concentration: too high causing non-specific priming
Solutions
1Use hot-start polymerase such as OneTaq Hot Start DNA Polymerase; set up reactions on ice with chilled components and add to thermocycler preheated to denaturation temperature
2Increase annealing temperature in 1–2°C increments up to 5°C above calculated Tm
3Optimize Mg²⁺ concentration by testing 0.2–1 mM increments