Team:Calgary/Project/Collaboration

From 2013.igem.org

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<h1>Collaboration</h1>
<h1>Collaboration</h1>
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<p>The <a href="https://2013.igem.org/Team:Paris_Bettencourt"><span class="Yellow"><b>Paris Bettencourt</b></a>-<a href="https://2013.igem.org/Team:Calgary"><span class="Yellow"><b>Calgary</b></span></a> iGEM collaboration started last June when a few members from each team met at the <a href="http://sb6.biobricks.org/">SB6.0 synbio conference</span></a> in London. After a few beers and lab stories, we learned that despite coming from the opposite sides of the globe, we were using synthetic biology to build biosensors to sense DNA. While our systems were targeted solve different problems, we were struck by a number of commonalities between these projects. Please see the Figure 1 for a breakdown of these differences.</p>
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<p>The <a href="https://2013.igem.org/Team:Paris_Bettencourt"><span class="Yellow"><b>Paris Bettencourt</b></a>-<a href="https://2013.igem.org/Team:Calgary"><span class="Yellow"><b>Calgary</b></span></a> iGEM collaboration started last June when a few members from each team met at the <a href="http://sb6.biobricks.org/"><span class="Yellow"><b>SB6.0 synbio conference</b></span></a> in London. After a few beers and lab stories, we learned that despite coming from the opposite sides of the globe, we were using synthetic biology to build biosensors to sense DNA. While our systems were targeted solve different problems, we were struck by a number of commonalities between these projects. Please see the Figure 1 for a breakdown of these differences.</p>
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<p>As we shared our projects, we recalled how there was a lack of DNA biosensor parts in the Parts Registry. Moreover, we complained about the lack of organization of biosensors in the registry. The veteran iGEMers on each team mentioned that biosensors had consistently finished as grand prize winners in previous years of iGEM. We were curious how biosensors have evolved since the beginning of iGEM and how our projects fit into the context of the iGEM Parts Registry.</p>
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<p>As we shared our projects, we recalled how there was a <span class="Yellow"><b>lack of DNA biosensor parts</b></span> in the Parts Registry. Moreover, we complained about the lack of organization of biosensors in the registry. The veteran iGEMers on each team mentioned that biosensors had consistently finished as grand prize winners in previous years of iGEM. We were curious how biosensors have evolved since the beginning of iGEM and how our projects fit into the context of the iGEM Parts Registry.</p>
<h2>SensiGEM - A biosensor database</h2>
<h2>SensiGEM - A biosensor database</h2>

Revision as of 22:38, 27 September 2013

Collaboration

The Paris Bettencourt-Calgary iGEM collaboration started last June when a few members from each team met at the SB6.0 synbio conference in London. After a few beers and lab stories, we learned that despite coming from the opposite sides of the globe, we were using synthetic biology to build biosensors to sense DNA. While our systems were targeted solve different problems, we were struck by a number of commonalities between these projects. Please see the Figure 1 for a breakdown of these differences.

Figure 1. The Calgary and Paris Bettencourt biosensors both sense DNA, albeit with some differences in how they function mechanistically.

As we shared our projects, we recalled how there was a lack of DNA biosensor parts in the Parts Registry. Moreover, we complained about the lack of organization of biosensors in the registry. The veteran iGEMers on each team mentioned that biosensors had consistently finished as grand prize winners in previous years of iGEM. We were curious how biosensors have evolved since the beginning of iGEM and how our projects fit into the context of the iGEM Parts Registry.

SensiGEM - A biosensor database

We decided to collaborate to answer these questions. Since our initial meeting in London, members of each team have conferenced weekly on Skype. After accustoming ourselves to the eight hour time difference, we developed SensiGEM, a collaborative database in which we catalogued all the biosensors in the history of iGEM.

Before sinking our teeth into past Wikis, we realized that we had different definitions of biosensors. We asked each other a fundamental question: What is a biosensor? We developed the following definition:

A biosensor is an engineered system that relies on biological systems or components to detect and report a condition. The condition(s) detected and reported could encompass an environmental, biological, chemical or synthetic aspect or compound in the sensor’s environment or surroundings.

Once agreeing on the nature of biosensors, we split up the Wikis from 2007 onward between Calgary and Paris Bettencourt. We analyzed 936 project Wikis from 2007 to 2013 by hand, incorporating the projects which matched our biosensor definition into the collaborative SensiGEM database. We included 229 projects on the database, some of which were biosensors as per the definition, as well as other projects containing biosensor elements that aligned with our definition.

We designed this database with future iGEM teams in mind, with tools for efficient navigation biosensors according to inputs, outputs, and their intended application. We made both SensiGEM's source code and underlying data available under the permissive MIT license. This means that other teams can either collaborate with us on our version of the database or host their own independent copies. We foresee SensiGEM as a resource where future iGEM teams can showcase their biosensors.

Lessons from SensiGEM

We conducted some preliminary analysis of the database in SensiGEM to see how our projects stand in the current iGEM biosensor landscape. Please see Figures 2 and 3 below.

Figure 2. The approach Calgary has taken using an in vitro sensor comprised of isolated, non-living protein components is rare within iGEM. There was an all time high of 12 of these projects in 2010.

Figure 3. Since 2007, fewer than 10 iGEM biosensors involve inputs of nucleic acids. Henceforth, Paris Bettencourt and Calgary are significantly expanding the variety of nucleic acid biosensors in the iGEM registry.

In Figure 2, we can see that Calgary's approach of using non-living, in vitro protein components is not typical of biosensors in iGEM. We advocate this approach for two reasons. Firstly, we envision components such as our robust ferritin reporter as being more field stable compared to systems in living cells. Secondly, our system overcomes potential concerns of deploying synthetic bacteria in the broader environment since there are no living components in our sensor.

From Figure 3, we have can see that 5 DNA biosensors were added to the iGEM Parts Registry since 2007. This means that about one half a percent of projects since 2007 were DNA biosensors! Since Paris Bettencourt and Calgary are launching two novel DNA sensing components, we are significantly expanding the variety of DNA biosensor tools in iGEM. Moreover, each of our respective systems are modular and can be modified to sense most any DNA segment of interest, which means that other teams could use apply these components to a variety of applications.

Looking toward finals

Given the similarities between each of our systems in overall function, we have begun development of BioBricks to apply each system to the other team's problem. By testing each system on a different problem, we intend to show how each system can be deployed as a modular, platform technology.