Team:Caltech/Protocols
From 2011.igem.org
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For both: culture initially for 3 days, then reculture for 7 days. Then test for DNA and continue cultures.<br/><br/></p> | For both: culture initially for 3 days, then reculture for 7 days. Then test for DNA and continue cultures.<br/><br/></p> | ||
- | <p>'''Fosmid kit''' | + | <p>'''Fosmid kit'''<br/> |
+ | http://www.epibio.com/pdftechlit/171pl1010.pdf</p><br/> | ||
<p>'''Gibson Assembly (Adapted from Cambridge 2010)'''<br/> | <p>'''Gibson Assembly (Adapted from Cambridge 2010)'''<br/> | ||
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4. Cool, then transform into chemically competent cells<br/></p><br/> | 4. Cool, then transform into chemically competent cells<br/></p><br/> | ||
- | <p>'''Mobio PowerMax Soil kit''' | + | <p>'''Mobio PowerMax Soil kit'''<br/> |
+ | http://www.mobio.com/images/custom/file/protocol/12988-10.pdf</p><br/> | ||
<p>'''Pulse Gel Field Electrophoresis''':<br/> | <p>'''Pulse Gel Field Electrophoresis''':<br/> | ||
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Final Extension: 72°C for 5 minutes</p><br/> | Final Extension: 72°C for 5 minutes</p><br/> | ||
- | <p>'''Qiagen Miniprep kit''' | + | <p>'''Qiagen Miniprep kit'''<br/> |
+ | www.qiagen.com/hb/qiaprepminiprep<br/></p><br/> | ||
<p>'''Transforming DNA from Distribution Plates:'''<br/> | <p>'''Transforming DNA from Distribution Plates:'''<br/> |
Revision as of 22:23, 27 July 2011
Project |
Back to Timeline . Recipes for Mixes Enrichment cultures
2. Place 8 test tubes in 30°C shaker and 8 test tubes in room temperature shaker.
2. Add small amounts (around 50mL or 50mg) of the ten LA river samples into each flask. For both: culture initially for 3 days, then reculture for 7 days. Then test for DNA and continue cultures. Fosmid kit Gibson Assembly (Adapted from Cambridge 2010) Mobio PowerMax Soil kit Pulse Gel Field Electrophoresis: Phusion PCR
Qiagen Miniprep kit Transforming DNA from Distribution Plates: Taq PCR (16s insert)
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