Part:BBa_J23113:Experience
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Applications of BBa_J23113
Evaluation of Anderson promoter J23113 in B. subtilis by iGEM-Team LMU-Munich 2012
This Anderson promoter was evaluated without fused RFP with the lux operon as a reporter in B. subtilis. See the new BioBrick BBa_K823010 without RFP and have a look at the [http://2012.igem.org/Team:LMU-Munich/Data/Anderson Data] from the evaluation in B. subtilis.
User Reviews
UNIQ3ea1828a6dd08515-partinfo-00000000-QINU UNIQ3ea1828a6dd08515-partinfo-00000001-QINU
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for iGEM-Team Goettingen 2012 |
Characterization experiment by qrtPCR on BBa_J23100, BBa_J23104, BBa_J23105, BBa_J23106, BBa_J23109, BBa_J23112, BBa_J23113, BBa_J23114 by iGEM Team Göttingen (by C. Krüger and J. Kampf)DescriptionWe used quantitative real time PCR to examine the expression rate of eight different constitutive promoter constructs of from the parts registry. The reported activities of these promoters are given as the relative fluorescence of these plasmids in strain TG1 ([http://2012.igem.org/Team:Goettingen/Project/Methods#Quantitative_Real-Time_PCR parts registry: part:BBa_J23100]). Promoter constructs were cloned into the vector pSB1C3 and expressed in E.coli BL21DE3 grown in LB-media (lysogeny broth). The measurements were performed for each construct and reference as a triplet. Additionally, we concluded H2O as negative control to predict possible contamination. For the evaluation of our results, the 2–ΔΔCT (Livak) Method was applied.
The data were compared to the determined expression rates from the part registry in the following figure.
You can find detailed information for our qrtPCR approach [http://2012.igem.org/Team:Goettingen/Project/Methods#-.3E_Experimental_design here]. Results & DiscussionOverall, each tested promoter construct indicated differences in expression rates in comparison to values from the “parts registry”. In fact, both data-sets were collected by methods which produce data at different points after gene expression. A common trend was detected for the strongest promoters J23100, J23104, J23105 and J23109 together with the weakest promoters J23112 and J23113. Conspicuously, the promoter J23109 revealed for qrtPCR and for relative fluorescence measurements nearly the same expression rates. The expression rates of J23114 and J23106 indicated massive differences in their expression rates and no common trend with the expression values from “parts registry”. We detected for six of our eight promoters comparable positioning in the ranking of expression rates (see Table, ranking). The promoters characterized as relative strong promoters were also in our case responsible for higher expression rates and the other way around, the promoters characterized as weak ones were in our case responsible for very low expression rates. In the case of promoter J23114 and J23106, the data-sets exhibited a completely different characterization compared to those in the “parts registry”. |