No visible band or very faint band on gel despite proper thermal cycling parameters. The reaction components may be at suboptimal or inhibitory concentrations.
Common Causes
1dNTP concentration incorrect (too high causes Mg2+ depletion; too low causes insufficient nucleotides)
2Mg2+ concentration insufficient or omitted (1.5 mM required in final reaction)
3Primer concentration incorrect (too high increases nonspecific binding; too low causes inefficient annealing; use 0.2–1 µM)
4Enzyme concentration too low (incomplete replication) or enzyme omitted/inactive
5Template amount insufficient or template omitted
Solutions
1Each dNTP should be present at 200 µM in final reaction; verify concentration to avoid Mg2+ depletion
2Use 1.5 mM Mg2+ in final reaction; ensure component is not omitted
3Use well-designed primers at 0.2–1 µM in final reaction; verify correct concentration supplied by manufacturer; do not use less than 0.02 µM
4Use adequate units of enzyme matching template length/difficulty; if enzyme suspected inactive, run PCR with fresh polymerase from different batch
5Increase template amount or increase cycles in increments of 5; add template if omitted; verify template is present and undamaged