Team:Tufts/Project

From 2014.igem.org

(Difference between revisions)
 
(26 intermediate revisions not shown)
Line 9: Line 9:
<td style="border:2px solid black;" colspan="3" align="center" height="150px"bgColor=#0099FF>
<td style="border:2px solid black;" colspan="3" align="center" height="150px"bgColor=#0099FF>
<h1 style="color:white">Tufts iGEM 2014</h1>
<h1 style="color:white">Tufts iGEM 2014</h1>
-
<p style="color:#E7E7E7"> <a href="https://2014.igem.org/wiki/index.php?title=Team:Tufts/Project&action=edit"style="color:#FFFFFF"> Click here  to edit this page!</a> </p>
 
</td>
</td>
</tr>
</tr>
Line 21: Line 20:
<tr heigth="15px"></tr>
<tr heigth="15px"></tr>
<tr heigth="75px">  
<tr heigth="75px">  
-
 
<td style="border:2px solid #0099FF;" align="center" height ="45px" bgColor=black>   
<td style="border:2px solid #0099FF;" align="center" height ="45px" bgColor=black>   
Line 30: Line 28:
<td style="border:2px solid #0099FF;" align="center"  height ="45px"  bgColor=black>  
<td style="border:2px solid #0099FF;" align="center"  height ="45px"  bgColor=black>  
-
<a href="https://igem.org/Team.cgi?year=2014&team_name=Tufts"style="color:#0099FF"> Official Team Profile </a></td>
+
<a href="https://igem.org/Team.cgi?year=2014&team_name=Tufts"style="color:#0099FF"target="_blank"> Official Team Profile </a></td>
<td style="border:2px solid #0099FF" align="center"  height ="45px" bgColor=black>   
<td style="border:2px solid #0099FF" align="center"  height ="45px" bgColor=black>   
Line 57: Line 55:
<!--end navigation menu -->
<!--end navigation menu -->
</tr>
</tr>
-
 
</tr>
</tr>
-
 
</td>
</td>
-
 
<tr> <td colspan="3"  height="15px"> </td></tr>
<tr> <td colspan="3"  height="15px"> </td></tr>
<tr><td bgColor="#e7e7e7" colspan="3" height="1px"> </tr>
<tr><td bgColor="#e7e7e7" colspan="3" height="1px"> </tr>
Line 67: Line 62:
<tr><td width="100%">
<tr><td width="100%">
-
<p> <h3>Ribosponge Project Description:</h3> <br>
+
<a href = "https://2014.igem.org/Team:Tufts/Project#backgrounds"><h5>Jump to Backgrounds</h5></a>
 +
<a href = "https://2014.igem.org/Team:Tufts/Project#methods"><h5>Jump to Methods</h5></a>
 +
<h2> Summaries </h2>
 +
<tr> <td width="100%">
 +
<h3>Robust biofilm formation using a cyclic-di-GMP aptamer and investigating ethics and applications of engineered bactiophage</h3>
 +
A long, noncoding massively expressed regulatory RNA (merRNA) discovered in Bdellovibrio
 +
bacteriovorus is present in high levels during its dormant phase. The merRNA is believed to sequester
 +
cyclic-di-GMP, much like a sponge. Since cyclic-di-GMP is a second messenger for various cellular
 +
functions, including motility and biofilm formation, the Tufts iGEM team introduced this merRNA
 +
sequence into E. coli. Constitutive expression of this merRNA transcript was shown to increase biofilm
 +
formation. This property can be useful in microbe-based approaches to environmental remediation.
 +
Earlier designs for phage delivery of the merRNA to disrupt biofilms inspired an investigation into the
 +
policy surrounding engineered bacteriophage. Tufts iGEM will be convening a panel of experts from
 +
various disciplines to put forth recommendations for the responsible use of phage in therapeutic and
 +
industrial applications. A proposal will be drafted for a silk bandage containing a phage cocktail which
 +
can prevent and treat infection by antibiotic-resistant bacteria.
 +
</td></tr>
 +
 +
<tr><td>
 +
<p> <h3>Ribosponge Project Description:</h3>
We have devised a method to introduce a DNA sequence which encodes an RNA aptamer (i.e. - an  
We have devised a method to introduce a DNA sequence which encodes an RNA aptamer (i.e. - an  
-
 
