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<a class="navi" href="https://2015.igem.org/Team:Manchester-Graz/Project/Experiments"><img src="https://static.igem.org/mediawiki/2015/3/30/Manchester-Graz_Experiments.jpg"></a>
 
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<div id="twitterboxsmall"><a class="twitter-timeline" href="https://twitter.com/iGEMMancGraz" data-widget-id="619465263411499008" height="900" width="180">Tweets by @iGEMMancGraz</a> <script>!function(d,s,id){var js,fjs=d.getElementsByTagName(s)[0],p=/^http:/.test(d.location)?'http':'https';if(!d.getElementById(id)){js=d.createElement(s);js.id=id;js.src=p+"://platform.twitter.com/widgets.js";fjs.parentNode.insertBefore(js,fjs);}}(document,"script","twitter-wjs");</script>
 
<div id="twitterboxsmall"><a class="twitter-timeline" href="https://twitter.com/iGEMMancGraz" data-widget-id="619465263411499008" height="900" width="180">Tweets by @iGEMMancGraz</a> <script>!function(d,s,id){var js,fjs=d.getElementsByTagName(s)[0],p=/^http:/.test(d.location)?'http':'https';if(!d.getElementById(id)){js=d.createElement(s);js.id=id;js.src=p+"://platform.twitter.com/widgets.js";fjs.parentNode.insertBefore(js,fjs);}}(document,"script","twitter-wjs");</script>
 
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<h1>Vector design</h1>
 
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<p> <div id="pictureright"><img src="https://static.igem.org/mediawiki/2015/d/d3/System_new_website.png" alt="System_new" width="500"><br><b>Figure 1</b> Schematic representation of our quorum sensing based regulatory system.</div></p>
 
<p style="text-align:justify">Our vector is based on two quorum sensing (QS) systems. The EsaR/I system belongs to the plant pathogen <i>Pantoea stewartii</i>, formerly known as <i>Erwinia stewartii</i>, the causative agent of Stewart’s Wilt(1). Contrary to common QS-systems EsaR/I uses a repressor based rather than an activator-based system. EsaR binds to its corresponding binding sites on the PesaRC promoter and represses the expression of the genes under the promoter’s control (2,3). When a certain concentration of 3-oxohexanoyl-homoserinelactone (3OC6-HSL) that is produced by the EsaI-synthase, is reached, it leads to an allosteric confirmation change in EsaR’s structure that inhibits its repressor function. When positioned in the -60 region of the PesaS-promoter EsaR can also work as an activator too, by facilitating RNA-polymerase recruitment (2). <br><br></p>
 
  
<p style="text-align:justify">The second QS-System we are using, CepR/I, belongs to the opportunistic pathogen <i>Burkholderia cenocepacia</i>. Similar to the LuxR/I system, CepR acts as an activator of its corresponding promoter, PaidA, when a certain level of octanoyl-homoserinelactone (C8-HSL) is reached (4). C8-HSL is produced by CepI. CepR also binds 3OC6-HSL, however will not work as an activator, as the additional two carbon-atoms are mandatory, for CepR’s RNA-Polymerase-recruiting ability (4). This way CepR works as an competitive binding site for 3OC6-HSL, that putatively allows us to reach higher cell densities and thus higher 3OC6-HSL concentration before the EsaR/I expression system gets activated. <br><br></p>
 
