Difference between revisions of "Team:UAlberta/Description"

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          <h1><strong>Project Description</strong></h1>
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<p style="text-align:center;"><img src="https://static.igem.org/mediawiki/2017/5/54/T--UAlberta--Overview.png" width="70%"></p>
            <h1>Description</h1>
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          <h2>What is RISE?</h2>
            <div class="col-lg-4" style="border: 2px solid #222222;">
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          <p>The Recombinant Protein Interaction Screening and Enrichment (RISE) system is a tool designed to provide an easily measurable and quantifiable protein screening process. Based upon a modified BACTH system and directed evolution, the RISE system utilizes buoyancy as a readily observable readout of the relative strength of protein-protein interactions that also facilitates separation of desirable variants from undesirable ones.</p>
              <img width="200px" height="200px">
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          <h3>Why did we develop RISE?</h3>
            </div>
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          <p>Existing screening methods, such as phage display and the yeast 2-hybrid system, have several drawbacks. They can be costly both in terms of time and money, and don’t have readily observable read outs. We wanted to improve on these techniques to provide a screening method that is easily observable and efficient. An added advantage of the RISE system is that it can be easily automated so that a machine would select for the most buoyant bacteria from the top of each culture and perform the enrichment process independently.</p>
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          <h3>How does it work? </h3>
            <p>Lorem ipsum dolor sit amet, consectetur adipiscing elit. Fusce fringilla velit ac lorem ultricies faucibus. Fusce placerat nulla tortor, eget gravida risus sagittis sit amet. Curabitur et auctor eros. Donec rutrum lobortis arcu id volutpat. Suspendisse rhoncus neque nec accumsan mattis. Sed suscipit iaculis molestie. Ut ut maximus turpis. Nunc finibus erat quis sem venenatis, nec interdum leo fermentum. Nulla et consectetur enim. Nam pulvinar dapibus luctus. Donec non metus vel elit aliquet euismod.</p> </div>
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          <p>The RISE system uses buoyancy as an indicator of protein-protein interaction strength. This buoyancy phenotype allows for a simple enrichment system, where the most buoyant bacteria, that is those expressing the strongest protein-protein interactions, can be easily selected at each round of enrichment since they will be at the uppermost part of the culture. The enrichment process – that is, the repeated re-culturing of the top layer of the culture – is meant to weed out false positives. This process ultimately results in selection for the strongest interactions over multiple generations of cell culture growth</p>
 
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          <h3>Protein interactions → buoyancy?</h3>
      <p>Nulla quis congue risus. Aenean eu orci sit amet leo eleifend pulvinar a eu purus. Ut non diam nulla. Ut imperdiet urna ac lectus ullamcorper scelerisque. Mauris hendrerit elementum sem vel placerat. Suspendisse imperdiet erat orci, iaculis aliquet libero ornare quis. Sed orci nisi, egestas a ornare nec, imperdiet sed dui. Donec tempus, sem eget luctus aliquam, purus risus porta metus, tincidunt consectetur elit justo eget odio. Nulla non mauris posuere, fringilla eros in, iaculis risus. Curabitur molestie malesuada accumsan. Sed non malesuada diam. Maecenas et blandit erat.</p>
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          <p>To provide a reliable read out of protein-protein interaction strength, we have employed the use of a modified BACTH system. In the BACTH system the two subunits of adenylate cyclase, T25 and T18, are fused to two proteins of interest. When the proteins interact, T18 and T25 are brought together, re-establishing adenylate cyclase activity and therefore resuming cAMP production. The newly synthesized cAMP will then bind to the catabolite activator protein (CAP), which in turn upregulates the transcription of downstream genes.</p>
 
