Team:INSA Toulouse/contenu/project/biological construction/input

From 2013.igem.org

(Difference between revisions)
 
(11 intermediate revisions not shown)
Line 74: Line 74:
<div class="maincontent" style="width: 720px; margin: 25px 0 25px 0; float: right;">
<div class="maincontent" style="width: 720px; margin: 25px 0 25px 0; float: right;">
-
   <h1 class="title1">Biological Modules</h1>
+
   <h1 class="title1">Biological Modules: Input</h1>
-
   <h2 class="title2">Input</h2>
+
   <h2 class="title2"></h2>
-
   <p class="texte">For the input, it was needed to use a signal that can easily represents an “ON and OFF” switch. The use of lights to represent the inputs was our first idea: a blue and a red light.  
+
   <p class="texte">For the input, we needed a signal that could easily represents "ON" and "OFF" states. Light came as a natural solution because it is easily switchable to "ON" and "OFF" states and color can be varied to represent several inputs (A and B).
-
<br> <br> In the final E.calculus design, each sensor enables transcription of a specific recombinase (TP901 for the red sensor and Bxb1 for the blue sensor). </p>
+
<br> <br> In the final <i>E. calculus</i> design, each light sensor will promote the transcription of a specific recombinase (TP901 for the red sensor and Bxb1 for the blue sensor). </p>
    
    
<br>
<br>
   <p class="texte"><span class="spantitle">Blue light system </span></br>
   <p class="texte"><span class="spantitle">Blue light system </span></br>
-
<br> The blue light sensor uses the couple YF1-FixJ/FixK2 promoter. This couple was already used by iGEM11_Uppsala-Sweden team and described in literature (Andreas Möglich et al. 2009. <a href="http://www.ncbi.nlm.nih.gov/pubmed/19109976"> Design and Signaling Mechanism of Light-Regulated Histidine Kinases.</a>). YF1 is the fusion of the LOV protein and an histidine kinase. With no light, YF1 can phosphorylate FixJ and the phosphorylated FixJ activates the PfixK2 promoter. In presence of a 480 nm wavelength light, YF1 can no longer phosphorylate FixJ and there is no activation of the PfixK2 promoter. </p>
+
  <p class="texteleft"> <i> General principle</i>
 +
<br> The blue light sensor uses the couple YF1-FixJ/FixK2 promoter. This setup was already used by the iGEM11_Uppsala-Sweden team and also described in the litterature (<a href="http://www.ncbi.nlm.nih.gov/pubmed/19109976" target="_blank"> Andreas Möglich et al. 2009. Design and Signaling Mechanism of Light-Regulated Histidine Kinases.</a>). YF1 is the fusion of the LOV protein with an histidine kinase. In the absence of light, YF1 can activate FixJ (phosphorylaion) which in return activates the PfixK2 promoter. In the presence of a 480 nm wavelength light, YF1 can no longer phosphorylate FixJ leading to extinction of the PfixK2 promoter.
 +
  </p>
-
   <p class="texteleft"> <i> Blue light system characterization </i>
+
   <p class="texteright"> <i> Blue light module characterization </i>
-
<br> <br> To characterize the blue light sensor, a modified RFP was used as the output instead of the recombinase Bxb1. In darkness, RFP is supposed to be express whereas in presence of blue light, no RFP is transcripted. See the results on this page :  <a href="https://2013.igem.org/Team:INSA_Toulouse/contenu/lab_practice/results"> Results</a>
+
<br>To characterize the blue light sensor, a modified RFP was used as the output instead of the recombinase Bxb1. In darkness, RFP is supposed to be expressed whereas in the presence of blue light, no RFP should be produced. Results are described on <a href="https://2013.igem.org/Team:INSA_Toulouse/contenu/lab_practice/results/blue_sensor">this page</a>.
   </p>
   </p>
-
<img style="width:340px;" src="https://static.igem.org/mediawiki/2013/5/51/Blue_blue_blue_light.png" class="imgcontentright" />
+
<img style="width:700px;" src="https://static.igem.org/mediawiki/2013/thumb/3/35/Scheme_blue_sensor.jpg/800px-Scheme_blue_sensor.jpg" class="imgcontentright" />
Line 104: Line 106:
<br>
<br>
   <p class="texte"><span class="spantitle">Red light system</span></br>
   <p class="texte"><span class="spantitle">Red light system</span></br>
-
<br> The red light sensor uses CpH8, a chimeric receptor interacting with the promoter OmpC. CpH8 is the fusion of PCB photoreceptor and EnvZ histidine kinase (essential to be used in E.coli deficient in wild-type EnvZ). PCB requires biosynthesis of two genes : ho1 and PcyA. With no light, Cph8 is phosphylated and can activate the ompC promoter. In presence of a 660 nm wavelength light, cph8 is no longer phosphoryalated and can not activate the ompC promoter. (Levskaya A. and al. <a href="http://www.ncbi.nlm.nih.gov/pubmed/16306980">Synthetic biology: engineering Escherichia coli to see light.</a> 2005) </p>
+
      <p class="texteleft"><i>General principle</i>
 +
<br> The red light sensor uses CpH8, a chimeric receptor interacting with the promoter OmpC. CpH8 is the fusion of the PCB photoreceptor with the EnvZ histidine kinase. It is therefore essential to use a wild-type EnvZ deficient <i>E. coli</i>. The biosynthesis of PCB requires also two other genes : ho1 and PcyA. In the absence of light, Cph8 is phosphylated and can activate the OmpC promoter. In the presence of a 660 nm wavelength light, CpH8 is no longer phosphorylated and can not activate the OmpC promoter. (<a href="http://www.ncbi.nlm.nih.gov/pubmed/16306980" target="_blank">Levskaya A. and al. 2005. Synthetic biology: engineering Escherichia coli to see light.</a>) </p>
   <p class="texteright"><i>Red light system characterization</i>
   <p class="texteright"><i>Red light system characterization</i>
-
<br> <br> The system is similar to the blue light sensor, a modified RFP was used as the output instead of the recombinase TP901. In darkness, RFP is supposed to be express whereas in presence of red light, no RFP is transcripted. We succeed to obtain the construction but needed time to characterize it. More details here : <a href="https://2013.igem.org/Team:INSA_Toulouse/contenu/lab_practice/results"> Results</a>
+
<br> <br> The system is similar to the blue light sensor and a modified RFP was used as the output instead of the recombinase TP901. In darkness, RFP is supposed to be expressed whereas in presence of red light, no RFP is produced. We obtained the final construction but had not enough time to characterize it. More details here: <a href="https://2013.igem.org/Team:INSA_Toulouse/contenu/lab_practice/results/red_sensor"> Results</a></p>
-
  </p><img src="https://static.igem.org/mediawiki/2013/1/16/Light_system_-_red_-_340px.png" class="imgcontentleft" />
+
<img style="width:700px;" src="https://static.igem.org/mediawiki/2013/5/5a/Scheme_red_sensor.jpg" class="imgcontentleft" />

