Difference between revisions of "Team:Technion Israel/Modifications/narx"

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As the results showed that NarX-Tar strain failed to show any response to sodium nitrate. Moreover, as the reporter gene (GFP) showed no indication of expression, this subproject was put aside.
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It is unfortunate that the NarX-Tar clone wasn't successful, as it could have served as an additional proof of concept the S.Tar platform, in addtion to the other strains we have cloned.
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Revision as of 10:19, 16 October 2016

S.tar, by iGEM Technion 2016

S.Tar, by iGEM Technion 2016

Introduction

The NarX sensor protein of E. coli binds nitrite and nitrate and induces the expression of proteins involved in anaerobic respiration (1). As a proof of concept of our platform, the Tar chemoreceptor LBD was replaced with the NarX LBD. A protocol which was previously shown to be successful has been recovered (1). This work resulted in a NarX-Tar chimera, comprised by the NarX LBD and Tar’s cytoplasmic region. The chimera was supposed to function as a repellent chemoreceptor to nitrite and nitrate.

Design and Implementation

To produce this chimera, the protein sequence of both the LBD and the linker region of NarX were obtained from the literature (1). Using the DNA sequences of both mentioned segments and Tar’s cytoplasmic region, that were obtained from the complete E. coli genome sequence (2)

we built a Biobrick device (part not submitted) which was then transformed to bacteria that lacks chemoreceptors - UU1250 (Parkinson J S, University of Utah). The transformation was followed by different assays in order to test the chemotactic ability of the chimera. As in the PctA, first a 3D model was generated using the website Phyre2, to insure the correct folding of all parts of the chimera. Later, a “Chip Microscope assay” was conducted. In this assay a suspension of the bacteria was confined into an “ibidi” microchannel chip and the bacterial concentration was monitored in a fixed point for the whole experiment. Later on, a solution of a repellent, sodium nitrate, in the concentrations of 10-2M and 10-6Mwas added to the channel. .

Lastly, GFP was fused to the NarX-Tar chimera's C terminus in order to validate the location of the expressed chemoreceptor on the both poles of the bacterial membrane. The reporter protein was monitored using fluorescence microscopy followed by a FACS.

Results

The results of the 3D structure were not promising, as the folding was not achieved in the correct manner as can be seen in figure 1. The expected results of the Chip Microscope assay were a decrease of the bacterial concentration overtime. Nevertheless, the strain showed no response to different concentrations of sodium nitrate, in other words it chimera did not function as expected. Lastly, the testing of the clone carrying the GFP fused to the chimera both with the FACS and fluorescence microscopy showed no indication to fluorescence, as can be seen in figure 2.

Outlook

As the results showed that NarX-Tar strain failed to show any response to sodium nitrate. Moreover, as the reporter gene (GFP) showed no indication of expression, this subproject was put aside. It is unfortunate that the NarX-Tar clone wasn't successful, as it could have served as an additional proof of concept the S.Tar platform, in addtion to the other strains we have cloned.



Referances

1. R Ward, S.M., Delgado, A., Gunsalus, R.P., and Manson, M.D. (2002). A NarX-Tar chimera mediates repellent chemotaxis to nitrate and nitrite. Mol. Microbiol. 44, 709–719.

2. The complete E coli genome sequence.



S.tar, by iGEM Technion 2016