Team:NYU/Project

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!align="center"|[[Team:NYU|Home]]
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!align="center"|[[Team:NYU/Team|Team]]
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!align="center"|[https://igem.org/Team.cgi?year=2010&team_name=NYU Official Team Profile]
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!align="center"|[[Team:NYU/Project|Project]]
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!align="center"|[[Team:NYU/Parts|Parts Submitted to the Registry]]
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!align="center"|[[Team:NYU/Modeling|Modeling]]
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You are provided with this team page template with which to start the iGEM season.  You may choose to personalize it to fit your team but keep the same "look." Or you may choose to take your team wiki to a different level and design your own wiki.  You can find some examples <a href="https://2008.igem.org/Help:Template/Examples">HERE</a>.
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<li><a class="bannertoplinks" href="https://2010.igem.org/Team:NYU/Project">Project</a>
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You <strong>MUST</strong> have a team description page, a project abstract, a complete project description, a lab notebook, and a safety page. PLEASE keep all of your pages within your teams namespace.
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                        <li><a class="bannerlinks" href="https://2010.igem.org/Team:NYU/Experiments">Experiments</a></li>
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                        <li><a class="bannerlinks" href="https://2010.igem.org/Team:NYU/Assembly">Overlap Assembly</a></li>
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                        <li><a class="bannerlinks" href="https://2010.igem.org/Team:NYU/Team">NYU</a></li>
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                        <li><a class="bannerlinks" href="https://2010.igem.org/Team:NYU/CornellMed">Cornell Med</a></li>
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                </ul>  
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                        <li><a class="bannerlinks" href="https://2010.igem.org/Team:NYU/Sponsors">Sponsors</a></li>
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                        <li><a class="bannerlinks" href="http://www.sciencehouse.com">ScienceHouse</a></li>
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                        <li><a class="bannerlinks" href="http://www.nysynbio.org">NY synbio</a></li>
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[[Image:NYU_OverviewSideF_1.png|200px|right]]
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{|align="justify"
 
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|Russ, this should be the part where you talk about how you came up with the project idea.
 
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|[[Image:NYU_logo.png|200px|right|frame]]
 
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|This part should serve as the official abstract describing the project. Unless the two paragraphs in the project details section below is the abstract?
 
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|[[Image:NYU_team.png|right|frame|Your team picture]]
 
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|align="center"|[[Team:NYU | Team Example]]
 
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[[Image:NYU_logo.png|220px|left]]
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Our goal is to use the tools of synthetic biology to make a biological machine capable of antibody discovery. To do this, we have decided to learn from our own immune system by porting its own antibody discovery strategies into an engineered strain of yeast. This yeast will be capable of screening a library of antibodies against a target antigen, recombining the antibody gene ''in vivo'' and then either secreting or surface displaying the resulting antibody protein for a variety of purposes.  Our hope is to demonstrate the feasibility of using the yeast cell not only as a vessel for antibody discovery but as a streamlined processing unit that can discover and also begin production of new antibodies - all in one test tube!
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Our game plan for the international genetically engineered machine competition is to construct a yeast strain capable of independent antibody discovery. Instead of relying on antibody display that require high-throughput fluorescent screening, currently the dominant method for microbial antibody discovery, our strain will be able to select for high antibody binding without outside influence. We will accomplish this by linking the antibody library and antigen with the split ubiquitin system, which will allow the yeast cells to sense the amount of antibody::antigen complexing.
 
