DNA SEQUENCING(SANGER)
1. For double-stranded DNA templates:
a. Denature template: 10ml DNA (5-10g or alkaline lysis mini prepDNA)
8ml ddH2 O 2ml 2N NaOH -incubate 30' at 37℃.
b. Dry-ice precipitate: 10ml 4M NH4 OAc
100ml EtOH -70% EtOH wash -vacuum dry briefly -resuspend in 7ml ddH2 O
2. Annealing reaction:7ml template
2ml Sequenase reaction buffer 1ml primer (2-3pmol T3, T7, etc.) -incubate 10' at 65℃ -remove the entire heat block to RT and cool slowly to <30℃ -chill on ice for use in Step 7.
3. While cooling, pipet 2.5ml of each Termination Mix into a 96-well microtiter dish. Use red- capped tubes for dGTP rxns or orange-capped tubes for dITP rxns. Cover the dish with sealing tape and set aside for Steps 6 & 8.
4. Dilute Labeling Mix (green-capped dGTP) 1:5 to working concentration with ddH2 O.
5. Dilute Sequenase Version 2.0 1:8 with ice-cold Enzyme Dilution Buffer.
6. Prewarm termination mixes from Step 3 in the 37℃ bath.
7. Labeling reaction: 10ml annealing reaction (Step 2)
1.0ml 0.1M DTT 2.0ml Diluted Labeling Mix 0.5ml [35S]dATP 2.0ml Diluted Sequenase -mix and incubate 2-5' at RT.
8. Termination reaction: Transfer 3.5ml of the labeling rxn to each termination well, mix and incubate 5' at 37℃.
9. Stop rxns by adding 4ml Stop Solution.
10. Heat samples for 3-5' at 90-100℃ just prior to loading.