Team:Caltech/Recipes
From 2011.igem.org
(Difference between revisions)
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[[Team:Caltech/Notebook|Back to Timeline]] . [[Team:Caltech/Protocols|Back to Methods]]<br/><br/> | [[Team:Caltech/Notebook|Back to Timeline]] . [[Team:Caltech/Protocols|Back to Methods]]<br/><br/> | ||
- | + | ==50% glycerol Stock:== | |
* 50 mL glycerol | * 50 mL glycerol | ||
* 50 mL nanopure water | * 50 mL nanopure water | ||
<br/> | <br/> | ||
- | + | ==Agar/LB plate (Autoclaved):== | |
* 1 L nanopure water | * 1 L nanopure water | ||
* 10 g tryptone | * 10 g tryptone | ||
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<br/> | <br/> | ||
- | + | ==Ampicillin Stock== | |
*Mass out amount needed for 50 mg/ml or 100 mg/ml stock of ampicillin trihydrate | *Mass out amount needed for 50 mg/ml or 100 mg/ml stock of ampicillin trihydrate | ||
*Add a small amount of nanopure water | *Add a small amount of nanopure water | ||
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<br/> | <br/> | ||
- | + | ==Chloramphenicol Stock== | |
*for 25 mg/ml stock solution (usually, chloramphenicol is used at 12.5 µg/ml or 25 µg/ml) | *for 25 mg/ml stock solution (usually, chloramphenicol is used at 12.5 µg/ml or 25 µg/ml) | ||
*add 250 mg chloramphenicol to 10 ml 100% ethanol | *add 250 mg chloramphenicol to 10 ml 100% ethanol | ||
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<br/> | <br/> | ||
- | + | ==Enrichment Minimal Media== | |
* 1.0712 g K2 HPO4 | * 1.0712 g K2 HPO4 | ||
* 0.5239 g KH2 PO4 | * 0.5239 g KH2 PO4 | ||
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<br/> | <br/> | ||
- | + | ==Gibson Mix (1.33x)== | |
For 25 aliquots of 15 μl each: | For 25 aliquots of 15 μl each: | ||
* 50 μl of Taq Ligase | * 50 μl of Taq Ligase | ||
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* (375 μl total) <br/><br/> | * (375 μl total) <br/><br/> | ||
- | + | ==IPTG stock== | |
For 1000x stock (.1M) | For 1000x stock (.1M) | ||
*.0238 g IPTG | *.0238 g IPTG | ||
*1 mL sterile water<br/><br/> | *1 mL sterile water<br/><br/> | ||
- | + | ==Ligation Reaction== | |
for 20 uL rxn | for 20 uL rxn | ||
*2 uL T4 buffer | *2 uL T4 buffer | ||
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Total of between 50 and 100ng DNA<br/><br/> | Total of between 50 and 100ng DNA<br/><br/> | ||
- | + | ==p450 degradation testing solution== | |
For a 200uL reaction: | For a 200uL reaction: | ||
*2mM substrate | *2mM substrate | ||
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*buffer<br/><br/> | *buffer<br/><br/> | ||
- | + | ==Phusion PCR== | |
For a 50uL reaction: | For a 50uL reaction: | ||
* 1 uL template DNA | * 1 uL template DNA | ||
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* 25 uL Phusion master mix<br/><br/> | * 25 uL Phusion master mix<br/><br/> | ||
- | + | ==SOC Media== | |
for 250 ml (adapted from [http://openwetware.org/wiki/SOC OpenWetWare]) | for 250 ml (adapted from [http://openwetware.org/wiki/SOC OpenWetWare]) | ||
*1.25 g yeast extract | *1.25 g yeast extract | ||
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*after cooling below 50°C, add 5 mL filter-sterilized 20% glucose solution.<br/><br/> | *after cooling below 50°C, add 5 mL filter-sterilized 20% glucose solution.<br/><br/> | ||
- | + | ==Restriction Digest== | |
for 50uL rxn | for 50uL rxn | ||
*as much DNA as needed | *as much DNA as needed | ||
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*1 uL restriction enzyme each<br/><br/> | *1 uL restriction enzyme each<br/><br/> | ||
- | + | ==Taq PCR (for 16s insert)== | |
For a 25uL reaction: | For a 25uL reaction: | ||
*sterile water: 19.8uL | *sterile water: 19.8uL | ||
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<br/> | <br/> | ||
- | + | ==X-gal stock (50x)== | |
For 20mg/mL, total 0.5mL volume: | For 20mg/mL, total 0.5mL volume: | ||
*10mg X-gal | *10mg X-gal | ||
*0.5mL DMSO<br/>}} | *0.5mL DMSO<br/>}} |
Revision as of 10:46, 17 September 2011
Project |
Back to Timeline . Back to Methods 50% glycerol Stock:
Agar/LB plate (Autoclaved):
Ampicillin Stock
Chloramphenicol Stock
Enrichment Minimal Media
Gibson Mix (1.33x)For 25 aliquots of 15 μl each:
IPTG stockFor 1000x stock (.1M)
Ligation Reactionfor 20 uL rxn
H&subO make up to 20 uL p450 degradation testing solutionFor a 200uL reaction:
Phusion PCRFor a 50uL reaction:
SOC Mediafor 250 ml (adapted from [http://openwetware.org/wiki/SOC OpenWetWare])
Restriction Digestfor 50uL rxn
Taq PCR (for 16s insert)For a 25uL reaction:
X-gal stock (50x)For 20mg/mL, total 0.5mL volume:
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