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| + | |
| + | <div style="width:100%;"><font style="font-size:15px;font-weight:500;">Show all:</font></div> |
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| + | <a href="#showmodelling"><div class="orange_news_block1 showmodelling" style="background: #F9A7B0;border-radius:15px;color:black;float:left;height:40%;width:40%;margin-left:6%;padding-top:5%;margin-top:3px;"><center> |
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| + | </div></a> |
| + | <br><br><br><br><br> |
| + | </div> |
| + | <br> |
| + | <h1>Introduction: how we constructed our biosensor</h1> |
| + | In order to be able to use our model and to determine whether DcmR acts as a repressor or activator in the presence of DCM we designed and constructed the following two plasmid system. We primarily used Gibson assembly methods and source most of the necessary DNA from gblocks(synthesised oligonucleotides) we had designed based in the sequenced genome of Methylobacterium DM4. This system will also form the DCM biosensor and will be integrated with an electronic circuit to complement this genetic one:<br><br> |
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- | <h1>Introduction: what are we optimising?</h1>
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- | Having started by characterizing the genetic circuit of our system, we now focused our attention on developing the most effective biosensor for our system. Mathematical modelling was crucial in both maximizing the efficiency of the design process and guiding the experiments carried out in the wet lab.
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- | <br><br>
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- | Having characterized the genetic circuit <a href="https://2014.igem.org/Team:Oxford/biosensor_characterisation">(see the characterisation section)</a>, the next steps were to:
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- | <br><br>
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- | • Analyse the behaviour of our system in the presence of different quantities of input.<br>
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- | • Guide the biochemists in the selection process of variables such as Ribosome Binding Strength (RBS) to maximize the performance of our biosensor.
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- | <br><br>
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- | As previously stated, the power of computer modelling was highlighted during the design of our biosensor. Having built models of the biosensor system, we could then use them to predict its behaviour under different conditions and for a range of different values for variable parameters such as activation and degradation rates of our genes. This was crucial in saving both time and money- eliminating the need to run each of these variable combinations in a lab.
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- | <h1black>Insert biochem here?</h1black> | + | <h1white>Insert biochem here?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
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- | <h1black>Insert biochem here?</h1black></div></a> | + | <h1white>Insert biochem here?</h1white></div></a> |
| <div class="list"> | | <div class="list"> |
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| <h1>Biochemistry...</h1> | | <h1>Biochemistry...</h1> |
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| <h1white>What happens when we change the amount of each input added?</h1white> | | <h1white>What happens when we change the amount of each input added?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
| </div></a> | | </div></a> |
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| <h1white>What happens when we change the amount of each input added?</h1white></div></a> | | <h1white>What happens when we change the amount of each input added?</h1white></div></a> |
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| <img src="https://static.igem.org/mediawiki/2014/5/51/Oxford_varying_ATC_and_DCM.png" style="margin-left:0%; float:right; margin-right:0%; position:relative; width:45%;" /> | | <img src="https://static.igem.org/mediawiki/2014/5/51/Oxford_varying_ATC_and_DCM.png" style="margin-left:0%; float:right; margin-right:0%; position:relative; width:45%;" /> |
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- | <h1black>Insert biochem here?</h1black> | + | <h1white>Insert biochem here?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
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| <h1>Biochemistry...</h1> | | <h1>Biochemistry...</h1> |
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| <h1white>Modelling the biosensor to optimise ’ON’ and ‘OFF’ response</h1white> | | <h1white>Modelling the biosensor to optimise ’ON’ and ‘OFF’ response</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
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- | <h1white>Modelling the biosensor to optimise ’ON’ and ‘OFF’ response</h1white> | + | <h1white>Modelling the biosensor to optimise ’ON’ and ‘OFF’ response</h1white></div></a> |
