Part:BBa_K2705011
PliaG&43-3
PliaG&43-3 is a promoter which is artificially combined PliaG with P43 and modified.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
The original part PliaG(BBa_K823000)
PliaG(BBa_K823000) is a weak, constitutive promoter from B. subtilis. It’s responsible for the transcription of the last four genes of the liaIHGFSR locus and therefore for the production of the components of the LiaRS system, which is important for the detection of cell wall antibiotics (Jordan et al., 2006). PliaG was evaluated with the lux operon as well as the lacZ as reporter. For more details, visit the Data page of the LMU-Munich Team 2012 or get an overview of the whole project Beadzillus.( http://2012.igem.org/Team:LMU-Munich)
Design
We improved the part PliaG(BBa_K823000) which is a weak, constitutive promoter of Bacillus subtilis. Inspired by the relatively strong constitutive promoter P43(BBa_K143013), we chose to mimic its structure, which can be recognized by both sigma factor 55 (the major sigma factor A) and sigma factor 37 (the lag phase sigma factor B). As the promoter PliaG is a constitutive Bacillus subtilis σA promoter, we replace some part of the promoter PliaG sequence with the σB recognition site at the same relative position which the σB recognition site to the σA recognition site of the promoter P43 to create the new promoter PliaG&43. On the basis of this, we made 2 adjustments to create another new promoter P liaG&43-3. The first one is to adjust the sequence of the -35 region of PliaG (from CGTATC to TTGACA). The other one is adjustments to the spacing between -35 region and -10 region from 19 bp to 17 bp.
Luminescence measurements
The constitutive promoters PliaG&43-3 (BBa_K2705011) was evaluated in the reporter vector pHT01-Px-GFP. The promoter activity results in gene expression and production of the protein green fluorescence protein(GFP). The fluorescence intensity(FI) was measured by the Multimode Plate Reader Enspire(PerkinElmer). All clones showed a normal growth behavior. As the σB recognition site of P43 we added is for the lag phase, we tested the FI at the very beginning (the lag phase, Fig.1) of its life. PliaG&43-3outperformed the original promoter PliaG at the lag phase, whose activity is about 1.34 times as high as that of PliaG.
None |