  
<p style="text-align:justify">Our vector is designed in a way that EsaR, EsaI and CepR are constitutively expressed by the PesaS-promoter. As long as the 3OC6-HSL concentration is low enough, EsaR will additionally increase its own transcription, creating a positive feedback loop. <div id="pictureleft" style="height:160px;"><img src="https://static.igem.org/mediawiki/2015/7/7a/Manchester-Graz_HSL_website.png" alt="HSL" width="350"><br> <b>Figure 2</b> Homoserinelactone synthesis by EsaI and CepI.</div> <p style="text-align:justify">When the 3OC6-HSL threshold is reached, transcription of the PesaRC initiates, while the PesaS-feedback loop is turned off. The activation of the promoter is shown and measured on the expression of cyan fluorescent protein (CFP). Additionally to the reporter gene also CepI gets expressed, resulting in the time-shifted activation of our second QS-system. When the C8-HSL threshold is reached, CepR can work as an activator of the PaidA promoter that transcribes monomer red fluorescent protein (mRFP) as a second reporter gene. <br>
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To avoid any leaky read through of transcription terminators, the constitutively expressed transcripts of the regulatory proteins of the two QS-systems as well as the beta-lactamase resistance marker, are positioned in the opposite direction of the auto-induced PaidA – and PesaRC –promoter (Figure 3). <br>Additionally PaidA is placed upfront of PesaRC. All reporter genes can easily be replaced by any other genes by standard cloning techniques. <br></p></p>
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<h1 style="margin-bottom: 60px;"> Project Outlines</h1>
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<div id="pictureright"> <img src="https://static.igem.org/mediawiki/2015/b/b3/Manchester-Graz_Human-Gutbacteria.jpg" alt="human gut bacteria" width="400"> <br> <b> Fig 1 </b>Administration of L-DOPA via bacteria in the patient's gut</div>
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<p style="text-align:justify">iGEM Manchester-Graz’s objective as a team is to find a better way to treat and alleviate the symptoms of Parkinson’s disease (PD) through the use of synthetic biology. Degradation of dopaminergic neurons and therefore low levels of dopamine is the main cause of Parkinson’s disease (PD), for which the current treatment involves oral doses of L-DOPA (or levodopa), which unlike dopamine itself is able to cross the blood-brain-barrier. Within the brain L-DOPA is enzymatically converted into dopamine and therefore able to relieve many of the motor symptoms of PD (Figure 1).</p>
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<p style="text-align:justify">Our aim is to take the first steps in the development of a novel technology of drug delivery by developing self-regulating drug-producing bacterial strains that, in the future, could be incorporated into patients’ gut microflora to secrete medicines directly inside the body. To control the bacterial L-DOPA production, we plan to develop a multidimensional cell density dependent auto-regulation system that could also be used to control other multistep enzyme pathways.</p>
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<div id="pictureleft"><img src="https://static.igem.org/mediawiki/2015/e/ef/Manchester-Graz_Pathway.jpg" alt="Pathway" width="300"> <br><b> Fig 2 </b>dopamine and L-DOPA biosynthesis pathways</div>
  
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<p style="text-align:justify">The Manchester section of the team are working on L-DOPA and dopamine biosynthesis in <i>E. coli </i>BL21 and Nissle 1917 via various enzyme pathways. The focus is on three enzyme pathways, the main one being the conversion of L-tyrosine to L-DOPA via tyrosine hydroxylase and tyrosinase. In addition we are also synthesising dopamine in two different ways using aromatic amino acid decarboxylase, cytochrome P450 and transaminase. Although the primary goal would be to implement the L-DOPA synthesis within patients, we also aim to create a greener, more efficient way of the industrial synthesis of each of the above products using our modified bacteria. (Figure 2) </p>
  
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<img src="https://static.igem.org/mediawiki/2015/3/3c/Menchaster-Graz_PEsa_Cep_Snap_Map.png" alt="pCERI Vector Map" width="541" height="574"><br> <b>Figure 3</b> Simplified map of pCERI Vector.
 
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<p style="text-align:justify">The Graz section are using two quorum sensing based mechanisms for an auto-regulated and time shifted consecutive induction of protein expression, first demonstrated using fluorescent protein synthesis (Figure 3). The fluorescent protein could then be exchanged with genes for the L- DOPA production such that at low cell density levels tyrosine synthesis will be channeled. After a certain biomass is reached actual L-DOPA production will be induced. </p>
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<p style="text-align:justify">Looking to the future this system could be further utilized to activate suicide genes in <i>E.coli </i>to avoid possible overgrowth of the native intestinal flora, which we aim to show proof of concept in both strains common to academic research as well as probiotics, specifically BL21 and Nissle 1917 respectively. Even though we cannot regulate the proliferation of our engineered strain yet, it allows us to provide an outlook of a possible application as a self-regulating drug dispensing system in the GI tract, which may have clinical applications in the future.</p><div id="pictureright"><img src="https://static.igem.org/mediawiki/2015/4/4f/Manchester-Graz_Cell_density.jpg" alt="cell%20density" width="400"><br><b>Fig 3 </b> Fluorescent protein synthesis dependent on different levels of cell density</div>
  