oligonucleotide sequence which binds to a specific molecule) into a non-pathogenic E. coli strain. We  
oligonucleotide sequence which binds to a specific molecule) into a non-pathogenic E. coli strain. We  
-
 
have dubbed this RNA aptamer a “ribosponge” due to its unique mode of action. The ribosponge binds  
have dubbed this RNA aptamer a “ribosponge” due to its unique mode of action. The ribosponge binds  
-
 
cyclic di-GMP, a secondary intracellular messenger which signals bacteria to enter a persistent or biofilm  
cyclic di-GMP, a secondary intracellular messenger which signals bacteria to enter a persistent or biofilm  
-
 
state. The signal is universal among many species such as E. coli, P. aeruginosa, and M. tuberculosis.  
state. The signal is universal among many species such as E. coli, P. aeruginosa, and M. tuberculosis.  
-
 
Blocking the signal of c-di-GMP by binding it with an aptamer could prevent the persistent state in these  
Blocking the signal of c-di-GMP by binding it with an aptamer could prevent the persistent state in these  
-
 
and other pathogens. In order to ferry the sequence encoding the aptamer from our non-pathogenic E.  
and other pathogens. In order to ferry the sequence encoding the aptamer from our non-pathogenic E.  
-
 
coli into other bacteria of the same species, we plan on using an M13 phage which does not kill the  
coli into other bacteria of the same species, we plan on using an M13 phage which does not kill the  
-
 
bacteria.
bacteria.
-
 
The project has also inspired our collaboration with the Rathneau Institute and SYNENERGENE as we  
The project has also inspired our collaboration with the Rathneau Institute and SYNENERGENE as we  
-
 
look at the feasability of developing ribosponge into a product, and examine the regulatory, legal, and  
look at the feasability of developing ribosponge into a product, and examine the regulatory, legal, and  
-
 
ethical challenges of packing it into a bacteriophage.</p>
ethical challenges of packing it into a bacteriophage.</p>
</td> </tr>
</td> </tr>
-
<br>
 
-
<tr> <td width="100%">
 
-
<h3>Synthetic Antibody Proposal</h3> <br>
 
 +
<!--<tr> <td width="100%">
 +
<h3>Synthetic Antibody Proposal</h3>
Monoclonal antibodies are proteins produced by the immune system to selectively bind  
Monoclonal antibodies are proteins produced by the immune system to selectively bind  
-
 
foreign molecules and induce immune response. Given  
foreign molecules and induce immune response. Given  
-
 
their high affinity and specificity of binding to their target  
their high affinity and specificity of binding to their target  
-
 
molecules, monoclonal antibodies are applied clinically  
molecules, monoclonal antibodies are applied clinically  
-
 
and in research to create detection assays, therapeutics, and  
and in research to create detection assays, therapeutics, and  
-
 
diagnostics. However, their production requires harming animals, and it  
diagnostics. However, their production requires harming animals, and it  
-
 
is costly, time consuming, and for certain molecules  
is costly, time consuming, and for certain molecules  
-
 
impossible.  
impossible.  
The goal of our research is to create an alternative detection molecule, a synthetic  
The goal of our research is to create an alternative detection molecule, a synthetic  
-
 
antibody, which can be produced more quickly, at a lower cost, using much simpler and more  
antibody, which can be produced more quickly, at a lower cost, using much simpler and more  
-
 
accessible methods. The product of our research will be a template plasmid, a synthetic DNA  
accessible methods. The product of our research will be a template plasmid, a synthetic DNA  
-
 
molecule that will cause bacteria to express our synthetic antibodies. The template plasmid will  
molecule that will cause bacteria to express our synthetic antibodies. The template plasmid will  
-
 
allow researchers to “plug-and-play” different detection regions onto the constant region of an  
allow researchers to “plug-and-play” different detection regions onto the constant region of an  
-
 
antibody. We will also validate this approach by demonstrating the efficacy of our synthetic  
antibody. We will also validate this approach by demonstrating the efficacy of our synthetic  
-
 
antibodies in a proof-of-concept experiment, in which our synthetic antibody will be used to  
antibodies in a proof-of-concept experiment, in which our synthetic antibody will be used to  
-
 