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          <h3>Engineering BACTH</h3>
      <p>Sed ornare nunc vel erat ultricies pretium. Curabitur fermentum est ac blandit bibendum. Sed tristique tellus vitae cursus dignissim. Maecenas venenatis et est et dictum. Mauris ultrices odio massa, nec euismod mauris efficitur at. Vestibulum at magna feugiat, rutrum est quis, volutpat nulla. Mauris est massa, vestibulum aliquet odio sed, posuere lobortis mauris. Nullam ante neque, aliquam vel velit nec, congue porttitor sem. Proin id tincidunt eros, quis tempus enim. Nam vitae nisi mauris. Proin vel dui nec enim aliquet dignissim ac nec dui. Duis ac neque sit amet eros sollicitudin molestie. Vivamus eleifend, erat vitae accumsan aliquet, ipsum libero suscipit ipsum, quis auctor elit purus a nisi.</p>
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          <p>The commercially available BACTH kit consists of the T25 and T18 subunits on two separate plasmids. This posed an issue for our project, as increased plasmid number has an inverse relationship with transformation efficiency. In order to increase our cloning success, we have engineered a simplified BACTH system in which both subunits are contained in a single plasmid.</p>
      <h1>Section</h1>
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          <h3>Gvp 3.0</h3>
      <p>Nam non augue ante. Sed id aliquam augue. Morbi malesuada orci sit amet porta sagittis. Nullam et mattis ipsum. Mauris neque lorem, finibus ut mauris ut, condimentum condimentum elit. Donec ligula erat, commodo vitae lorem eget, gravida mattis mi. Duis tempor lacus non leo euismod cursus. Pellentesque rhoncus enim sit amet justo tempor, id dictum libero viverra. Proin aliquet magna vitae facilisis maximus. Etiam ex mi, laoreet et consequat eu, elementum at tellus. Duis maximus ipsum vel molestie porta. Pellentesque fringilla urna tellus, at hendrerit nunc tempus in. Interdum et malesuada fames ac ante ipsum primis in faucibus. Etiam pellentesque leo sapien, in porta velit cursus vel. Duis justo eros, tristique nec dignissim at, suscipit id lorem. Vestibulum eu lectus ut velit vestibulum molestie.</p>
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          <p>Gvp 3.0 is a gene cluster encoding repeats of gas vesicle proteins gvp A and gvp C. When transcribed, gvp A and gvp C combineto form gas vesicles, conferring buoyancy to the bacterial cell.</p>
 
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          <h3>How can RISE be used?</h3>
      <p>Sed non tellus dui. Etiam rutrum condimentum libero sit amet mattis. Sed porta, est nec scelerisque imperdiet, justo neque laoreet leo, sit amet ornare sem dolor auctor tortor. Aenean eu libero odio. Maecenas felis mi, tristique id tincidunt non, vulputate at nisl. Donec vel diam ac tortor commodo molestie. Morbi sit amet neque nisi. Interdum et malesuada fames ac ante ipsum primis in faucibus. Quisque finibus vehicula erat, in posuere nulla ornare eu. Aliquam commodo, erat non laoreet commodo, velit massa consequat ligula, sed elementum ex lectus a dui. Orci varius natoque penatibus et magnis dis parturient montes, nascetur ridiculus mus. Nullam semper, enim id pulvinar feugiat, ante urna convallis augue, eget mattis mauris ligula vel libero. Praesent at lorem a mi fermentum blandit.</p>
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          <p>The RISE system has a diverse range of applications:</p>
 
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          <ul>
      <p>Nunc lobortis lobortis nulla, eget iaculis orci dignissim eu. Phasellus malesuada sit amet enim sed sodales. Donec convallis mauris vel suscipit elementum. Proin suscipit ac lorem non porta. Nulla facilisi. Curabitur a nisl ac lorem luctus commodo. Quisque eget interdum elit, vel volutpat velit. Orci varius natoque penatibus et magnis dis parturient montes, nascetur ridiculus mus. Class aptent taciti sociosqu ad litora torquent per conubia nostra, per inceptos himenaeos. Suspendisse vitae suscipit ante. Aliquam ac ex porttitor, consectetur augue ac, placerat augue. Phasellus suscipit purus sed lacinia ultricies. Suspendisse consectetur laoreet sem at ullamcorper.</p>
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            <li>Protein-based drug development</li>
      <h1>Section</h1>
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            <li>Imaging (developing peptides that bind to proteins in body- attach radioisotope domain as marker)</li>
      <p>Curabitur viverra diam vitae metus fringilla volutpat eget in sapien. Vestibulum non erat eget neque pulvinar suscipit. Suspendisse condimentum neque at porta aliquet. Donec egestas vel lorem eget volutpat. Ut arcu libero, viverra nec vehicula eu, porta ac metus. Aliquam pulvinar tempus enim quis gravida. Mauris id sem erat. Donec iaculis euismod pellentesque.</p>
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            <li>Foundational research</li>
 
