Team:UNIST Korea/project/abstract

From 2011.igem.org

(Difference between revisions)

Revision as of 05:22, 4 October 2011

Team

Project

Experiment

CHOp-Coli-LATE

Recently, microbe-driven fermentation products are gaining increased importance.

However, release of these microbes to the open environment would pose increasing threat to the society due to the possibility of changes expected in the indigenous microbial population and horizontal gene transfer.

Hence, we have engineered a synthetic self-killing system for the famous industrial workhorse, Escherichia coli.

High temperature (37⁰C), native quorum sensing molecule (AI-2) and the darkness present in the fermentor will keep the self-killing system turned off.

Environmental signals such as low temperature (25 ⁰C), foreign quorum sensing molecules and light encountered by the E. coli outside of the fermentor would trigger the self-killing device.

Unlike other lysis device, we have introduced a novel self-killing device that chops up the DNA.

Thus, this system would not only favor cell death but also ensure that all the genetic materials are destroyed and guarantee that there would be no horizontal gene transfer

Retrieved from "http://2011.igem.org/Team:UNIST_Korea/project/abstract"

@@ Line 179: / Line 179: @@
 <img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/>
-Recently, microbe-driven fermentation products are gaining increased importance. However, release of these microbes to the open environment would pose increasing threat to the society due to the possibility of changes expected in the indigenous microbial population and <b>horizontal gene transfer</b>. Hence, we have engineered a synthetic self-killing system for the famous industrial workhorse, <i>Escherichia coli</i>. High temperature (37⁰C), native quorum sensing molecule (AI-2) and the darkness present in the fermentor will keep the self-killing system turned off. Environmental signals such as low temperature (25 ⁰C), foreign quorum sensing molecules and light encountered by the <i>E. coli</i> outside of the fermentor would trigger the self-killing device. Unlike other lysis device, we have introduced a novel self-killing device that chops up the DNA. Thus, this system would not only favor cell death but also ensure that all the genetic materials are destroyed and guarantee that there would be no horizontal gene transfer
+Recently, microbe-driven fermentation products are gaining increased importance. <br/><br/>
+<img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/>
+ However, release of these microbes to the open environment would pose increasing threat to the society due to the possibility of changes expected in the indigenous microbial population and <b>horizontal gene transfer</b>.<br/><br/>
+<img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/> Hence, we have engineered a synthetic self-killing system for the famous industrial workhorse, <i>Escherichia coli</i>. <br/><br/>
+<img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/>High temperature (37⁰C), native quorum sensing molecule (AI-2) and the darkness present in the fermentor will keep the self-killing system turned off.<br/><br/>
+<img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/> Environmental signals such as low temperature (25 ⁰C), foreign quorum sensing molecules and light encountered by the <i>E. coli</i> outside of the fermentor would trigger the self-killing device. <br/><br/>
+<img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/>Unlike other lysis device, we have introduced a novel self-killing device that chops up the DNA. <br/><br/>
+<img src="http://lornapblog.files.wordpress.com/2011/05/big-tick.jpg" width="32" height="32"/>Thus, this system would not only favor cell death but also ensure that all the genetic materials are destroyed and guarantee that there would be no horizontal gene transfer