Team:LMU-Munich/Project

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=== Evaluate Promoters ===
=== Evaluate Promoters ===
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Another goal is to produce promoters of ''Bacillus subtilis'' in BioBrick mode and to evaluate them. These well-defined promoters are then part of the Bacillus BioBrickBox which we will send to the registry but they can also be useful in our one project to express our fusion crust proteins on the outside of our spores. Therefore we will use different promoters, which are the constitutive promoters from the Anderson collection from the partsregistry, the constitutive promoters P''liaG'', P''veg'' and P''lepA'' from ''B. subtilis'' as well as the inducible promoter P''liaI'' from ''B. subtilis''. For the characterization of the different promoters we will clone them upstream of reporter genes (lux operon, lacZ) to measure their activity in ''Bacillus subtilis''. Therefore we use e.g. the two reporter vectors from ''B. subtilis'' which are also part of the Bacillus BioBrickBox. The first vector contains the lux operon as a reporter. This is why the activity of the promoter can be measured as luminescence with the plate reader (BioTek) which is a result of the expression of the luceiferase. The second reporter vector used for the evaluation of the promoters is ??? which contains the reporter gene ''lacZ''. The promoter activity leads to the production of the enzyme beta-galactosidase which cleaves the substrate ONPG. The product is detectable with the photometer and refers to the promtoer activity.
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Another goal is to produce promoters of ''Bacillus subtilis'' in BioBrick mode and to evaluate them. These well-defined promoters are then part of the Bacillus BioBrickBox which we will send to the registry but they can also be useful in our one project to express our fusion crust proteins on the outside of our spores. Therefore we will use different promoters, which are the constitutive promoters from the Anderson collection from the partsregistry, the constitutive promoters P''liaG'', P''veg'' and P''lepA'' from ''B. subtilis'' as well as the inducible promoter P''liaI'' from ''B. subtilis''. For the characterization of the different promoters we will clone them upstream of reporter genes (lux operon, lacZ) to measure their activity in ''Bacillus subtilis''. Therefore we use e.g. the two reporter vectors from ''B. subtilis'' which are also part of the ''Bacillus'' BioBrickBox. The first vector contains the lux operon as a reporter. This is why the activity of the promoter can be measured as luminescence with the plate reader (BioTek) which is a result of the expression of the luceiferase. The second reporter vector used for the evaluation of the promoters is pSBBs1C-''lacZ'' which contains the reporter gene ''lacZ''. The promoter activity leads to the production of the enzyme beta-galactosidase which cleaves the substrate ONPG. The product is detectable with the photometer and refers to the promtoer activity.
There are three types of promoters which will be evaluated in this project as a part of the so-called BioBrickBox:  
There are three types of promoters which will be evaluated in this project as a part of the so-called BioBrickBox:  

Revision as of 15:02, 18 August 2012

iGEM Ludwig-Maximilians-Universität München Beadzillus

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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".

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