Latest revision as of 18:01, 4 October 2013

logo


Biological Modules: Input

For the input, we needed a signal that could easily represents "ON" and "OFF" states. Light came as a natural solution because it is easily switchable to "ON" and "OFF" states and color can be varied to represent several inputs (A and B).

In the final E. calculus design, each light sensor will promote the transcription of a specific recombinase (TP901 for the red sensor and Bxb1 for the blue sensor).


Blue light system

General principle
The blue light sensor uses the couple YF1-FixJ/FixK2 promoter. This setup was already used by the iGEM11_Uppsala-Sweden team and also described in the litterature ( Andreas Möglich et al. 2009. Design and Signaling Mechanism of Light-Regulated Histidine Kinases.). YF1 is the fusion of the LOV protein with an histidine kinase. In the absence of light, YF1 can activate FixJ (phosphorylaion) which in return activates the PfixK2 promoter. In the presence of a 480 nm wavelength light, YF1 can no longer phosphorylate FixJ leading to extinction of the PfixK2 promoter.

Blue light module characterization
To characterize the blue light sensor, a modified RFP was used as the output instead of the recombinase Bxb1. In darkness, RFP is supposed to be expressed whereas in the presence of blue light, no RFP should be produced. Results are described on this page.




Red light system

General principle
The red light sensor uses CpH8, a chimeric receptor interacting with the promoter OmpC. CpH8 is the fusion of the PCB photoreceptor with the EnvZ histidine kinase. It is therefore essential to use a wild-type EnvZ deficient E. coli. The biosynthesis of PCB requires also two other genes : ho1 and PcyA. In the absence of light, Cph8 is phosphylated and can activate the OmpC promoter. In the presence of a 660 nm wavelength light, CpH8 is no longer phosphorylated and can not activate the OmpC promoter. (Levskaya A. and al. 2005. Synthetic biology: engineering Escherichia coli to see light.)

Red light system characterization

The system is similar to the blue light sensor and a modified RFP was used as the output instead of the recombinase TP901. In darkness, RFP is supposed to be expressed whereas in presence of red light, no RFP is produced. We obtained the final construction but had not enough time to characterize it. More details here: Results

Retrieved from "http://2013.igem.org/Team:INSA_Toulouse/contenu/project/biological_construction/input"