Generator
p(osmY).GF

Part:BBa_J45995

Designed by: Stephen Payne   Group: iGEM06_MIT   (2006-10-30)
Revision as of 21:26, 8 October 2022 by Bnabuageel (Talk | contribs) (William and Mary iGEM 2022)

Stationary phase dependent GFP generator

BBa_J45995 is a composite part consisting of an Escherichia coli osmY stationary phase promoter (BBa_J45992) and a GFP generator (BBa_E0840). Thus, BBa_J45995 produces fluorescence in stationary phase cultures.

Usage and Biology

See BBa_J45992 for details on the osmY stationary phase promoter.


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 BsaI.rc site found at 872


William and Mary iGEM 2022

The 2022 William and Mary iGEM team created two composite parts to improve part BBa_J45995. One of our parts is BBa_K4174001 and the other is BBa_K417002. Like BBa_J45995, these parts use an osmY promoter, which is induced by the host cell's entry into stationary phase. In typical E. coli cells, osmY, which helps cells transition into stationary phase when under osmotic or metabolic stress, is not produced during exponential growth phase but is produced during stationary phase. Specifically, the osmY promoter is induced by the rpoS (ribosome polymerase sigma S) at the onset of stationary phase (Chang 2002). In part BBa_K4174001, this promoter is partnered with a mRFP1 coding region, and this construct fluoresces red once the host cell has entered stationary phase. In part BBa_K417002, this promoter is partnered with a sfGFP coding region, and this construct fluoresces green once the host cell has entered stationary phase. More information about the design and characterization of each of these parts can be found below.

    BBa_K417001 Design & Characterization
  • In this composite part, we have replaced GFP with mRFP1 from Mutalik et al. 2013 and added unique nuclotide sequences (UNSs) 1 and 10 sequences (Torella et al, 2014) to the ends of the construct.
  • We elected to use monomeric red fluorescent protein 1 (mRFP1) as opposed to the original GFP, as it allows for the construction of an alternative fluorescent reporter.
  • We added UNS1 and UNS10 sequences to make this part compatible with Gibson Assembly with our pSB1C3 backbone, as we also added UNS1 and UNS10 to our backbone.

To test the effectiveness of our improved parts, our team grew the original construct (BBa_J45995), our mRFP1 construct, and our sfGFP construct (BBa_K4174001) in E. coli NEB5α in a plate reader. They were grown at 37°C using continuous shaking. For red fluorescence measurements, we used an excitation value of 584 nm and an emission value of 610 nm. For green fluorescence measurements, we used an excitation value of 485 nm and an emission value of 528 nm. The values for red fluorescence are reported below.

improve-a-part-red-fluorescence-graph.png

Based on the graph above, the bacterial cells engineered with our mRFP1 construct appear to have entered stationary phase around 16 hours. As seen in the graph, our mRFP1 construct produces more red fluorescence than the original circuit. The other measurements taken are for our sfGFP construct and untransformed E. coli NEB5α cells, both of which serve as negative controls for red fluorescence.

improveapart-smaller.png

As seen in the image above, qualitative results reveal that our mRFP1 construct produces more red fluorescence than the original construct. Here, our mRFP1 construct is on the far left, and is visibly more red that the original GFP construct.


BBa_K417002 Design & Characterization

In this composite part, we have replaced GFP with sfGFP from Ceroni et al. 2015, replaced RBS BBa_B0030 with an RBS containing region from Ceroni et al. 2015, removed the scar sequences, and added UNS1 and UNS10 sequences to the ends.

  • We elected to use super-folder green fluorescent protein (sfGFP) as opposed to the original GFP, as it folds more readily in Escherichia coli, thus serving as a more effective assay (Pédelacq 2006).
  • We switched the original RBS with an RBS containing region used with the sfGFP sequence in Ceroni (2015)'s paper. Our team had previously used those parts together successfully, so we elected to use them together again.
  • We added UNS1 and UNS10 sequences to make this part compatible with Gibson Assembly with our backbone, as we also added UNS1 and UNS10 to our pSB1C3 backbone.

To test the effectiveness of our improved parts, our team grew the original MIT 2006 construct, our improved sfGFP construct, and our improved RFP construct in E. coli NEB5α in a plate reader. They were grown at 37°C using continuous shaking. For green fluorescence, we used an excitation value of 485 and an emission value of 528. For red fluorescence, we used an excitation value of 584 and an emission value of 610. The values for green fluorescence are reported below.

normalized-green-fluorescence.png

As seen in the graph above, both the sfGFP and MIT GFP constructs enter stationary phase right before 14 hours, but our improved sfGFP circuit is much more fluorescent. The other constructs are our RFP construct and untransformed E. coli cells, both of which serve as negative controls for green fluorescence.

improveapart-smaller.png

As seen in the image above, qualitative results reveal that our improved constructs are more fluorescent than the original construct. Here, sfGFP is on the far right, and is visibly more brightly green that the original GFP construct.

[edit]
Categories
//classic/reporter/pret
s
Parameters
None