Composite

Part:BBa_K3771093

Designed by: KAO, YI-CHING   Group: iGEM21_NCKU_Tainan   (2021-10-17)
Revision as of 13:08, 18 October 2021 by Karin100699 (Talk | contribs)


SoxR-PsoxS-sfGFP


Description


This composite part consists of the soxR gene (BBa_K223000), promoter PsoxS (BBa_K3771048), and sfGFP (BBa_K1321337). The soxR and the soxS gene are components of the soxRS regulon, which is important for E. coli to sense and respond to the oxidants. When SoxR protein is fully oxidized, it becomes a powerful transcription activator of the soxS promoter (PsoxS) (up to 100-fold), leading to the expression of the downstream gene[1].



Usage and Biology


This composite part was ligated with the pSAA vector and transformed into E. coli. We conducted colony PCR to verify whether E. coli uptake the correct plasmid. The size of the PCR product was as expected. The part has been confirmed by sequencing and has no mutations.


Fig. 1. The electrophoresis result of colony PCR. M: Marker; Lane 1, 2: pSAA-soxR-PsoxS-sfgfp (3327 bp); Lane 3: pSAA-PsoxS-sfgfp (2691 bp).​


The promoter strength under oxidative stress of PsoxS with its activator, SoxR, is determined by the expression level of sfGFP, which is their reporter. While using hydrogen peroxide (H2O2) as the inducer, the intensity of soxR-PsoxS shows no significant difference under different concentrations of hydrogen peroxide (Fig. 2). However, soxR-PsoxS is well induced by using paraquat (PQ), which is a commonly used agent to induce oxidative stress for bacteria (Fig. 3 & 4).


Fig. 2. Relative fluorescence intensity of soxR-PsoxS after 4.5-hour incubation with hydrogen peroxide in various concentrations.


Fig. 3. Relative fluorescence intensity of soxR-PsoxS after 4.5-hour incubation with hydrogen peroxide in low concentrations.


Fig. 4. Relative fluorescence intensity of soxR-PsoxS after 4.5-hour incubation with hydrogen peroxide in high concentrations.


We compared the relative fluorescence intensity of sfGFP expressed by different promoters under the stimulation by different concentrations of paraquat. As expected, sfGFP expression level of J23100 shows no difference between the groups with and without paraquat. PsoxS with its activator, SoxR (BBa_K3771093), is highly activated under oxidative stress and has the highest gene expression level compared to J23100 (BBa_K3771050), PkatG (BBa_K3771091), and PsoxS (BBa_K3771092) solely (Fig. 5). Moreover, we compared the efficiency of our design with (BBa_K3771099), in which the concept came from the 2018 Imperial College London iGEM team. Different from our design, they used a mutant PsoxS promoter with RiboJ (BBa_K2862010) and expressed SoxR by J23101 promoter. However, the sfGFP expression by BBa_K2862010 was quite low (Fig. 6).

Fig. 5. Comparison of different promoter strengths by relative fluorescence intensity after 4.5-hour incubation with paraquat in high concentrations.


Fig. 6. Comparison of different promoter strengths by relative fluorescence intensity after 4.5-hour incubation with paraquat in low concentrations.



References


1. Pomposiello PJ, Demple B. Redox-operated genetic switches: the SoxR and OxyR transcription factors. Trends Biotechnol. 2001;19(3):109-114. doi:10.1016/s0167-7799(00)01542-0

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 596


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