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<a href="#Solution">Solution</a> | <a href="#Solution">Solution</a> | ||
<a href="#Our Design">Our Design</a> | <a href="#Our Design">Our Design</a> | ||
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<h1>Introduction</h1> | <h1>Introduction</h1> | ||
<!-- <h2 style="text-align: left;"> The Impacts of Excess Fluoride:</h2> --> | <!-- <h2 style="text-align: left;"> The Impacts of Excess Fluoride:</h2> --> | ||
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− | <p2 style="font-size:18px;"> Granite and volcanic rocks are extremely high in fluoride | + | |
+ | <p2 style="font-size:18px;"> Granite and volcanic rocks are extremely high in fluoride due to large amounts of fluoride-rich minerals including biotite, fluorite, amphibole, and apatite. These high-fluoride rock deposits rise through faults and hot springs into groundwater. Prolonged exposure to high levels of fluoride correlates to diseases such as dental and skeletal fluorosis. These diseases can severely impact young children, whose enamel is still developing. Please see our interview with <a href="https://2018.igem.org/Team:East_Chapel_Hill/MaikoSuzuki">Maiko Suzuki</a> to learn specifically how fluorosis manifests in the teeth. | ||
<br><br> | <br><br> | ||
− | Unfortunately, mitigating fluoride problems has proven to be very expensive and challenging | + | Unfortunately, mitigating fluoride problems has proven to be very expensive and challenging. One of the issues we are attempting to address with our project is diligently tracking fluoride concentrations after treatment attempts. In rural communities, even once there has been treatment to high-fluoride water, it is difficult to monitor fluoride concentrations after the treatment. |
<br><br> | <br><br> | ||
<a name="Solution"></a> | <a name="Solution"></a> | ||
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<h1> Our Design </h1> | <h1> Our Design </h1> | ||
<p2 style="font-size:18px;"> | <p2 style="font-size:18px;"> | ||
+ | <p2 style="text-align:left;" font-size:18px;"> | ||
We modified the previously developed chloramphenicol acetyltransferase operon (CHOP) by the 2017 East Chapel Hill iGem. We used Gibson overhangs with homology to pSB1A3 so we could clone the operon into the pSB1A3 vector. This operon was designed so that future users may easily test a library of promoters and riboswitches simply by cutting with restriction enzyme HindIII. One may even test the expression of a new gene by using the XhoI restriction enzyme. | We modified the previously developed chloramphenicol acetyltransferase operon (CHOP) by the 2017 East Chapel Hill iGem. We used Gibson overhangs with homology to pSB1A3 so we could clone the operon into the pSB1A3 vector. This operon was designed so that future users may easily test a library of promoters and riboswitches simply by cutting with restriction enzyme HindIII. One may even test the expression of a new gene by using the XhoI restriction enzyme. | ||
</p2> | </p2> | ||
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<img src="https://static.igem.org/mediawiki/2018/d/d1/T--East_Chapel_Hill--OPERON.png" style="width:75%;height:auto;"> | <img src="https://static.igem.org/mediawiki/2018/d/d1/T--East_Chapel_Hill--OPERON.png" style="width:75%;height:auto;"> | ||
− | <figcaption> <I>Schematic of operon BBa_K2843000 | + | <figcaption> <I>Schematic of operon BBa_K2843000</I> |
− | + | </figcaption> | |
− | + | </figure> | |
− | + | </center> | |
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− | </ | + | <p2 style="text-align:left;" font-size:18px;"> |
− | <a | + | The fluoride binding mutant has two point mutations that prevent the antiterminator loop from forming. Therefore, fluoride can’t bond and there should be no growth. This acts as a control to verify that bacterial growth is directly a result of fluoride concentrations. |
− | < | + | <br><br><br> |
− | + | <img src="https://static.igem.org/mediawiki/2018/c/c1/T--East_Chapel_Hill--LOWFBM.png" style="width:75%;height:auto;"> </img> | |
− | + | <figcaption> <I>The figure above shows the conserved fluoride riboswitch</I> | |
+ | <br><br><br> | ||
+ | <img src="https://static.igem.org/mediawiki/2018/a/aa/T--East_Chapel_Hill--fbmhighfluoride.png" style="width:75%;height:auto;"> | ||
+ | <figcaption> <I>The figure above shows the 2 point mutation of the fluoride riboswitch, creating the fluoride binding mutant</I> | ||
+ | <br></br><br></br> | ||
+ | </p2> | ||
</html> | </html> |
Latest revision as of 03:38, 18 October 2018
Description
Introduction
Unfortunately, mitigating fluoride problems has proven to be very expensive and challenging. One of the issues we are attempting to address with our project is diligently tracking fluoride concentrations after treatment attempts. In rural communities, even once there has been treatment to high-fluoride water, it is difficult to monitor fluoride concentrations after the treatment.
We hope that the operon we have developed may assist the monitoring of fluoride concentrations in small, low-technology villages after treatment of the water has been administered.
Solution
About the Riboswitch
Riboswitches may be translational or transcriptional. A transcriptional riboswitch has a “switching sequence” in the aptamer that directs the formation of a transcriptional terminator, which signals to RNA polymerase to stop transcription. One may think of this process as an “on” or “off” switch, with “on” allowing for transcription of a gene. When the aptamer (ligand-binding) region of the fluoride riboswitch interacts with fluoride, the terminator is not formed allowing the RNA polymerase to proceed and transcribe the downstream gene.
In nature, this riboswitch regulates the expression of genes that are able to pump high levels of fluoride out of the cell. The crcB gene in E.coli bacteria encodes the fluoride efflux channel, which is capable of pumping fluoride out of the cell so that it is no longer toxic. In our experiments, we used a modified crcB E.coli strain so that fluoride may accumulate in the cell.