Reporter

Part:BBa_K1031803

Designed by: He Shuaixin   Group: iGEM13_Peking   (2013-09-09)
Revision as of 02:16, 28 September 2013 by Robinbin (Talk | contribs) (Introduction)

Pu-B0031-sfGFP-Terminator (XylR)

For detailed information concerning XylR and Pu promoter, please visit 2013 Peking iGEM Biosensor XylR


Introduction

Promoter structure

Pu promoter which is activated by XylR, is σ54 dependent. It is composed of three elements. The UBS (Upstream Binding Site) site which is responsible for interacting with XylR transcriptional factor. The IHF binding site which allows IHF to participate, enhancing transcription efficiency. -24 and -12 region interact with σ54 factor of RNA polymerase, enabling the formation of open complex. (Fig.1)

Figure.1 Structure of Pu promoter. The UAS of this promoter shown as blue sequence in the blue frame interacts with DmpR. IHF binding site is shown in green in the green frame. The orange sequence indicates σ54 binding site as -24 region and -12 region. The G in red represents +1 site.


Gene cluster and chemical pathway

XylR is an intensively studied regulatory protein mined from Pseudomonas putida[1]. It responds strongly to toluene, xylene and 4-chlro-toluene, while weakly to 3-methyl benzyl alcohol[1]. XylR activates the Pu promoter to express the "upper pathway" (XylMABC) when exposed to m-xylene (Fig.2). It also activates the Ps1<i> promoter, thus to produce another transcriptional activator, called XylS, to turn on the expression of the downstream pathway (<i>XylXYZLTEGFJGKIH, the meta-cleavage operon)[1][2](Fig.2, Fig.3). Notably, the entire regulatory network is also controlled by several global regulatory elements, such as IHF. This provides an explanation for the genetic-context-dependent performance of XylR-Pu pair; namely, when expressed in different bacterial species, the regulatory performance of XylR/Pu pair often fails[3]. Therefore, fine-tuning is probably necessary.

Figure.2 The regulatory network of TOL pathway, including the xyl gene cluster, XylS and XylR. XylR is the master regulator that regulates Pu promoter (controls "upper pathway", XylMABC) and Ps2 promoter (controls the expression of XylS, thus to indirectly activate the expression of "downstream pathway“, XylXYZLTEGFJGKIH). The xylene or its derivatives are supposed to be the typical inducers of XylR.


Fig.3 The TOL degradation pathway. The supposed inducers of XylR, toluene and its derivatives, are highlighted in blue.


Protein structure

The XylR protein consists of FOUR domains (Fig.4): Domain A is the sensor domain, which will conduct a conformational change upon effector binding. Previous studies showed that Domain A inhibits the DNA binding affinity of Domain C before the conformational change[4][5]. Domain B is a linker domain; mutations in this domain will disrupt the functional coupling and spatial interactions between Domain A and C[6].

Domain C is the effector-binding domain with ATPase activity that is crucial for XylR dimerization. A subdomain in domain C is assumed to account for the dimerization. Domain D is the DNA binding domain featured by helix-turn-helix motif whose DNA binding is sequence-specific.

Fig.4 Schematic organization of XylR protein domains. From N-terminal to C-terminal: the sensor domain A, the linker domain B, the dimerization domain C and the DNA binding domain D.


Mechanism

XylR is capable of forming tetramer when bound with ATP[7]. Without ATP binding, the XylR dimers bind to two sequence-specific DNA sites. As a typical σ54-dependent transcriptional activator, with the binding of ATP, two dimers of XylR tend to further cooperatively tetramerize, thus to bend the promoter region DNA with the help of integrated host factor (IHF). As a result, the transcription will be launched by the interaction between the XylR tetramer and RNA Polymerase (RNAP). ATP hydrolysis provides energy for this process[8].(Fig 5)

Fig.5 The mechanism of σ54-dependent transcription activation by XylR. Step1, RNAP recruitment by σ54; XylR has formed dimers when binding to DNA. Step2, formation of XylR tetramer, coupled with ATP hydrolysis. Step3, RNAP ready to initiate transcription. Step4, transcription start with σ54 released. See the main text for more detailed explanation of transcription activation at the Pu promoter.


Previous engineering effort

Random mutagenesis on XylR Domain B has been performed in previous studies Ref.[9]. One XylR mutant, referred to as XylR28 in ref. [9], carries 4 point mutations in Domain A and Domain B. These point mutations endow XylR with a remarkably improved response to 2.4-DNT and TNT and a reduced response to its natural inducer, m-xylene, indicating the directed evolution may provide possibility to engineer XylR to respond to compounds that it doesn't naturally sense[6].

As discussed above, the XylR/Pu pair usually needs fine-tuning. Promoter engineering is considered to be an answer. A XylR-conrolled Pu promoter shows a high basal level. But the cognate promoter of XylR homolog, DmpR, has a fairly low basal level. We found that XylR could activate the Po promoter of DmpR. A hybrid promoter has been accordingly designed using the binding site of XylR from the Pu promoter. This design has shown that the basal level of the hybrid promoter is low and the XylR binding affinity is high[12].

Sequence and Features

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal NheI site found at 167
  • 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 219



Construction

Pc promoter J23114 is selected to initiate the transcription of XylR. Based on this circuit, we constructed a library of RBS (Ribosome Binding Site) including B0031[1], B0032[2], B0033[3] and B0034[4] for tunning for expression level of reporter gene sfGFP. K1031803 consists of Pu promoter, RBS B0031 and reporter gene sfGFP (Fig 6).

