Team:Paris Bettencourt/Notebook/Odor Library
From 2014.igem.org
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- | <p>It worked!<img src='https://www.evernote.com/shard/s399/res/98825efa-7552-40d9-a853-1d557a0ce014/KR004618.BMP?resizeSmall&width= | + | <p>It worked! |
+ | <li><img src='https://www.evernote.com/shard/s399/res/98825efa-7552-40d9-a853-1d557a0ce014/KR004618.BMP?resizeSmall&width=400'><>/li</p> | ||
<h5>Date 1</h5> | <h5>Date 1</h5> |
Revision as of 15:18, 17 September 2014
Odor Library
Notebook
June
June 26th
Goal
Design plasmid for limonene synthase
Procedure
Used MG1665 strain, the RBS with the highest initial rate and the sequence of r-limonene synthase from genBank. Added polyhistidine tail to the construct. Submitted the construct to Jake.
Results
Designed plasmid for limonene synthase using the software geneious. Found a biobricks part containing this sequence. For the purpose of saving budget, we would first transform this standard part into cell and later modify it.
June 27th
Goal
: transform the bioBricks limonene synthase(BBa_I742111) part into e.coli.
Procedure
Results
transformed the plasmid containing limonene synthase sequence from biobricks into E.Coli. Colonies seen on both plates. Glycerol Stock made: PB. 018 and PB. 019
June 28th
Goal
Made chemical competent cell following standard protocol with MG1665 strains.
Procedure
Results
The transformed cell were grown for 20 hours and the transformation was successful. The plates were put into the 4 degree fridge for making stocks on Monday.
July
July 1st
Goal
to design the primers and gBlock to modify the BioBricks part BBa_I742111.
Procedure
Results
July 7th
Goal
to extract plasmid of biobricks I742111 from the transformed cells.
Procedure
Results
July 8th
Goal
Amplify limonene synthase gene sequence for E.coli
Procedure
Reagent | Volume |
1x | |
Nuclease-free water | 71 ul |
5x Phusion HF Buffer | 20 ul |
10 mM dNTPs | 2 ul |
Forward Primer (10 uM) | 1 ul |
Reverse Primer (10 uM) | 1 ul |
Template Plasmid | 1 ul |
Phusion DNA Polymerase | 1 ul |
DMSO | 3 ul |
Total Volume | 100 ul |
Temperature | Time | >Function | |
start | 98 C | 30 sec | melt |
cycle 1 | 98 C | 10 sec | melt |
cycle 2 | 51 C | 30 sec | anneal |
cycle 3 | 72 C | 30 sec | extend |
finish | 72 C | 5 min | extend |
blind | 10 C | forever | blind |
Results
PCR product at the expected length.
July 9th
Goal
Procedure
Reagent | Volume |
Nuclease-free water | 27.5 ul |
10x FD Buffer | 5 ul |
DNA | 12.5 ul |
AgeI | 2.5 ul |
Xbal | 2.5 ul |
Total Volume | 50 ul |
Results
The PCR product is at expected length. Purified product has a very low concentration(2.5ng/ul), meaning the PCR product was a mixture of multiple segments and didn't give ideal result. Therefore proceed to PCR again.
July 16th
Goal
Amplify limonene synthase gene sequence for E.coli
Procedure
Reagent | Volume |
1x | |
Nuclease-free water | 71 ul |
5x Phusion HF Buffer | 20 ul |
10 mM dNTPs | 2 ul |
Forward Primer (10 uM) | 1 ul |
Reverse Primer (10 uM) | 1 ul |
Template Plasmid | 1 ul |
Phusion DNA Polymerase | 1 ul |
DMSO | 3 ul |
Total Volume | 100 ul |
Temperature | Time | >Function | |
start | 98 C | 30 sec | melt |
cycle 1 | 98 C | 10 sec | melt |
cycle 2 | 51 C | 30 sec | anneal |
cycle 3 | 72 C | 2.5 min | extend |
finish | 72 C | 5 min | extend |
blind | 10 C | forever | blind |
Results
It worked!
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August
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September
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October
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