From 2014.igem.org
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Methods and Protocols |
Project |
Miniprep
We used QIAGEN's miniprep reagents and protocol.
- Pellet cells at 4000 rpm, 4C for 12 minutes
- Resuspend cells with 200ul buffer P1, transfer to microcentrifuge
- Add 200 ul lysis buffer P2, cap and shake. Do not allow reaction to continue for more than 5 minutes.
- Add 300 ul Neutralization buffer N3, cap and shake.
- Pellet cells at 13000 rpm for 10 minutes with tabletop centrifuge.
- Apply supernatant to spin column.
- Centrifuge for 60s. Discard flow through.
- Add 750 ul wash buffer PE to column.
- Centrifuge for one minute. Discard flow through.
- Centrifuge again for one minute to get rid of excess wash buffer.
- Transfer column to microcentrifuge tube. Add 50 ul elution solution EB to the column, let stand for 1-5 minutes.
- Centrifuge for 60s. Determine concentration of DNA product and store at -20C
Gel Extraction
We used QIAGEN's Gell extraction protocol and reagents.
- Use razor to excise gel slice containing desired DNA.
- Slice this gel finely and place in a microcentrifuge tube.
- Add 750 ul QG buffer to tube.
- Incubate at 50C while shaking tubes at 500 rpm. You may need to vortex the tubes occasionally. Continue until the gell has completely dissolved. This is usually around 10 min.
- Add something
Transformation Protocol
- Thaw competent cells on ice.
- To a microcentrifuge tube, add 50ul cells if using homestock, 25ul if using commercial cells.
- Add 1-2 ul of desired DNA.
- Incubate on ice for 30 min.
- Heat shock at 42C for 30 sec.
- Ice shock cells for 2 min.
- Add 450 ul SOC broth media.
- Incubate at 30C while shaking at 300 rpm for 60 min.
- Incubate appropriate antibiotic plates at 37C.
- Plate cells. Incubate overnight at 37C.
Dinosaur
This is a dinosaur!!
Some Other Protocol
Well, aren't we interesting
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