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Team:Caltech/Protocols
From 2011.igem.org
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and then add 5 mg of whatever chemical used in two flasks, one with vitamins and one without. | and then add 5 mg of whatever chemical used in two flasks, one with vitamins and one without. | ||
| - | Transforming DNA Protocol: | + | <p>Transforming DNA Protocol: |
1) Thaw competent cells on ice: 15K, 15J, 15O, 15M. | 1) Thaw competent cells on ice: 15K, 15J, 15O, 15M. | ||
2) Get 10 micro Liters of pure water. | 2) Get 10 micro Liters of pure water. | ||
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9) Heat Shock for 45 sec by using a water bath set to 42°C and then thawing on ice for 2 min. | 9) Heat Shock for 45 sec by using a water bath set to 42°C and then thawing on ice for 2 min. | ||
10)Pipette 500 micro Liters of S.O.C. (LB + glucose) into each competent cell tubes. | 10)Pipette 500 micro Liters of S.O.C. (LB + glucose) into each competent cell tubes. | ||
| - | (STILL CONFUSED ABOUT THIS PROTOCOL NOT SURE IF RIGHT) | + | (STILL CONFUSED ABOUT THIS PROTOCOL NOT SURE IF RIGHT)</p> |
| - | Making Plates: | + | <p>Making Plates: |
1) Fill the bottom of plate with the LB/Agar solution. | 1) Fill the bottom of plate with the LB/Agar solution. | ||
2) Add 100 mg/mL of antibiotics into the plate. | 2) Add 100 mg/mL of antibiotics into the plate. | ||
| - | 3) Shake gently. | + | 3) Shake gently.</p> |
Putting 100 mg soil into each tube, shake | Putting 100 mg soil into each tube, shake | ||
| - | Starter Competent Cell Culture Recipe? | + | <p>Starter Competent Cell Culture Recipe? |
- Take the competent cell tubes out of the freezer. | - Take the competent cell tubes out of the freezer. | ||
- Vortex it and take 100 micro Liters from it and pipette it into the labeled plates. | - Vortex it and take 100 micro Liters from it and pipette it into the labeled plates. | ||
- Put in some beads and shake gently. | - Put in some beads and shake gently. | ||
| - | - Put the dirty beads away in the dirty bead container. | + | - Put the dirty beads away in the dirty bead container.</p> |
Revision as of 06:39, 21 June 2011
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Project |
Recipe for Agar/LB plate: 1) Fill two bottles with 500 g of nanopure water, 10 g of Tryptone, 10 g of NaCl, 5 g of yeast extract, and 15 g of Agar. 2) Shake and then autoclave.Recipe for 50% Glycerol Stock: 1) Pour 50 mL of Glycerol and 50 mL of pure water into a graduated cylinder. 2) Cover with parafilm and turn over a couple of times to mix. 3) Use the Nalgene vacuum to sterilize the stock. 4) Use the bunsen burner to keep air sterile and close the cap. Recipe for Enrichment Minimal Media consists of
and then add 5 mg of whatever chemical used in two flasks, one with vitamins and one without. Transforming DNA Protocol: 1) Thaw competent cells on ice: 15K, 15J, 15O, 15M. 2) Get 10 micro Liters of pure water. 3) Pipette out DNA from the source plate and put it in the appropriate tubes. 4) Flick the competent cells in the tube gently. 5) Pipette 40 micro Liters of competent cells into the DNA. 6) Pipette 2 micro Liters of the DNA and put it in the competent cell tubes. 7) Stir a but. 8) Leave on ice for 30 minutes. 9) Heat Shock for 45 sec by using a water bath set to 42°C and then thawing on ice for 2 min. 10)Pipette 500 micro Liters of S.O.C. (LB + glucose) into each competent cell tubes. (STILL CONFUSED ABOUT THIS PROTOCOL NOT SURE IF RIGHT) Making Plates: 1) Fill the bottom of plate with the LB/Agar solution. 2) Add 100 mg/mL of antibiotics into the plate. 3) Shake gently. Putting 100 mg soil into each tube, shake Starter Competent Cell Culture Recipe? - Take the competent cell tubes out of the freezer. - Vortex it and take 100 micro Liters from it and pipette it into the labeled plates. - Put in some beads and shake gently. - Put the dirty beads away in the dirty bead container.
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