  
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<p style="text-align:justify">Throughout the course of the project we also aim to shape our actions in accordance to the opinions of academics, charities, industry leaders and the public. This includes what implications our project will have for patients both economically and in terms of quality of life and whether the real world implementation of this technology is feasible. We will also compare ethical opinions throughout outreach about our project and synthetic biology in general across the two countries our team spans and assess this in a wider sociological context. We feel as a team that the issues and human practices surrounding our project are just as important as the project itself and as such we endeavour to tackle a wide selection of concerns.</p>
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<div style="background-color:#373737; width: 745px; height:200px; color: white; padding:10px;"><div id="pictureright"><img src="https://static.igem.org/mediawiki/2015/2/23/Manchester-Graz_System_description_website.png" alt="System_description" width="190"></div>
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1) http://www.ipm.iastate.edu/ipm/info/plant-diseases/stewarts-wilt<br>
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2) Shong et al (2013) Engineering the esaR Promoter for Tunable Quorum Sensing- Dependent Gene Expression <br>
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3) Shong et al (2013) Directed Evolution of the Quorum-Sensing Regulator EsaR for Increased Signal Sensitivity <br>
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4) Weingart et al (2005) Direct binding of the quorum sensing regulator CepR of Burkholderia cenocepacia to two target promoters <br>in vitro
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Revision as of 07:43, 31 July 2015

iGEM Manchester Header

iGEM Manchester - Graz Project

Project Outlines

human gut bacteria
Fig 1 Administration of L-DOPA via bacteria in the patient's gut

iGEM Manchester-Graz’s objective as a team is to find a better way to treat and alleviate the symptoms of Parkinson’s disease (PD) through the use of synthetic biology. Degradation of dopaminergic neurons and therefore low levels of dopamine is the main cause of Parkinson’s disease (PD), for which the current treatment involves oral doses of L-DOPA (or levodopa), which unlike dopamine itself is able to cross the blood-brain-barrier. Within the brain L-DOPA is enzymatically converted into dopamine and therefore able to relieve many of the motor symptoms of PD (Figure 1).

Our aim is to take the first steps in the development of a novel technology of drug delivery by developing self-regulating drug-producing bacterial strains that, in the future, could be incorporated into patients’ gut microflora to secrete medicines directly inside the body. To control the bacterial L-DOPA production, we plan to develop a multidimensional cell density dependent auto-regulation system that could also be used to control other multistep enzyme pathways.

Pathway
Fig 2 dopamine and L-DOPA biosynthesis pathways

The Manchester section of the team are working on L-DOPA and dopamine biosynthesis in E. coli BL21 and Nissle 1917 via various enzyme pathways. The focus is on three enzyme pathways, the main one being the conversion of L-tyrosine to L-DOPA via tyrosine hydroxylase and tyrosinase. In addition we are also synthesising dopamine in two different ways using aromatic amino acid decarboxylase, cytochrome P450 and transaminase. Although the primary goal would be to implement the L-DOPA synthesis within patients, we also aim to create a greener, more efficient way of the industrial synthesis of each of the above products using our modified bacteria. (Figure 2)

The Graz section are using two quorum sensing based mechanisms for an auto-regulated and time shifted consecutive induction of protein expression, first demonstrated using fluorescent protein synthesis (Figure 3). The fluorescent protein could then be exchanged with genes for the L- DOPA production such that at low cell density levels tyrosine synthesis will be channeled. After a certain biomass is reached actual L-DOPA production will be induced.

Looking to the future this system could be further utilized to activate suicide genes in E.coli to avoid possible overgrowth of the native intestinal flora, which we aim to show proof of concept in both strains common to academic research as well as probiotics, specifically BL21 and Nissle 1917 respectively. Even though we cannot regulate the proliferation of our engineered strain yet, it allows us to provide an outlook of a possible application as a self-regulating drug dispensing system in the GI tract, which may have clinical applications in the future.

cell%20density
Fig 3 Fluorescent protein synthesis dependent on different levels of cell density

Throughout the course of the project we also aim to shape our actions in accordance to the opinions of academics, charities, industry leaders and the public. This includes what implications our project will have for patients both economically and in terms of quality of life and whether the real world implementation of this technology is feasible. We will also compare ethical opinions throughout outreach about our project and synthetic biology in general across the two countries our team spans and assess this in a wider sociological context. We feel as a team that the issues and human practices surrounding our project are just as important as the project itself and as such we endeavour to tackle a wide selection of concerns.