Team:Evry/Interlab Study/Results
From 2014.igem.org
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Our team achieved the 19 constructions of the Anderson library. Constructions were first designed in a software(Geneious v. 6.1.6)and then relized on web lab using iGEM 2014 Distribution kit. Verifications were made by eletrophoresis gel analytic PCR amplification and sequencing. Glycerol stock of 3 colonies per constructions were conserved and used for the measurments of GFP expression. | Our team achieved the 19 constructions of the Anderson library. Constructions were first designed in a software(Geneious v. 6.1.6)and then relized on web lab using iGEM 2014 Distribution kit. Verifications were made by eletrophoresis gel analytic PCR amplification and sequencing. Glycerol stock of 3 colonies per constructions were conserved and used for the measurments of GFP expression. | ||
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- | Unfortunatly, we did not collect satisfying data for the 19 constructions although assays were repeated several times. The data profile was repeatable under people, apparatus and strain. However exploitable data were collected for 5 constructions (100, 104, 105, 107 and 118) for which | + | Unfortunatly, we did not collect satisfying data for the 19 constructions although assays were repeated several times. The data profile was repeatable under people, apparatus and strain. However exploitable data were collected for 5 constructions (100, 104, 105, 107 and 118) for which the relationship between corrected GFP fluorescence and OD 600 nm is linear that corresponded to the expected profile for a constitutive promoter. Corrected GFP fluorescence intensity at OD 600 nm = 0.45 of these 5 constructions were compared on the bar chart below. |
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- | Hypothesis to explain | + | Hypothesis to explain data acquisition problems: |
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Revision as of 00:51, 18 October 2014
Interlab study - Aim & Results
The goal of the interlab study is to obtain GFP fluorescence data from the iGEM teams all around the world for about twenty constructions. This will permit to observe the result repeatability across technics, strains and teams.
There were two sub-parts in this study:
There were two sub-parts in this study:
- The mandatory one: obtain fluorescence data for three specific genetic devices expressing GFP and compare them.
- The Extra Credit assignments: we choose to study the entire Anderson library of constitutive prokaryotic promoters (J23100 to J23119).
This library corresponds to 19 constitutive promoters containing some nucleotide mutations on the -35 and the -10, as shown Used Biobricks and plasmids . The idea is to compare the expression strength of promoters according to mutations, from the maximum amount of fluorescence data in order to have significant results.
Required Devices
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The three required constructions shown various fluorescence intensity at OD 600 nm = 0.5, as shown on graph and bar chart below. As shown on corrected GFP fluorescence intensity according to OD 600 nm, the relationship between corrected GFP fluorescence and OD 600 nm is linear that corresponded to the expected profile for a constitutive promoter.
Theoritically constructions I20260 and J3101 were similar, constructions and alignments in sillico matched perfectly. The difference between these constructions lies on the assembly way. However we obtained, as some other teams (University of Oxford, Paris-Bettencourt and ITESM-CEM), significant GFP expression difference. There is probably a Biobrick standard construction problem, which relates to the traited question on our Phylosophy subsection.
Theoritically constructions I20260 and J3101 were similar, constructions and alignments in sillico matched perfectly. The difference between these constructions lies on the assembly way. However we obtained, as some other teams (University of Oxford, Paris-Bettencourt and ITESM-CEM), significant GFP expression difference. There is probably a Biobrick standard construction problem, which relates to the traited question on our Phylosophy subsection.
Entire Anderson library of constitutive promoters (J23100-J23119)
|
|
Our team achieved the 19 constructions of the Anderson library. Constructions were first designed in a software(Geneious v. 6.1.6)and then relized on web lab using iGEM 2014 Distribution kit. Verifications were made by eletrophoresis gel analytic PCR amplification and sequencing. Glycerol stock of 3 colonies per constructions were conserved and used for the measurments of GFP expression.
Unfortunatly, we did not collect satisfying data for the 19 constructions although assays were repeated several times. The data profile was repeatable under people, apparatus and strain. However exploitable data were collected for 5 constructions (100, 104, 105, 107 and 118) for which the relationship between corrected GFP fluorescence and OD 600 nm is linear that corresponded to the expected profile for a constitutive promoter. Corrected GFP fluorescence intensity at OD 600 nm = 0.45 of these 5 constructions were compared on the bar chart below.
Hypothesis to explain data acquisition problems:
Unfortunatly, we did not collect satisfying data for the 19 constructions although assays were repeated several times. The data profile was repeatable under people, apparatus and strain. However exploitable data were collected for 5 constructions (100, 104, 105, 107 and 118) for which the relationship between corrected GFP fluorescence and OD 600 nm is linear that corresponded to the expected profile for a constitutive promoter. Corrected GFP fluorescence intensity at OD 600 nm = 0.45 of these 5 constructions were compared on the bar chart below.
Hypothesis to explain data acquisition problems: