Wrong PCR program Forgot gel stain Forgot to turn the gel on Spilled the sample Not enough mastermix Too high voltage, gel liquified Frameshift mutation Too short elongation time Primer insertion Forgot template Wrong annealing temp Wrong salt/buffer concentration No band in the positive control Sample spillover into next lane Didn't mix properly Ran gel too long Didn't mix with sample buffer Prepared agarose gel with dH2O Forgot marker Multiple annealing sites Ran gel backwards Used protein marker as DNA ladder Wrong primers Band in the negative control Wrong PCR program Forgot gel stain Forgot to turn the gel on Spilled the sample Not enough mastermix Too high voltage, gel liquified Frameshift mutation Too short elongation time Primer insertion Forgot template Wrong annealing temp Wrong salt/buffer concentration No band in the positive control Sample spillover into next lane Didn't mix properly Ran gel too long Didn't mix with sample buffer Prepared agarose gel with dH2O Forgot marker Multiple annealing sites Ran gel backwards Used protein marker as DNA ladder Wrong primers Band in the negative control
(Print)
Wrong
PCR program
Forgot gel stain
Forgot to turn the gel on
Spilled the sample
Not enough mastermix
Too high voltage, gel liquified
Frameshift mutation
Too short elongation time
Primer insertion
Forgot template
Wrong annealing temp
Wrong
salt/buffer concentration
No band in the positive control
Sample spillover into next lane
Didn't mix properly
Ran gel too long
Didn't mix with sample buffer
Prepared agarose gel with dH2O
Forgot marker
Multiple annealing sites
Ran gel backwards
Used protein marker as DNA ladder
Wrong primers
Band in the negative control
