Coding
luxr

Part:BBa_C0062

Designed by: Vinay S Mahajan, Voichita D. Marinescu, Brian Chow, Alexander D Wissner-Gross and Peter Carr   Group: Antiquity   (2003-01-31)
Revision as of 18:29, 18 October 2019 by Ao Shen (Talk | contribs)

luxR repressor/activator, (no LVA?)

In complex with HSL, LuxR binds to the Lux promoter, activating transcription from Pr BBa_R0062, and repressing transcription from Pl BBa_R0063.

The lux cassette of V. fischeri contains a left and a right promoter. The right promoter gives weak constitutive expression of downstream genes.This expression is up-regulated by the action of the Lux activator, LuxR complexed to HSL. Two molecules of LuxR protein form a complex with two molecules the signalling compound homoserine lactone (HSL). This complex binds to a palindromic site on the promoter, increasing the rate of transcription.


Usage and Biology

We improved this part by using it in a part which allows for the constitutive expression of LuxR (BBa_K1893004). This part also includes the pLux promoter, so that genes placed downstream the promoter will be expressed when induced with 3OC6-AHL. We also made a part which allows for the characterisation of LuxR, as we placed GFP downstream the pLux promoter (BBa_K1893005). The part is currently being characterised.

Unspecified.

Sequence and Features


Barcodes are discontinued, but one was appended to the sequence of this part. Composite parts using this part will include the barcode. More ...

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
    COMPATIBLE WITH RFC[1000]


  • Allergen characterization of BBa_C0062: Not a potential allergen

The Baltimore Biocrew 2017 team discovered that proteins generated through biobrick parts can be evaluated for allergenicity. This information is important to the people using these parts in the lab, as well as when considering using the protein for mass production, or using in the environment. The allergenicity test permits a comparison between the sequences of the biobrick parts and the identified allergen proteins enlisted in a data base.The higher the similarity between the biobricks and the proteins, the more likely the biobrick is allergenic cross-reactive. In the full-length alignments by FASTA, 30% or more amount of similarity signifies that the biobrick has a Precaution Status meaning there is a potential risk with using the part. A 50% or more amount of identity signifies that the biobrick has a Possible Allergen Status. In the sliding window of 80 amino acid segments, greater than 35% signifies similarity to allergens. The percentage of similarity implies the potential of harm biobricks’ potential negative impact to exposed populations. For more information on how to assess your own biobrick part please see the “Allergenicity Testing Protocol” in the following page http://2017.igem.org/Team:Baltimore_Bio-Crew/Experiments


For the biobrick Part BBa_C0062, there was a 0% of identity match and 0% similarity match to the top allergens in the allergen database. This means that the biobrick part is not of potential allergen status. In 80 amino acid alignments by FASTA window, no matches found that are greater than 35% for this biobrick. This also means that there is not of potential allergen status.


>Internal Priming Screening Characterization of BBa_C0062: Has 1 possible internal priming site between this BioBrick part and the VR primer.

The 2018 Hawaii iGEM team evaluated the 40 most frequently used BioBricks and ran them through an internal priming screening process that we developed using the BLAST program tool. Out of the 40 BioBricks we evaluated, 10 of them showed possible internal priming of either the VF2 or VR primers and sometime even both. The data set has a range of sequence lengths from as small as 12 bases to as large as 1,210 bases. We experienced the issue of possible internal priming during the sequence verification process of our own BBa_K2574001 BioBrick and in the cloning process to express the part as a fusion protein. BBa_K2574001 is a composite part containing a VLP forming Gag protein sequence attached to a frequently used RFP part (BBa_E1010). We conducted a PCR amplification of the Gag-RFP insert using the VF2 and VR primers on the ligation product (pSB1C3 ligated to the Gag + RFP). This amplicon would serve as template for another PCR where we would add the NcoI and BamHI restriction enzyme sites through new primers for ligation into pET14b and subsequent induced expression. Despite gel confirming a rather large, approximately 2.1 kb insert band, our sequencing results with the VR primer and BamHI RFP reverse primer gave mixed results. Both should have displayed the end of the RFP, but the VR primer revealed the end of the Gag. Analysis of the VR primer on the Gag-RFP sequence revealed several sites where the VR primer could have annealed with ~9 - 12 bp of complementarity. Internal priming of forward and reverse primers can be detrimental to an iGEM project because you can never be sure if the desired construct was correctly inserted into the BioBrick plasmid without a successful sequence verification.

For the BioBrick part BBa_C0062, the first location of the internal priming site is on the 628-634 base number of the BioBrick and on the 14-20 base number of the VR primer.


Contribution: SiCAU-China 2017

Authors:Wenwen Lin

Summary:The QS system LuxR/LuxI has been widely used in kinds of logic circuit. But this year we find that LuxR can not always work well in E.coli. The LuxR, in E.coli, will not work when E.coli enter into stationary phase. This characteristic may be useful to users who will use LuxR as an activating transcription. (more details)

BBa C0062 SiCAU-China contribution.png

Contribution

Group: Valencia_UPV iGEM 2018
Author: Adrián Requena Gutiérrez, Carolina Ropero
Summary: We adapted the part to be able to assemble transcriptional units with the Golden Gate assembly method
Documentation: In order to create our complete [http://2018.igem.org/Team:Valencia_UPV/Part_Collection Printeira Part Collection] of parts compatible with the Golden Gate assembly method, we have made the part BBa_K2656016 which is BBa_C0062 adapted to the Golden Gate Technology.