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| As described above, the ideal biosensor is binary and its fluorescence response can only take two values. This relies on the system having two feature- a fast response time to concentration changes and a large amplitude of response. Having previously established the ideal concentrations of DCM and ATC <u>(see above)</u> for the biosensor, our next task was to predict what combination of controllable variables would result in the ideal binary behaviour. This is a very important step in synthetic biology because it allows us to crudely optimise the design before construction even begins. To test the response of our biosensor, we used a step function of DCM the initial and sudden contact of DCM with our bacteria and then removing DCM through <u>spinning the cells(?)</u>. In the real system, the DCM input would be a step in and then a gradual negative ramp as the DCM was degraded. | | As described above, the ideal biosensor is binary and its fluorescence response can only take two values. This relies on the system having two feature- a fast response time to concentration changes and a large amplitude of response. Having previously established the ideal concentrations of DCM and ATC <u>(see above)</u> for the biosensor, our next task was to predict what combination of controllable variables would result in the ideal binary behaviour. This is a very important step in synthetic biology because it allows us to crudely optimise the design before construction even begins. To test the response of our biosensor, we used a step function of DCM the initial and sudden contact of DCM with our bacteria and then removing DCM through <u>spinning the cells(?)</u>. In the real system, the DCM input would be a step in and then a gradual negative ramp as the DCM was degraded. |
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- | <h1black>Insert biochem here?</h1black> | + | <h1white>Insert biochem here?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
| </div></a> | | </div></a> |
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- | <h1black>Insert biochem here?</h1black></div></a> | + | <h1white>Insert biochem here?</h1white></div></a> |
| <div class="list"> | | <div class="list"> |
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| <h1>Biochemistry...</h1> | | <h1>Biochemistry...</h1> |
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- | <h1white>Should we aim for high or low RBS strength?</h1white> | + | <h1white>Should we aim for high or low RBS strength?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
| </div></a> | | </div></a> |
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- | <h1white>Should we aim for high or low RBS strength?</h1white> </div></a> | + | <h1white>Should we aim for high or low RBS strength?</h1white></div></a> |
| <div class="list"> | | <div class="list"> |
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| <img src="https://static.igem.org/mediawiki/2014/e/e8/Oxford_change_RBS_strength.png" style="margin-left:0%; float:right; margin-right:0%; position:relative; width:65%;" /> | | <img src="https://static.igem.org/mediawiki/2014/e/e8/Oxford_change_RBS_strength.png" style="margin-left:0%; float:right; margin-right:0%; position:relative; width:65%;" /> |
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- | <h1black>Insert biochem here?</h1black> | + | <h1white>Insert biochem here?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
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- | <h1black>Insert biochem here?</h1black></div></a> | + | <h1white>Insert biochem here?</h1white></div></a> |
| <div class="list"> | | <div class="list"> |
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| <h1>Biochemistry...</h1> | | <h1>Biochemistry...</h1> |
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- | <h1white>Should we aim for high or low degradation rate?</h1white> | + | <h1white>Should we aim for high or low degradation rate?</h1white> |
| <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> | | <img src="https://static.igem.org/mediawiki/2014/4/4d/Oxford_plus-sign-clip-art.png" style="float:right;position:relative; width:2%;" /> |
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| <img src="https://static.igem.org/mediawiki/2014/6/67/Oxford_change_degradation_rate.png" style="margin-left:0%; float:right; margin-right:0%; position:relative; width:65%;" /> | | <img src="https://static.igem.org/mediawiki/2014/6/67/Oxford_change_degradation_rate.png" style="margin-left:0%; float:right; margin-right:0%; position:relative; width:65%;" /> |
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| In an ideal world, we would like to have a very high expression rate (for a high steady state amplitude of fluorescence), a high degradation rate (for a fast responding biosensor) and a high copy number of the plasmid in each cell. Conversely though, optimising these parameters puts stress on the cells. This leads to the system not actually being as optimal as the model might have predicted. Here we identify the weakness in preliminary models. We will have to actually develop the bacteria and run the experiments in the lab before we will know if our biosensor will respond this well to the DCM. After this, we will work at creating secondary models which should be able to give more reliable predictions. Ideally we would be able to then make more bacteria and the Engineering-Biochemistry cycle would continue. | | In an ideal world, we would like to have a very high expression rate (for a high steady state amplitude of fluorescence), a high degradation rate (for a fast responding biosensor) and a high copy number of the plasmid in each cell. Conversely though, optimising these parameters puts stress on the cells. This leads to the system not actually being as optimal as the model might have predicted. Here we identify the weakness in preliminary models. We will have to actually develop the bacteria and run the experiments in the lab before we will know if our biosensor will respond this well to the DCM. After this, we will work at creating secondary models which should be able to give more reliable predictions. Ideally we would be able to then make more bacteria and the Engineering-Biochemistry cycle would continue. |
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