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Team:LMU-Munich/Data
From 2012.igem.org
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===Crust Promoter Evaluation=== | ===Crust Promoter Evaluation=== | ||
{| "width=100%" style="text-align:center;"| | {| "width=100%" style="text-align:center;"| | ||
| - | |<p align="justify"> | + | |<p align="justify">Three sporulation-dependent promoters (blablabla) were constructed, two of which show the expected behavior.</p> |
|[[File:Promotoren.png|200px|link=Team:LMU-Munich/Data/crustpromoters]] | |[[File:Promotoren.png|200px|link=Team:LMU-Munich/Data/crustpromoters]] | ||
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===GFP-'''Sporo'''bead Evaluation=== | ===GFP-'''Sporo'''bead Evaluation=== | ||
{| "width=100%" style="text-align:center;"| | {| "width=100%" style="text-align:center;"| | ||
| - | |<p align="justify"> | + | |<p align="justify">They glow! GFP was successfully displayed on the spore crust as demonstreted by fluorescence microscopy</p> |
|[[File:Sporobead Constructs Dada sheet preview.png|200px|link=Team:LMU-Munich/Data/gfp_spore]] | |[[File:Sporobead Constructs Dada sheet preview.png|200px|link=Team:LMU-Munich/Data/gfp_spore]] | ||
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==='''Sporo'''bead Purification=== | ==='''Sporo'''bead Purification=== | ||
{| "width=100%" style="text-align:center;"| | {| "width=100%" style="text-align:center;"| | ||
| - | |<p align="justify">We compared different ways of purifying ''Bacillus'' spores from vegetative cells</p> | + | |<p align="justify">We compared different ways of purifying ''Bacillus'' spores from vegetative cells: Lysosome is the best!</p> |
|[[File:Purification preview.png|200px|link=Team:LMU-Munich/Data/Sporepurification]] | |[[File:Purification preview.png|200px|link=Team:LMU-Munich/Data/Sporepurification]] | ||
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===Knockouts of germination genes === | ===Knockouts of germination genes === | ||
{| "width=100%" style="text-align:center;"| | {| "width=100%" style="text-align:center;"| | ||
| - | |<p align="justify"> | + | |<p align="justify">We successfully prevented spore germination by multiple gene knockouts</p> |
|[[File:LMU Knockout previewii.jpg|200px|link=Team:LMU-Munich/Data/Knockout]] | |[[File:LMU Knockout previewii.jpg|200px|link=Team:LMU-Munich/Data/Knockout]] | ||
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===Suicide Switch === | ===Suicide Switch === | ||
{| "width=100%" style="text-align:center;"| | {| "width=100%" style="text-align:center;"| | ||
| - | |<p align="justify"> | + | |<p align="justify">Death upon germination: We developed a novel safety strategy as a back-up to knockouts.</p> |
|[[File:PlatereaderSuicideSwitch1.jpg|200px|link=Team:LMU-Munich/Data/Suicideswitch]] | |[[File:PlatereaderSuicideSwitch1.jpg|200px|link=Team:LMU-Munich/Data/Suicideswitch]] | ||
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Revision as of 21:28, 26 September 2012
The LMU-Munich team is exuberantly happy about the great success at the World Championship Jamboree in Boston. Our project Beadzillus finished 4th and won the prize for the "Best Wiki" (with Slovenia) and "Best New Application Project".
[ more news ]
Data
Here you will find all of our project data.
BacillusBioBrickBox
Evaluation of B. subtilis vectors
Seven novel vectors were constructed and four already proven to work in B. subtilis |  |
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Anderson Promoter Evaluation
Eleven Anderson promoters were measured in B. subtilis and showed relatively weak activity. | 
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Constitutive Bacillus Promoters
Three novel B. subtilis promoter BioBricks (PliaG, Pveg, PlepA) were constructed and functionality verified by luminescence and β-galactosidase assays. | 
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Inducible Bacillus Promoters
A novel antibiotic-inducible promoter,PliaI, was constructed and carefully evaluated. | 
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Sporobeads
Crust Promoter Evaluation
Three sporulation-dependent promoters (blablabla) were constructed, two of which show the expected behavior. | 
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GFP-Sporobead Evaluation
They glow! GFP was successfully displayed on the spore crust as demonstreted by fluorescence microscopy | 
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Sporobead Purification
We compared different ways of purifying Bacillus spores from vegetative cells: Lysosome is the best! | 
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GerminationSTOP
Knockouts of germination genes
We successfully prevented spore germination by multiple gene knockouts | 
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Suicide Switch
Death upon germination: We developed a novel safety strategy as a back-up to knockouts. | 
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Inverter
β-galactosidase assay of Inverter with lacZα
β-galactosidase assay of Inverter with lacZα dependent on Arabinose concentrations | 
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Trashcan
Things that were a pain in the neck!
cgeA and PcgeA
Unexpected restriction sites combined with no activity at all | 
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MazF
The story of trying to clone a toxine from E. coli in E. coli | 
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Xylose-promoters
All constructs involving Xylose-inducible promoter refused cloning or evaluation. | 
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For our big breakthroughs, or to follow specific projects, see the individual project pages:
