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- | <td><p class="STYLE19">The design for the cell I: The genetic circuit can be divided into three different functional sections. <br> | + | <td bgcolor="#03438A"><p class="STYLE19">The design for the cell I: The genetic circuit can be divided into three different functional sections. <br> |
Cell 2 is similarly designed as Cell 1.</p> </td> | Cell 2 is similarly designed as Cell 1.</p> </td> | ||
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- | <td><p class="STYLE19">The first one in the graph is the detecting Section. By using this section you can detect the cell density according to the intensity of the red fluorescence. The detecting section is especially useful when you incubate two different kinds of E.coli in a coculture.</p> | + | <td bgcolor="#03438A"><p class="STYLE19">The first one in the graph is the detecting Section. By using this section you can detect the cell density according to the intensity of the red fluorescence. The detecting section is especially useful when you incubate two different kinds of E.coli in a coculture.</p> |
<p class="STYLE19">The second section is the Helper section. We call it helper section because the LuxR protein is the prerequisite for the activation of PLux. Here we used a constitutive promoter to express the LuxR protein. The core section is the toggle switch. Toggle switch is a genetic device that can switch between two convertible states, which, here, represents a different survival strategy for the cells each. </p> | <p class="STYLE19">The second section is the Helper section. We call it helper section because the LuxR protein is the prerequisite for the activation of PLux. Here we used a constitutive promoter to express the LuxR protein. The core section is the toggle switch. Toggle switch is a genetic device that can switch between two convertible states, which, here, represents a different survival strategy for the cells each. </p> | ||
<p class="STYLE19"></p></td> | <p class="STYLE19"></p></td> | ||
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- | <td><span class="STYLE19">When adding Arobinose/AHL different genes will get expressed behind the two mutually-repressive promoters. That means when added into the culture AHL will diffuse into the cell bind the LuxR protein and form a complex which can activate the LuxPr promoter and then the genes of rhII capR and araC will get expressed. Then the araC protein will bind to the PBad/araC promoter and repress the expression of the aiiA and another capR gene. However, you can turn the switch to the other side by adding Arobinose. When adding arobinose into the culture, the repression functional molecular AraC protein will get released from the PBad/AraC promoter. With the expression of the aiiA gene the signal molecular will get digested and therefore decrease to a proper level which is not high enough to activate the LuxPr promoter.<br> | + | <td bgcolor="#03438A"><span class="STYLE19">When adding Arobinose/AHL different genes will get expressed behind the two mutually-repressive promoters. That means when added into the culture AHL will diffuse into the cell bind the LuxR protein and form a complex which can activate the LuxPr promoter and then the genes of rhII capR and araC will get expressed. Then the araC protein will bind to the PBad/araC promoter and repress the expression of the aiiA and another capR gene. However, you can turn the switch to the other side by adding Arobinose. When adding arobinose into the culture, the repression functional molecular AraC protein will get released from the PBad/AraC promoter. With the expression of the aiiA gene the signal molecular will get digested and therefore decrease to a proper level which is not high enough to activate the LuxPr promoter.<br> |
The most important thing in this section is the capacity of the two different promoters LuxPr and PBad/araC are quite different. When the LuxRr promoter is activated, its higher capacity will express more chloromycetin resistant protein and another important thing is by sensing the AHL which is sent out by cell-two it can produce another kind of signal molecular BHL. | The most important thing in this section is the capacity of the two different promoters LuxPr and PBad/araC are quite different. When the LuxRr promoter is activated, its higher capacity will express more chloromycetin resistant protein and another important thing is by sensing the AHL which is sent out by cell-two it can produce another kind of signal molecular BHL. | ||
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- | <td colspan="2"><p><strong><span class="STYLE7">Mutualism and <a name="OLE_LINK1">Competition</a></span></strong></p></td> | + | <td colspan="2" bgcolor="#03438A"><p><strong><span class="STYLE7">Mutualism and <a name="OLE_LINK1">Competition</a></span></strong></p></td> |
