Difference between revisions of "Team:Toulouse/Description/Regulation"

Revision as of 13:16, 17 September 2015

iGEM Toulouse 2015

Regulation

In order to respect the bee life cycle and to optimize our solution fighting Varroa destructor infestation of domestic bees, we have integrated a regulation system to our genetic construction: a day/night (or circadian) switch. In daytime, the bees are working outside to pollinate, and so, go back and forth at the beehive entrance, bringing potentially varroas inside the hive. In nighttime, bees are less active. Hence, we want our ApiColi to produce either butyric acid in daytime to attract varroa toward a physical trap, or formic acid to kill it by night.

We based our reflexion on a light response system built in E. coli [1] The genetic system has been designed to be switched on and off in response to light[2]. In our project, we have further improved the process in order to control two alternative genetic programs depending on light.

The core of the light sensor is composed of the membrane proteins PCB and Cph8. PCB is a chromophore (phycocyabilin) originating from cyanobacteria Synechocystis sp. PCC 6803. Cph8 is a hybrid protein between the red light response domain of Cph1 (a phytochrome-like protein from Synechocystis sp PCC 6803) and the intracellular domain of the histidin kinase EnvZ (an osmolarity sensor protein) from E. coli. The synthesis of PCB requires the expression of both Ho1 (heme oxygenase gene) and PcyA (biliverdin reductase gene). [3]

Light and Dark conditions

When there is no light, Cph8 autophosphorylates its EnvZ intracellular domain while consuming one molecule of ATP. The phosphoryl group will be subsequently transferred to the transcription factor OmpR, which then, will upregulate genes expressed from the OmpC promoter.
On the contrary, when there is light, PCB prevents the Cph8 autophosphorylation. Hence OmpR is not activated and there is no expression of genes under P_OmpC control.

This circadian switch is further enhanced with a combination of cI repressor and lacI repressor which enables ApiColi to produce butyric acid (polycistron B) when there is light, while formic acid is not produced, and conversely to produce formic acid (polycistron A) during the night and no butyric acid. Without light, polycistronic A genes, corresponding to the formate pathway, are transcribed The first protein, encoded by the cI gene downregulates the P_Lac promotor, hence, the polycistronic gene B is not transcribed. When there is light, there is no more expression of the polycistronic gene A, thus there is no more repression of the polycistronic gene B. Thus, there is production of butyrate via the expression of polycistronic gene B. In this same genetic element, there is a protein that represses the polycistronic gene A expression.

References

[1] 2005 Nature, levskaya, synthetic biology: engineering E. coli to see light
[2] 2013 PLOS, lee switchable gene expression in E. coli using a miniaturized photobioreactor
[3] PNAS, 2001, gabetta, Genetic engineering of phytochrome biosynthesis in bacteria

@@ Line 67: / Line 67: @@
 bees, we have integrated a regulation
 system to our genetic construction: <b>a day/night (or circadian) switch</b>.
-During the day, the bees are working outside doing pollination,
+In daytime, the bees are working outside to pollinate,
-so they make back and forth at the beehive entrance.
+and so, go back and forth at the beehive entrance, bringing potentially varroas inside the hive.
-This is when they can bring varroas into the hive.
+In nighttime, bees are less active. Hence,
-During the night they are less active. Hence,
+we want our <b>ApiColi</b> to produce either butyric acid in daytime to
-we want our <b>ApiColi</b> to produce butyric acid to
+attract varroa toward a physical trap, or formic acid to kill it by night.
-attract varroa into the physical trap by day, and formic acid to kill it by night.
 </p>
@@ Line 90: / Line 89: @@
 We based our reflexion on a light response system built in E. coli [1]
-This system has then been used to design a genetic response
+The genetic system has been designed to be switched on and off in response to light[2].
-that can be switched on and off by light [2].
+In our project, we have further improved the
-In our project, we have further enhanced the
+process in order to control two
-process in order to be able to produce two
+alternative genetic programs depending on light.
-different genetic expressions depending on light.
 <br>
 <br>
@@ Line 102: / Line 100: @@
 originating from cyanobacteria
 <i>Synechocystis sp.</i> PCC 6803. Cph8
-is the result of the fusion between
+is a hybrid protein between
 the <b>red light response domain of Cph1</b>
-(a phytochrome-like protein that comes
+(a phytochrome-like protein
 from Synechocystis sp PCC 6803) and the
-<b>intracellular histidin kinase EnvZ</b>
+<b>intracellular domain of the histidin kinase EnvZ</b>
 (an osmolarity sensor protein) from <i>E. coli.</i></b>
-Synthesis of PCB requires the expression of Ho1
+The synthesis of PCB requires the expression of both Ho1
 (heme oxygenase gene) and PcyA (biliverdin reductase gene). [3]
 </p>
@@ Line 119: / Line 117: @@
 <div class="group center">
 <p align="justify" style="font-size:15px;">
-When there is no light, Cph8 autophosphorylates its intracellular EnvZ domain while consuming one molecule of ATP. This activates the transcription factor OmpR by transferring its phosphate to it. OmpR-P therefore upregulates genes under control of the promoter P<sub>OmpC</sub>.
+When there is no light, Cph8 autophosphorylates its EnvZ intracellular domain while consuming one molecule of ATP. The phosphoryl group will be subsequently transferred to the transcription factor OmpR, which then, will upregulate genes expressed from the OmpC promoter.
 <br>
 On the contrary, when there is light, PCB prevents the Cph8 autophosphorylation. Hence OmpR is not activated and there is no expression of genes under P<sub>OmpC</sub> control.