无标题文档

HZAU-China 2019's Characterization

Design

In order to fit the project and guide the experiment, our research object for characterization studies is LuxR protein.

The plasmids consists of promoter (one of J23102, J23105, J23109), RBS B0032, luxR, terminator B1002, luxPR promoter, gfp coding sequence E0040,rrnB T1 terminator and T7Te terminator in order on a pSB1C3 backbone. We aim to induce the transcription of the downstream GFP by luxPR promoter by artificially adding different concentrations of HSL and LuxR which can form an activator complex LuxR-HSL. The amount of LuxR-HSL can be detected by luxPR promoter. The higher intensity of GFP expressed by luxPR, the more LuxR-HSL complex there will be. In this way, we can get insight into the binding characteristics of LuxR and HSL.

Within 15 hours after the addition of HSL, the OD600 and fluorescence intensity were measured using a microplate reader.

Expectation

Fluorescence is expected to occur in all three cultures, as all of these include the GFP coding sequence. However, due to the different intensities of the three promoters , J23102, J23105 and J23109, we predict that the fluorescence intensity of the same promoter should increase with the increase of HSL concentration, and the fluorescence intensity at the same HSL concentration should increase as the intensities of the promoter arise.

Materials and Methods

Plasmids Construction

luxR, luxPR and gfp are directly taken from the iGEM 2019 distribution kit and the promoter, RBS and terminator are ligated between the parts by overlap extension PCR, and the constructed fragment is ligated to PSB1C3 by homologous recombination. The correct construction is confirmed by sequencing.

Inoculation and cultivation

1.Pick three isolated colonies with a sterile tip from each of the three LB plates and add each tip into 5mL LB medium with 170μg/mL chloramphenicol. Incubate overnight at 37℃ in a shaker with 200rpm. Take 100μL bacterial of each flask into 5mL fresh new LB and incubate for another 3-4 hours.

2.Add each kind of bacterial fluid into different lines of a sterile, black-coated 96-well plate. Add shaken bacterial solution and fresh medium with 170μg/ml chloramphenicol to a total of 100μL, and make sure the OD600 of each well is 0.05-0.08, measured by the plate reader.

3.Add 1μL HSL diluted in DMSO into each well. The final concentration range of HSL is from 10-8 to 0.1 mmol/L. Add 1μL DMSO without HSL served as positive controls. Blank controls are fresh LB medium with DH5α. Place the 96-well plate into the automatic microplate reader (Synergy H1 hybrid multi-mode reader). Incubate at 37℃ overnight and measure the fluorescence value(excitation: 485nm, emission: 528nm)and OD600 of each well every 30 minutes.

4.Data taken from the plate reader are exported to Excel and imported to Origin for analysis.

5.All experiments above are carried out in 3 biological replications.

Results and analysis

Due to the different expression levels of GFP, the metabolic pressure of bacteria is different, and the growth of bacteria with different constitutive promoters is different. Therefore, it is difficult to find a time point of the bacteria to achieve proper data between different constructs. Finally, we take the 11th hour after adding HSL to collect data since the bacteria in most groups are in platform stage or just have slight decrease.

Figure 1. Fluorescence/OD600 over the concentration of HSL. Data are collected after 11 hours’ induction. All experiments are carried out in three biological replications and the error bar indicates standard error.

From figure 1, for each constitutive promoter, the ratio of fluorescence intensity to OD600 increases as the concentration of HSL increases after 11 hours’ induction (Figure 1). As known to everyone, J23102 has the highest transcription intensity followed by J23105, and J23109 remains the lowest. When the concentration of HSL is higher than 101nM, the ratio of fluorescence intensity to OD600 increases substantially as the intensities of the promoters increase at the same HSL concentration. At higher concentrations of HSL, the ratio of fluorescence intensity to OD600 decreases abnormally, most likely due to excessive metabolic stress induced by high concentration of HSL. From figure 2 we can figure out that high concentration of HSL has put excessive metabolism pressure on the bacteria. Because, it is 103-104nm/L HSL that induce the highest fluorescence intensity. As the concentration of HSL reaches 105nm/L, the intensity significantly decreases, even becomes lower than the intensity of 102nm/L (Figure 2).

Figure 2. Dynamic curves of fluorescence over time. (a) Fluorescence intensity over time at different concentrations of HSL of J23102. (b) Fluorescence intensity over time at different concentrations of HSL of J23105. (c) Fluorescence intensity over time at different concentrations of HSL of J23109. All experiments are carried out in three biological replications and the error bar indicates standard error.

In conclusion, the binding ability of LuxR and HSL is strong, and only a few LuxR are needed to respond to HSL of different concentrations. Moreover, a high concentration of HSL will lead to excessive metabolic pressure of bacteria, so an appropriate concentration of HSL is very necessary. The most appropriate concentration of HSL is about 103 nM as we determined.

[edit]
Categories
//cds
//cds/transcriptionalregulator/activator
//cds/transcriptionalregulator/repressor
//function/cellsignalling
//function/regulation/transcriptional
Parameters
directionForward
functionMixed
ligandsHSL
proteinLuxR
swissproP12746
tagNone