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           </ul>
      <p>Pellentesque euismod condimentum risus at venenatis. Mauris tincidunt imperdiet mi, vel convallis enim convallis et. Proin pellentesque, neque id egestas gravida, libero mi condimentum enim, varius hendrerit turpis velit eget ex. Maecenas tristique consequat semper. Pellentesque sem tellus, sollicitudin et sem a, aliquam ultrices nibh. Etiam elit nibh, placerat et accumsan nec, ullamcorper ac leo. Duis mollis ipsum sed luctus laoreet. Mauris pharetra, dolor id tristique rhoncus, ligula ligula efficitur leo, at iaculis ligula nisi non sem. Nam luctus, leo ac dignissim aliquam, lorem neque bibendum nulla, ut dapibus dolor diam ut ante. Proin nunc risus, consectetur eget efficitur vitae, vestibulum et libero. Phasellus malesuada feugiat tellus, nec condimentum velit lobortis a. Nulla eget eleifend quam. Proin accumsan molestie quam, eget lobortis orci suscipit a. Phasellus sit amet feugiat arcu, quis iaculis est. Donec in ligula eu sem porta malesuada. Ut arcu lorem, suscipit nec elementum id, elementum sed leo.</p>
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<p>Vivamus eu semper nibh, id iaculis ante. Proin lobortis efficitur lorem, a vulputate odio congue quis. Nullam consequat, elit in euismod tempor, sem tellus rhoncus justo, in malesuada diam mauris a massa. Praesent mattis aliquet nibh sed posuere. Donec varius condimentum felis nec egestas. Praesent aliquam mattis rutrum. In euismod vulputate mauris. Phasellus tempus turpis sem. Fusce eu tellus non magna laoreet feugiat. Cras dictum in ipsum a mattis. Vivamus rutrum ligula eu fringilla viverra. Interdum et malesuada fames ac ante ipsum primis in faucibus. Morbi pellentesque sodales urna vel tincidunt. Aenean efficitur quam vitae pretium mattis. Class aptent taciti sociosqu ad litora torquent per conubia nostra, per inceptos himenaeos. Donec id justo convallis, euismod nunc a, fermentum neque.</p>
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Latest revision as of 03:57, 2 November 2017

What is RISE?

The Recombinant Protein Interaction Screening and Enrichment (RISE) system is a tool designed to provide an easily measurable and quantifiable protein screening process. Based upon a modified BACTH system and directed evolution, the RISE system utilizes buoyancy as a readily observable readout of the relative strength of protein-protein interactions that also facilitates separation of desirable variants from undesirable ones.

Why did we develop RISE?

Existing screening methods, such as phage display and the yeast 2-hybrid system, have several drawbacks. They can be costly both in terms of time and money, and don’t have readily observable read outs. We wanted to improve on these techniques to provide a screening method that is easily observable and efficient. An added advantage of the RISE system is that it can be easily automated so that a machine would select for the most buoyant bacteria from the top of each culture and perform the enrichment process independently.

How does it work?

The RISE system uses buoyancy as an indicator of protein-protein interaction strength. This buoyancy phenotype allows for a simple enrichment system, where the most buoyant bacteria, that is those expressing the strongest protein-protein interactions, can be easily selected at each round of enrichment since they will be at the uppermost part of the culture. The enrichment process – that is, the repeated re-culturing of the top layer of the culture – is meant to weed out false positives. This process ultimately results in selection for the strongest interactions over multiple generations of cell culture growth

Protein interactions → buoyancy?

To provide a reliable read out of protein-protein interaction strength, we have employed the use of a modified BACTH system. In the BACTH system the two subunits of adenylate cyclase, T25 and T18, are fused to two proteins of interest. When the proteins interact, T18 and T25 are brought together, re-establishing adenylate cyclase activity and therefore resuming cAMP production. The newly synthesized cAMP will then bind to the catabolite activator protein (CAP), which in turn upregulates the transcription of downstream genes.

Engineering BACTH

The commercially available BACTH kit consists of the T25 and T18 subunits on two separate plasmids. This posed an issue for our project, as increased plasmid number has an inverse relationship with transformation efficiency. In order to increase our cloning success, we have engineered a simplified BACTH system in which both subunits are contained in a single plasmid.

Gvp 3.0

Gvp 3.0 is a gene cluster encoding repeats of gas vesicle proteins gvp A and gvp C. When transcribed, gvp A and gvp C combineto form gas vesicles, conferring buoyancy to the bacterial cell.

How can RISE be used?

The RISE system has a diverse range of applications:

  • Protein-based drug development
  • Imaging (developing peptides that bind to proteins in body- attach radioisotope domain as marker)
  • Foundational research

Special thanks to all our sponsors!

Social Media

igem.ualberta@gmail.com