detect proteins on the surface of a cell.  
detect proteins on the surface of a cell.  
 +
The creation of synthetic antibodies in bacteria will allow researchers to circumvent the
 +
expensive, time consuming, and arduous process of monoclonal antibody production. The highly
 +
modular “plug-and-play” aspect of our template plasmid will make this tool simple to use and highly versatile, while the use of the constant
 +
region of a monoclonal antibody as the detection method will make this technology particularly powerful, as there already exists a large amount of chemistry, and protocols associated with different uses of the conserved domain. Thus, synthetic antibodies will provide yet another versatile tool for creating detection assays, diagnostics, and potentially even therapeutics for diseases such as cancers and autoimmune diseases.
-
The creation of synthetic antibodies in
+
</td></tr>
-
bacteria will allow researchers to circumvent the
+
<br><br>
 +
-->
-
expensive, time consuming, and arduous process
+
<tr> <td>
 +
<a name="backgrounds"> <h2> Backgrounds </h2> </a>
-
of monoclonal antibody production. The highly
 
-
 
-
modular “plug-and-play” aspect of our template
 
-
 
-
plasmid will make this tool simple to use and highly versatile, while the use of the constant
 
-
 
-
region of a monoclonal antibody as the detection method will make this technology particularly
 
-
 
-
powerful, as there already exists a large amount of chemistry, and protocols associated with different uses of the conserved domain. Thus, synthetic antibodies will provide yet another versatile tool for creating detection assays, diagnostics, and potentially even therapeutics for diseases such as cancers and autoimmune diseases.
 
 +
</td> </tr>
 +
<tr><td>
 +
<a name="methods"><h2>Methods</h2></a>
 +
<!--<a href = "https://static.igem.org/mediawiki/2014/2/24/LabNotebookAntibodyiGEM2014.pdf"> Antibody Lab Notebook </a> <br>-->
 +
<a href="https://static.igem.org/mediawiki/2014/a/a1/LabNotebookSpongeiGEM2014.pdf" target="_blank"> Sponge Lab Notebook </a>
</td></tr>
</td></tr>
-
<br><br>
 
<!--Project content  -->
<!--Project content  -->

Latest revision as of 01:27, 30 September 2014

Tufts iGEM 2014

Home Team Official Team Profile Project Parts Modeling Notebook Safety Attributions
Jump to Backgrounds
Jump to Methods

Summaries

Robust biofilm formation using a cyclic-di-GMP aptamer and investigating ethics and applications of engineered bactiophage

A long, noncoding massively expressed regulatory RNA (merRNA) discovered in Bdellovibrio bacteriovorus is present in high levels during its dormant phase. The merRNA is believed to sequester cyclic-di-GMP, much like a sponge. Since cyclic-di-GMP is a second messenger for various cellular functions, including motility and biofilm formation, the Tufts iGEM team introduced this merRNA sequence into E. coli. Constitutive expression of this merRNA transcript was shown to increase biofilm formation. This property can be useful in microbe-based approaches to environmental remediation. Earlier designs for phage delivery of the merRNA to disrupt biofilms inspired an investigation into the policy surrounding engineered bacteriophage. Tufts iGEM will be convening a panel of experts from various disciplines to put forth recommendations for the responsible use of phage in therapeutic and industrial applications. A proposal will be drafted for a silk bandage containing a phage cocktail which can prevent and treat infection by antibiotic-resistant bacteria.

Ribosponge Project Description:

We have devised a method to introduce a DNA sequence which encodes an RNA aptamer (i.e. - an oligonucleotide sequence which binds to a specific molecule) into a non-pathogenic E. coli strain. We have dubbed this RNA aptamer a “ribosponge” due to its unique mode of action. The ribosponge binds cyclic di-GMP, a secondary intracellular messenger which signals bacteria to enter a persistent or biofilm state. The signal is universal among many species such as E. coli, P. aeruginosa, and M. tuberculosis. Blocking the signal of c-di-GMP by binding it with an aptamer could prevent the persistent state in these and other pathogens. In order to ferry the sequence encoding the aptamer from our non-pathogenic E. coli into other bacteria of the same species, we plan on using an M13 phage which does not kill the bacteria. The project has also inspired our collaboration with the Rathneau Institute and SYNENERGENE as we look at the feasability of developing ribosponge into a product, and examine the regulatory, legal, and ethical challenges of packing it into a bacteriophage.

Backgrounds

Methods

Sponge Lab Notebook