Team:Wash U/French/Protocol
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'''Procedure''' | '''Procedure''' | ||
:list of steps | :list of steps | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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:Note: Restriction sites E=EcoR1-HF; X=Xba1; S=Spe1; P=Pst1; M=Mixed Site | :Note: Restriction sites E=EcoR1-HF; X=Xba1; S=Spe1; P=Pst1; M=Mixed Site | ||
:To view the full BioBrick Manual procedures, please click [http://partsregistry.org/Help:Transformation_Protocol here]. | :To view the full BioBrick Manual procedures, please click [http://partsregistry.org/Help:Transformation_Protocol here]. | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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'''Procedures''' | '''Procedures''' | ||
:List of Procedures | :List of Procedures | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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# Ligate the products. The result will be the upstream part connected to the downstream part in the destination plasmid. This new composite part can then be used to transform competent cells. | # Ligate the products. The result will be the upstream part connected to the downstream part in the destination plasmid. This new composite part can then be used to transform competent cells. | ||
:To view the full Biobrick Assembly manual, please click [http://ginkgobioworks.com/support/ here]. | :To view the full Biobrick Assembly manual, please click [http://ginkgobioworks.com/support/ here]. | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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# Transfer the tubes to an incubator set at 80C for another 20 minutes. This step will deactivate the restriction enzymes. | # Transfer the tubes to an incubator set at 80C for another 20 minutes. This step will deactivate the restriction enzymes. | ||
# Digestion is now finished and products should be stored at -20C. | # Digestion is now finished and products should be stored at -20C. | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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# Let the mix stand for 10 minutes at room temperature before incubating at 80C for 20 minutes (deactivates enzymes). | # Let the mix stand for 10 minutes at room temperature before incubating at 80C for 20 minutes (deactivates enzymes). | ||
# Store the products at -20C until they are needed for a transformation. | # Store the products at -20C until they are needed for a transformation. | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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'''Procedures''' | '''Procedures''' | ||
:text | :text | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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:Note:Expected yields are 4 umol PCB per 6g Spirulina | :Note:Expected yields are 4 umol PCB per 6g Spirulina | ||
:Thanks to Dr. Clark Lagarias for providing this protocol. [[Team:Wash_U/Project#References|ref]] | :Thanks to Dr. Clark Lagarias for providing this protocol. [[Team:Wash_U/Project#References|ref]] | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] |
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<font size="4"> | <font size="4"> | ||
=='''Glycerol Stock Solution'''== | =='''Glycerol Stock Solution'''== | ||
<font size="2"> | <font size="2"> | ||
'''Matériaux''' | '''Matériaux''' | ||
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# Centrifuge/screw top tubes | # Centrifuge/screw top tubes | ||
# 50% glycerol sol | # 50% glycerol sol | ||
# LB Cultures | # LB Cultures | ||
- | |||
'''Procedures''' | '''Procedures''' | ||
# Label centrifuge/screw top tubes | # Label centrifuge/screw top tubes | ||
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# Close & vortex to mix. | # Close & vortex to mix. | ||
# Put in -80 C. | # Put in -80 C. | ||
- | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de page]] | |
<font size="4"> | <font size="4"> | ||
- | == ''' | + | == '''Recettes''' == |
<font size="2"> | <font size="2"> | ||
'''Lysogeny Broth (LB) Media''' | '''Lysogeny Broth (LB) Media''' | ||
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*2.5 microliters EtBr (Caution: EtBr is a known carcinogen) | *2.5 microliters EtBr (Caution: EtBr is a known carcinogen) | ||
*Note: Jacob suggested adding 1.0 microliter EtBr to gel and 3.0 microliters to TAE buffer in rig. | *Note: Jacob suggested adding 1.0 microliter EtBr to gel and 3.0 microliters to TAE buffer in rig. | ||
- | [[Team:Wash_U/Protocol#Procedures| | + | [[Team:Wash_U/French/Protocol#Procedures|Haut de Page]] |
{{WashUbottom}} | {{WashUbottom}} |
Latest revision as of 14:11, 8 July 2009