Melbourne/Transformation Protocol
From 2007.igem.org
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*Applications: | *Applications: | ||
*#Amplification of Biobrick DNA for storage and use. | *#Amplification of Biobrick DNA for storage and use. | ||
- | *#Selection | + | *#Selection and amplification of ligated constructs. |
*Time to complete protocol: | *Time to complete protocol: | ||
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====Method from primary and secondary reagents==== | ====Method from primary and secondary reagents==== | ||
=====Primary & secondary Reagents Required including controls===== | =====Primary & secondary Reagents Required including controls===== | ||
- | *Competent cells | + | *[[Melbourne DH5a|Competent cells]] (from -70degree freezer) |
*DNA for transformation | *DNA for transformation | ||
- | *LB | + | *[[Melbourne/Secondary Reagent LB|LB]] (cupboard) |
- | *LB-agar plates with selective antibiotic | + | *[[Melbourne/Secondary Reagent Agar Plates|LB-agar plates]] with selective antibiotic (cool room) |
=====Method including controls===== | =====Method including controls===== | ||
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#Heat shock in water bath at 42 degrees for 1min. | #Heat shock in water bath at 42 degrees for 1min. | ||
#Incubate on ice for 15min. | #Incubate on ice for 15min. | ||
- | #Add 1mL LB. | + | #Add 1mL LB (flame tip before use). |
- | #Incubate at | + | #Incubate at 37 degrees for 1 hour. |
#Spin down cells and remove majority of LB. | #Spin down cells and remove majority of LB. | ||
#Resuspend cells in remaining LB. | #Resuspend cells in remaining LB. | ||
Line 28: | Line 28: | ||
#Incubate plate overnight at 37 degrees. | #Incubate plate overnight at 37 degrees. | ||
#Place in cold room until needed. | #Place in cold room until needed. | ||
+ | |||
=====Equipement Required===== | =====Equipement Required===== | ||
- | *1. | + | *[[Melbourne/1.7ml microcentrifuge|microcentrifuge: 1.7ml]] |
*Ice box | *Ice box | ||
*Pipettes | *Pipettes | ||
- | *42 degree water bath | + | *42 degree water bath (balance room) |
- | *37 degree incubator | + | *37 degree incubator |
*Bunsen burner | *Bunsen burner | ||
*Spreader | *Spreader | ||
+ | *[[Melbourne/primary ice|ice]] | ||
+ | |||
=====References===== | =====References===== | ||
* | * |
Latest revision as of 11:06, 29 September 2007
<Return to list of protocols> <Team home page>
- Applications:
- Amplification of Biobrick DNA for storage and use.
- Selection and amplification of ligated constructs.
- Time to complete protocol:
- Lab time: 10min, 10min, 10min, 15min.
- Waiting time: 45min, 15min, 1hour, overnight.
- Approximate cost of materials: $
Method from primary and secondary reagents
Primary & secondary Reagents Required including controls
- Competent cells (from -70degree freezer)
- DNA for transformation
- LB (cupboard)
- LB-agar plates with selective antibiotic (cool room)
Method including controls
- Add 1uL resuspended plasmid DNA to 50uL competent cells.
- Incubate on ice for 45min.
- Heat shock in water bath at 42 degrees for 1min.
- Incubate on ice for 15min.
- Add 1mL LB (flame tip before use).
- Incubate at 37 degrees for 1 hour.
- Spin down cells and remove majority of LB.
- Resuspend cells in remaining LB.
- Under a bunsen spread resuspended bacteria on agar plate on selective antibiotic.
- Incubate plate overnight at 37 degrees.
- Place in cold room until needed.
Equipement Required
- microcentrifuge: 1.7ml
- Ice box
- Pipettes
- 42 degree water bath (balance room)
- 37 degree incubator
- Bunsen burner
- Spreader
- ice
References