Fig.6 Construction of reporter circuit ''Pu''-B0031-sfGFP. The orange arrow represents ''Pu'' promoter for XylR. The green oval stands for RBS B0031. sfGFP coding sequence is shown with dark blue, while terminator B0015[https://parts.igem.org/Part:BBa_B0015] is in dark red.


Data shown

We obtained XylR from the TOL plasmid of Pseudomonas putida mt-2[11][13]. It was then exploited to build the XylR biosensor. We used a library of constitutive promoters (Pc) to control the expression level of XylR. We expected this would fine-tuning the performance of XylR biosensor, because previous studies indicated that, the expression level of XylR is critical for its regulatory performance on Pu promoter. Results showed that the XylR biosensor with a medium strong Pc promoter, BBa_J23106, works the best (Fig. 7).

Figure.7 The induction ratios of all 78 aromatic compounds obtained from the ON/OFF Test using Test Protocol 1.
(a) XylR biosensor could respond to several aromatics whose induction ratios are not sufficiently high. This result was inconsistent with previous studies [5], which is probably due to the vaporization of hydrophobic aromatic compounds, as we discussed in the main text. (b) The aromatics-sensing profile of XylR biosensor. The aromatic species that can elicit strong responses of XylR biosensor are highlighted in orange in the aromatics spectrum. The structure formula of the typical inducer(s) is also presented around the spectrum. The induction ratio was calculated by dividing the fluorescence intensity of biosensor exposed to object inducers by the basal fluorescence intensity of the biosensor itself. Click Here for the full names of aromatic compounds.


As shown in Fig.7, the performance of XylR is quite different from the previous studies. The conventional inducers for XylR, for instance, TOL, m-Xyl and 3-CITOL, could not elicit any significant responses. It was probably because that these hydrophobic aromatic compounds can vaporize and permeate the sealing film used in our experiment. Regarding this problem, we performed the ON/OFF Test using centrifuge tubes, rather than the conventional 96-well microplate. Results indicated that the XylR biosensor indeed could give response to conventional hydrophobic compounds such as TOL and m-Xyl if the vaporization could be prevented (Fig.8).

Figure.8 The induction ratios of hydrophobic aromatics compounds obtained from the ON/OFF Test using the new protocol (the same with Test Protocol 1 except that the experiments were performed in centrifuge tubes to avoid the vaporization).

Reference


[1] Abril, M. A., Michan, C., Timmis, K. N., & Ramos, J. (1989). Regulator and enzyme specificities of the TOL plasmid-encoded upper pathway for degradation of aromatic hydrocarbons and expansion of the substrate range of the pathway.Journal of bacteriology, 171(12), 6782-6790.
[2] Gerischer, U. (2002). Specific and global regulation of genes associated with the degradation of aromatic compounds in bacteria. Journal of molecular microbiology and biotechnology, 4(2), 111- 122.
[3] Valls, M., Silva‐Rocha, R., Cases, I., Muñoz, A., & de Lorenzo, V. (2011). Functional analysis of the integration host factor site of the σ54Pu promoter of Pseudomonas putida by in vivo UV imprinting. Molecular microbiology, 82(3), 591-601.
[4] Devos, D., Garmendia, J., Lorenzo, V. D., & Valencia, A. (2002). Deciphering the action of aromatic effectors on the prokaryotic enhancer‐binding protein XylR: a structural model of its N‐ terminal domain. Environmental microbiology, 4(1), 29-41.
[5] Salto, R., Delgado, A., Michán, C., Marqués, S., & Ramos, J. L. (1998). Modulation of the function of the signal receptor domain of XylR, a member of a family of prokaryotic enhancer-like positive regulators. Journal of bacteriology,180(3), 600-604.
[6] Garmendia, J., & De Lorenzo, V. (2000). The role of the interdomain B linker in the activation of the XylR protein of Pseudomonas putida. Molecular microbiology, 38(2), 401-410.
[7] Tropel, D., & Van Der Meer, J. R. (2004). Bacterial transcriptional regulators for degradation pathways of aromatic compounds. Microbiology and Molecular Biology Reviews, 68(3), 474-500.
[8] Pérez-Martín, J., & de Lorenzo, V. (1996). ATP Binding to the σ< sup> 54-Dependent Activator XylRTriggers a Protein Multimerization Cycle Catalyzed by UAS DNA. Cell, 86(2), 331-339.
[9] de las Heras, A., Chavarría, M., & de Lorenzo, V. (2011). Association of dnt genes of Burkholderia sp. DNT with the substrate‐blind regulator DntR draws the evolutionary itinerary of 2, 4‐ dinitrotoluene biodegradation. Molecular microbiology, 82(2), 287-299.
[10] de las Heras, A., & de Lorenzo, V. (2011). Cooperative amino acid changes shift the response of the σ54‐dependent regulator XylR from natural m‐xylene towards xenobiotic 2, 4‐ dinitrotoluene. Molecular microbiology, 79(5), 1248-1259.
[11] Garmendia, J., De Las Heras, A., Galvão, T. C., & De Lorenzo, V. (2008). Tracing explosives in soil with transcriptional regulators of Pseudomonas putida evolved for responding to nitrotoluenes. Microbial Biotechnology, 1(3), 236-246.
[12] Kim, M. N., Park, H. H., Lim, W. K., & Shin, H. J. (2005). Construction and comparison of< i> Escherichia coli whole-cell biosensors capable of detecting aromatic compounds. Journal of microbiological methods, 60(2), 235-245.
[13] Garmendia, J., Devos, D., Valencia, A., & De Lorenzo, V. (2001). À la carte transcriptional regulators: unlocking responses of the prokaryotic enhancer‐binding protein XylR to non‐natural effectors. Molecular microbiology, 42(1), 47-59.


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