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Basically, the single chain variable fragment (scFv) antibody will be fused to the N-terminal domain of ubiquitin (N-ub) and the target antigen will be fused to the C-terminal domain (C-ub). When the antibody and antigen form a complex, the two domains of ubiquitin are brought together and any protein that is fused downstream of C-ub will be cleaved from the rest of the complex by a ubiquitin protease. To use this mechanism to our advantage, we will fuse the Gal4 activator protein downstream of antigen::C-ub complex. So, when the antibody binds the antigen, Gal4p will be released, translocated into the nucleus and will affect transcription of genes that confer greater cell survival in the environment (either amino acid biosynthesis or, for a control, antibiotic resistance).
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Our plan for this year's competition is to construct an easy-to-use yeast strain capable of intracellular antibody discovery. The current dominant mode of microbial antibody discovery requires cellular surface display and high-throughput fluorescent screening.  Instead of using this method, we wanted our cells to be able to sense if the antibody they are translating will bind the target antigen.  
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== The Experiments ==
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[[Image:NYU_bind3.png|180px|left]]
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Using a modified form of the yeast two-hybrid screening system, the yeast cells are able to sense the amount of antibody::antigen interaction inside the cell.  When the antibody binds the target antigen it anchors the VP16 transcriptional activator near our response system. VP16 then increases the level of transcription of a reporter gene. If this gene encodes a nutritional marker, such as Ura3, only cells experiencing antibody:antigen interactions can be selected using selective media. Using this method the original population of our yeast strain will be able to, in essence, screen itself and our resulting yeast population will contain only antibodies that bind our antigen.
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In a research setting, once you have discovered the antibody you wish to use you must then reclone the gene for it into a secretion vector for production of pure antibody protein. This involves taking the plasmid out of the yeast cell, excising the antibody gene, ligating it into the second vector and then transforming it back into a suitable yeast strain.
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[[Image:NYU_Cre.jpg‎|350px|left]]
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To make this process faster and more easily accomplished, we have incorporated a recombination-based architecture into our system that will allow the cells to modify the antibody plasmid ''in vivo''. Using this system transcription of the antibody gene can go straight from screening to protein production in a matter of minutes. This concept has the capability to not only shave weeks off of current antibody discovery protocols, but opens the door to cellular programming for other methods, such as restructuring of antibody genes or performing more complex screenings for different purposes.
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== The Experiments ==
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In the spectrum of molecular biology, iGEM is a very short time frame. Because of this short time frame, our wet lab team having only two members and our extremely limited research budget, we felt that radical simplification of our experiments would allow us to demonstrate the feasibility of our ideas without requiring resources we simply did not have. Because many of the individual aspects that this project has brought together have been investigated with success, we were able to perform some experiments using proxies for the 'real thing'.
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== Results ==
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Please click [https://2010.igem.org/Team:NYU/Experiments Here] to see how we simulated each of the systems.

Latest revision as of 09:29, 27 October 2010



NYU OverviewSideF 1.png


NYU logo.png


Our goal is to use the tools of synthetic biology to make a biological machine capable of antibody discovery. To do this, we have decided to learn from our own immune system by porting its own antibody discovery strategies into an engineered strain of yeast. This yeast will be capable of screening a library of antibodies against a target antigen, recombining the antibody gene in vivo and then either secreting or surface displaying the resulting antibody protein for a variety of purposes. Our hope is to demonstrate the feasibility of using the yeast cell not only as a vessel for antibody discovery but as a streamlined processing unit that can discover and also begin production of new antibodies - all in one test tube!


Project Details

Our plan for this year's competition is to construct an easy-to-use yeast strain capable of intracellular antibody discovery. The current dominant mode of microbial antibody discovery requires cellular surface display and high-throughput fluorescent screening. Instead of using this method, we wanted our cells to be able to sense if the antibody they are translating will bind the target antigen.


NYU bind3.png


Using a modified form of the yeast two-hybrid screening system, the yeast cells are able to sense the amount of antibody::antigen interaction inside the cell. When the antibody binds the target antigen it anchors the VP16 transcriptional activator near our response system. VP16 then increases the level of transcription of a reporter gene. If this gene encodes a nutritional marker, such as Ura3, only cells experiencing antibody:antigen interactions can be selected using selective media. Using this method the original population of our yeast strain will be able to, in essence, screen itself and our resulting yeast population will contain only antibodies that bind our antigen.



In a research setting, once you have discovered the antibody you wish to use you must then reclone the gene for it into a secretion vector for production of pure antibody protein. This involves taking the plasmid out of the yeast cell, excising the antibody gene, ligating it into the second vector and then transforming it back into a suitable yeast strain.


NYU Cre.jpg

To make this process faster and more easily accomplished, we have incorporated a recombination-based architecture into our system that will allow the cells to modify the antibody plasmid in vivo. Using this system transcription of the antibody gene can go straight from screening to protein production in a matter of minutes. This concept has the capability to not only shave weeks off of current antibody discovery protocols, but opens the door to cellular programming for other methods, such as restructuring of antibody genes or performing more complex screenings for different purposes.



The Experiments

In the spectrum of molecular biology, iGEM is a very short time frame. Because of this short time frame, our wet lab team having only two members and our extremely limited research budget, we felt that radical simplification of our experiments would allow us to demonstrate the feasibility of our ideas without requiring resources we simply did not have. Because many of the individual aspects that this project has brought together have been investigated with success, we were able to perform some experiments using proxies for the 'real thing'.

Please click Here to see how we simulated each of the systems.