Difference between revisions of "Part:BBa K1127008"

(Characterization)
(Characterization)
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==Characterization==
 
==Characterization==
The device has LacZ alpha which is useful for characterization. To determine activity of the part, beta-galactosidase assay was performed using PNPG as the substrate. In all experiments, untransformed E. coli strain DH5 alpha or strain BL21 were used as our negative control. The protocols are described in more detail on the [http://2013.igem.org/Team:York_UK/Notebook.html?page=protocols].
+
The device has LacZ alpha which is useful for characterization. To determine activity of the part, beta-galactosidase assay was performed using PNPG as the substrate. In all experiments, untransformed E. coli strain DH5 alpha or strain BL21 were used as our negative control. The protocols are described in more detail on our wiki page [http://2013.igem.org/Team:York_UK/Notebook.html?page=protocols].
  
 
The experiments showed that E. coli strain DH5 alpha transformed with the device can respond to gold (AuCl4). In Figure 1A, production of the enzyme increased significantly in the presence of the full construct (DH5 alpha_AB) but reduced to the basal level in the absence of golS (DH5 alpha_A). This signifies the function of golS as a gold-dependent transcriptional activator.  
 
The experiments showed that E. coli strain DH5 alpha transformed with the device can respond to gold (AuCl4). In Figure 1A, production of the enzyme increased significantly in the presence of the full construct (DH5 alpha_AB) but reduced to the basal level in the absence of golS (DH5 alpha_A). This signifies the function of golS as a gold-dependent transcriptional activator.  

Revision as of 10:57, 3 October 2013

Gold sensing device (PgolTS+LacZ+GolS)

This is the device we use in our project so that the cell could recognize the presence of gold in its environment. GolS protein acts as a positive transcriptional regulator on PgolTS once it binds to gold. Part was designed so that you can detect and quantify the activity of the promoter via Beta-galactosidase assay. For convenience the ORF of LacZ is covered by restriction sites of SacII and SanDI which allows the cell to respond to gold by expressing something to meet your needs.

The promoter PgolTS has identical function to the part BBa_K310009 submitted by the team iGEM 2010 UIUC-Illinois [1]. However, our promoter is much cleaner as it does not contain non-promoter sequences which may interfere with transcription of the genes downstream. In addition, codon usage of our golS has been optimised specifically for E. coli to ensure efficient translation.

Introduction

Gold ions are toxic to most of the organisms and can cause serious environmental problems. The toxicity appears from interactions of gold ions with proteins and later on with the membrane causing the cells to lyse (1). Some of the microorganisms developed proteins that are sensitive to certain metal ions and can activated the expression of responsive elements. For example CueR from E. coli can bind to gold ions as well as copper ions (2). Due to lack of specificity this promoter is not very useful in synthetic biology. We decided to use part of the golT/S operon from Salmonella typhimurium, except for golT protein. This operon is regulated only by gold ions (3) therefore we took the promoter PgolT/S and transcription activator golS.

Characterization

The device has LacZ alpha which is useful for characterization. To determine activity of the part, beta-galactosidase assay was performed using PNPG as the substrate. In all experiments, untransformed E. coli strain DH5 alpha or strain BL21 were used as our negative control. The protocols are described in more detail on our wiki page [http://2013.igem.org/Team:York_UK/Notebook.html?page=protocols].

The experiments showed that E. coli strain DH5 alpha transformed with the device can respond to gold (AuCl4). In Figure 1A, production of the enzyme increased significantly in the presence of the full construct (DH5 alpha_AB) but reduced to the basal level in the absence of golS (DH5 alpha_A). This signifies the function of golS as a gold-dependent transcriptional activator.

In Figure 1B, E. coli strain BL21 has background expression of the enzyme. In contrast to the DH5 alpha (untransformed) and the DH5 alpha_B (transformed with golS), strong enzyme activities were observed in the absence of lacZ alpha - BL21 and BL21_B . This suggests that there may be beta-galactosidase in the chromosome of this E. coli strain.

In order to determine kinetics of the device, DH5 alpha were exposed to different gold concentrations for 16 hours to reach steady state. The response was non-linear with distinct phases - exponential phase (0.0uM - 2.5uM AuCl4), stationary phase (2.5uM - 10.0uM AuCl4) and logarithmic decline phase (not shown). According to the data, the device is very sensitive to the gold as low as 0.5uM; later on it became saturated from about 10uM onwards. This may be caused by intrinsic properties of the device. The data were fit to the nonlinear logistic model. In Figure 1C, simulated data were generated and plotted for comparison with the observations. For more information about modelling, please go to our wiki page [http://2013.igem.org/Team:York_UK/Notebook.html?page=modeling].

Figure 1D shows minimal activity of the promoter. What is more, it justifies the mathematical formulation of the model that there is no unknown process e.g. gold precipitation (between 0uM and 10uM AuCl4) otherwise the basal expression would be modified with increasing gold concentrations.

In Figure 2, we show streak plates of the E. coli strain DH5 alpha transformed with the whole device or one of the subparts. The growing media contained Xgal which turns blue in the presence of beta-galactosidase. It supports that PgolTS is the minimal unit for lacZ alpha expression.

Figures

IGEM York 2013 Figure1.jpg
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References

1. Goodman, C. M., McCusker, C. D., Yilmaz, T. & Rotello, V. M. Toxicity of Gold Nanoparticles Functionalized with Cationic and Anionic Side Chains. Bioconjugate Chem. 15, 897-900 (2004).

2. Stoyanpv, J. V. & Brown, N. L. The Escherichia coli copper-responsive copA promoter is activated by gold. J. Biol. Chem. 273, 1407-1410 (2003).

3. Wei, W. et al Engineering a gold-specific regulon for cell-based visual detection and recovery of gold. Chem. Sci. 3, 1780-1784 (2012). Sequence and Features


Assembly Compatibility:
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    COMPATIBLE WITH RFC[10]
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  • 21
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    Illegal AgeI site found at 701
  • 1000
    COMPATIBLE WITH RFC[1000]