Team:Austin Texas/Week of July 23 to July 29
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*Razan | *Razan | ||
**7/24- Amplified pACYC backbone successfully with new primers for both control and converter plasmids. | **7/24- Amplified pACYC backbone successfully with new primers for both control and converter plasmids. | ||
+ | **7/26- Performed overlap PCR of the 2 inserts (CRE and LasR for converter and GFP and LasR for control). | ||
+ | **7/27- Performed gibson assembly on the overlap PCR of the inserts and the pACYC backbone amplifications for both pconverter and control converter with successful transformation! | ||
== Design of Reporter Plasmid == | == Design of Reporter Plasmid == | ||
+ | |||
+ | * Ben | ||
+ | ** Prepped pReporter and pReporter.permaflipped DNA. | ||
+ | ** '''PCR:''' | ||
+ | *** pReporter: JE.rrnB.F, JE.GFPTerm.R | ||
+ | *** pReporter.permaflipped: JE.rrnB.F, JE.GFPTerm.R | ||
+ | *** '''Results:''' One correct-size band for pReporter.permaflipped; none for pReporter. Submitted for sequencing. Made frozen stock. Will retry colony PCR for pReporter. | ||
+ | ** '''Colony PCR:''' (retrying with Phusion + DMSO instead of Taq MM because I noticed JE.rrnB.F has poor secondary structure--probably why no products have shown up in these colony PCRs) | ||
+ | *** pReporter: JE.rrnB.F, JE.GFPTerm.R | ||
+ | *** '''Results:''' Correct-size band. Made frozen stock, prepped, and submitted for sequencing. | ||
== Spinach Aptamer == | == Spinach Aptamer == | ||
+ | *Logan | ||
+ | **7/23 - Grew cultures of 5' and 3' mCherry-SpA constructs, SpA, and mCherry alone for plate reader exp. Submitted 3' construct for sequencing. | ||
+ | **7/24 - Attempted Cuvette exp in plate reader: added 25uM DFHBI to solution, induced constructs in BL21 AI cells with 1 mM IPTG, 0.2% arabinose. Result: No fluorescence detected. (bad plate reader?) | ||
== CBB5 Caffeine Inducible Promoters == | == CBB5 Caffeine Inducible Promoters == |
Latest revision as of 01:02, 3 October 2012
Contents |
Notebook for week of July 23 to July 29
Design of Converter Plasmid
- Razan
- 7/24- Amplified pACYC backbone successfully with new primers for both control and converter plasmids.
- 7/26- Performed overlap PCR of the 2 inserts (CRE and LasR for converter and GFP and LasR for control).
- 7/27- Performed gibson assembly on the overlap PCR of the inserts and the pACYC backbone amplifications for both pconverter and control converter with successful transformation!
Design of Reporter Plasmid
- Ben
- Prepped pReporter and pReporter.permaflipped DNA.
- PCR:
- pReporter: JE.rrnB.F, JE.GFPTerm.R
- pReporter.permaflipped: JE.rrnB.F, JE.GFPTerm.R
- Results: One correct-size band for pReporter.permaflipped; none for pReporter. Submitted for sequencing. Made frozen stock. Will retry colony PCR for pReporter.
- Colony PCR: (retrying with Phusion + DMSO instead of Taq MM because I noticed JE.rrnB.F has poor secondary structure--probably why no products have shown up in these colony PCRs)
- pReporter: JE.rrnB.F, JE.GFPTerm.R
- Results: Correct-size band. Made frozen stock, prepped, and submitted for sequencing.
Spinach Aptamer
- Logan
- 7/23 - Grew cultures of 5' and 3' mCherry-SpA constructs, SpA, and mCherry alone for plate reader exp. Submitted 3' construct for sequencing.
- 7/24 - Attempted Cuvette exp in plate reader: added 25uM DFHBI to solution, induced constructs in BL21 AI cells with 1 mM IPTG, 0.2% arabinose. Result: No fluorescence detected. (bad plate reader?)
CBB5 Caffeine Inducible Promoters
- Peter
- 7/23- Cotransformation of PRA301-ndmApro LacZ reporter plasmid (with spectinomycin reporter) and ORF1 -4,5,6 plasmid minipreps. Ran out of PRA301-ndmApro plasmid, so only ORF1-4,5 were cotransformed. ORF1- 6 was transformed by itself as a control. Plated on kanamycin/XGal plates.
- 7/24- Cotransformation failed. Likely due to too much plasmid, mixed with poor transformation.