Generator

Part:BBa_K1741006

Designed by: Marta Żardecka   Group: iGEM15_UAM_Poznan   (2015-09-17)

sfGFP under short rhamnose promoter (very weak)

Both CRP sites were removed from the Rha1 promoter. It seems likely that RhaS binding site has been affected as well, so even though the resulting promoter is still induced by rhamnose, the induction is very weak.

Design

Legend:

RhaWT - rhamnose wild type

TeamUAMpoznanRhaWTseq.jpg


Rha1 - [BBa_K1741005]

TeamuampoznanRha1seq.jpg


Rha2 - [BBa_K1741006]

TeamuampoznanRhaS1.jpg


Our wild type rhamnose promoter is commercially available. However, we had to modify it to remove EcoRI restriction site to fit BioBrick standards. We achieved it by a single point mutation of cytosine to thymine - that is how Rha1 was created. Afterwards, we decided to further minimize the promoter sequence by removing the CRP site - we called this construct Rha2.


Results

Legend:

RhaWT - rhamnose wild type

Rha1 - [BBa_K1741005]

Rha2 - [BBa_K1741006]

Teamuampoznanrhamnoselbgraph.png Teamuampoznanrhamnosem9graph.png


The sfGFP fluorescence [RFU] was measured using Tecan fluorometer.

All three rhamnose promoters are induced by rhamnose and repressed by glucose. Turns out that single point mutation in EcoRI restriction site in Rha1 significantly increased the activity of the promoter as compared to the wild type construct. Rha2 is a weak promoter, perfect for people who would like to manufacture small amount of the protein of interest.

We also checked the tightness of our promoters.

All of our promoters are induced only by their respective sugars with a small exception of xylose promoters being slightly induced by arabinose and arabinose promoters being slightly induced by xylose. All of our promoters are repressed by glucose. Teamuampoznanpromoterscomparisongrpah.png



Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal SapI.rc site found at 148


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