Team:Arizona State/Experiments
Protocols
[1A] Polymerase Chain Reaction
PCR is used to rapidly amplify certain segments of DNA that are selected via designed primers. This protocol was used to accomplish a variety of goals, from extraction of parts from a cloning vector to the addition of restriction cut sites at the ends of parts.
- Defrost template, 2x Master Mix and primers
- Determine desired total working volume (~25uL)
- Label reaction tubes
- Create below reaction mix
- Place mixture in thermal cycler at settings shown below
| Part | Concentration | Volume for 25uL reaction |
|---|---|---|
| 2x Master Mix | 2x | 12.5uL |
| dsDNA Template | - | 1uL |
| Forward primer | - | 1uL |
| Reverse primer | - | 1uL |
| DI H2O | - | 9.5uL |
Sample Reaction
This is an example protocol used in the thermal cycler, durations and temperatures subject to change
| Step Name | # of Cycles | Temperature(℃) | Duration(min) |
|---|---|---|---|
| Initial | 1 | 98 | 3 |
| Denaturation | 30 | 98 | 0.5 |
| Annealing | 30 | 56 | 0.5 |
| Elongation | 30 | 72 | 0.5 |
| Final Elongation | 1 | 72 | 10 |
| Storage | 1 | 4 | ∞ |
[1B] PCR Cleanup
The Qiagen Qiaquick PCR cleanup kit was used to purify the thermal cycler product and remove remaining polymerases and nucleotides.
- Gather the solutions from the PCR cleanup kit
- Mix 5 times volume of Buffer PB with PCR reaction tube
- Add 10uL 3M sodium acetate
- Spin down the mixture in a QIAquick filter column at max speed for 60s. Discard flow-through and replace column into tube
- Add 750uL of Buffer PE to the mixture and spin down at max speed for 60s to wash. Discard flow-through and replace column
- Centrifuge the tube one more time to remove any remaining wash buffer
- Place column in clean 1.5mL plastic tube
- Add 30uL of Buffer EB to the column and let stand for 1min. Centrifuge at max speed for 1 min.
[2A] DNA Restriction Digest
- Gather DNA sample, digestion buffer, and restriction enzymes from cold storage
- Label tubes
- Create the below reaction mixture
- Place mixture in 37°C heat block for 10 minutes
| Component | Volume for 25uL reaction |
|---|---|
| DNA Sample | 15uL |
| 10x FastDigest Digestion Buffer | 2.5uL |
| Restriction Enzyme 1 | 1uL |
| Restriction Enzyme 2 | 1uL |
| DI H2O | 5.5uL |
[2B] Gel Verification/Extraction
- Make 1% gel by adding .6g of agarose to 60mL of 1x TAE buffer
- Swirl in glass flask and microwave for 40s
- Remove from microwave and swirl again. Microwave again for 40s
- Let cool until safe to touch. Add 6uL of SYBR safe red stain
- Pour mixture into gel mold with comb set up
- Fill gel electrophoresis apparatus with 1x TAE
- Remove comb from gel and submerge gel in apparatus
- Add 4uL of 1kb+ blue ladder to the first well
- Add samples mixed with loading dye to other wells
- Connect negative/positive ends to apparatus. Run at 110V
- Run for 30min-1hr. Remove and take to UV imager
- Photograph under UV light. If doing gel extraction, use scalpel to cut out blocks of gel containing desired bands
- Gel purify using Qiagen Gel Purification kit
- (If extracting)Use Nanodrop Spectrophotometer to measure DNA concentration
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