IGEM:Harvard/2006/Folding DNA nanostructures
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- working stocks
- 44 nM scaffold (20 μL)
- 0.99 μM each oligo
- goal
- 10 nM scaffold
- 100 nM each oligo
- 20 μL reaction volume
- calculations
- scaffold = (10 nM)/(44 nM) * 20 μL = 4.5 μL
- oligos = (100 nM)/(990 nM) * 20 μL = 2 μL
- reaction mixture
- 4.5 μL p7308 scaffold (44 nM)
- 2 μL oligos (990 nM)
- 2 μL 10x folding buffer (500 mM HEPES pH 7.5, 500 mM NaCl, 100 mM MgCl2)
- 11.5 μL dH2O
- annealing protocol
- 90[[:Category:{{{1}}}|{{{1}}}]] 5' → 65[[:Category:{{{1}}}|{{{1}}}]] 20' → 55[[:Category:{{{1}}}|{{{1}}}]] 20' → 45[[:Category:{{{1}}}|{{{1}}}]] 20' → 37[[:Category:{{{1}}}|{{{1}}}]] 30'
Gel Analysis
- Run 1% agarose gel, supplemented to 10 mM MgCl2
- Run at low voltage (80V) for 1.5 hours
| Lane | Contents | Loading Buffer |
| 0 | 1kb DNA ladder (10 μL) | 10x loading dye (1.1 μL) |
| 1 | control: +scaffold -oligos (10 μL) | 10x loading dye (1.1 μL) |
| 2 | control: -scaffold +oligos (10 μL) | 10x loading dye (1.1 μL) |
| 3 | folded nanotubes (10 μL) | 10x loading dye (1.1 μL) |