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- | <td width="408"><p class="STYLE19"><strong>Competition</strong></p> | + | <td width="408" bgcolor="#03438A"><p class="STYLE19"><strong>Competition</strong></p> |
<p class="STYLE15"> In the culture that both ampicillin and chloromycetin are available, it requires the expression of the both the resistant genes for both antibiotics for a strain’s survival. Without adding any signal molecular as the initially inducing factor into the culture the two kinds of E.coli can not communicate with each other so they will keep on the competent stage. In this stage each kind of cell must survive all by it self in some method as assimilating the nutrition in the culture. As a result the two different kinds of E.coli fight with each other for the space and nutrient ingredient. </p> | <p class="STYLE15"> In the culture that both ampicillin and chloromycetin are available, it requires the expression of the both the resistant genes for both antibiotics for a strain’s survival. Without adding any signal molecular as the initially inducing factor into the culture the two kinds of E.coli can not communicate with each other so they will keep on the competent stage. In this stage each kind of cell must survive all by it self in some method as assimilating the nutrition in the culture. As a result the two different kinds of E.coli fight with each other for the space and nutrient ingredient. </p> | ||
<p class="STYLE15">By adding some AHL into the culture, the LuxPr promoter will get activated by the AHL and LuxR complex. And then the expression product of the rhlI gene BHL will diffuse into the cell-two which can sense BHL-RhIR complex by binding to the PrhI promoter and turning on the expression of luxI kanR and lacI genes. The LacI protein will bind to the PBad/araC promoter and therefore stop the digestion of the signal molecular by the expression of the aiiA gene. At the same time the expression of the luxI gene will send out AHL .By using a very similar mechanism the cell-one can sense the AHL molecular.</p></td> | <p class="STYLE15">By adding some AHL into the culture, the LuxPr promoter will get activated by the AHL and LuxR complex. And then the expression product of the rhlI gene BHL will diffuse into the cell-two which can sense BHL-RhIR complex by binding to the PrhI promoter and turning on the expression of luxI kanR and lacI genes. The LacI protein will bind to the PBad/araC promoter and therefore stop the digestion of the signal molecular by the expression of the aiiA gene. At the same time the expression of the luxI gene will send out AHL .By using a very similar mechanism the cell-one can sense the AHL molecular.</p></td> | ||
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- | <td><p class="STYLE19"><strong>Mutualism</strong> <br> | + | <td bgcolor="#03438A"><p class="STYLE19"><strong>Mutualism</strong> <br> |
In this state the two kinds of cells communicate with each other by sensing the signal molecular sent by the counterpart.<br> | In this state the two kinds of cells communicate with each other by sensing the signal molecular sent by the counterpart.<br> | ||
It seems that with the help of each other both of them can live better in the harsh environment and the fact is the capacity of the LuxPr and PrhI are higher the than the Plac and Pbad/araC promoters. With higher expression of the ampicillin and chloromycetin resistant protein both of them can survive in the ultra-high antibiotic concentration. </p></td> | It seems that with the help of each other both of them can live better in the harsh environment and the fact is the capacity of the LuxPr and PrhI are higher the than the Plac and Pbad/araC promoters. With higher expression of the ampicillin and chloromycetin resistant protein both of them can survive in the ultra-high antibiotic concentration. </p></td> | ||
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- | <td><span class="STYLE11"><span class="STYLE4"><strong> | + | <td bgcolor="#03438A"><span class="STYLE11"><span class="STYLE4"><strong> |
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- | <td width=" | + | <td width="477"><div align="center"><span class="STYLE17"><a href="https://2008.igem.org/Experiment">Experiment</a></span> </div></td> |
- | <td width=" | + | <td width="493"><div align="center"><a href="https://2008.igem.org/Modle" class="STYLE18">Model</a></div></td> |
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Revision as of 11:38, 28 October 2008
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This idea was inspired by the theory of Prisoner’s Dilemma. As in prisoners’ dilemma, the bacteria in our design are faced with two solutions for coexistence, they could either choose to cooperate with one another by providing inducers to express their partners’ antibiotics-resistance genes or they could take a foe strategy in which no cooperation is needed for both strains’ survival. |
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