Team:Grenoble-EMSE-LSU

From 2013.igem.org

(Difference between revisions)
Line 22: Line 22:
<ul class="texte">
<ul class="texte">
<li id="titre">
<li id="titre">
-
                                 <h1 id="talke">TALK'E. Coli</h1>
+
                                 <h1 id="talke">TALK'E. coli</h1>
<h2>through Light Automated Cell Control (Lac²)</h2>
<h2>through Light Automated Cell Control (Lac²)</h2>
-
<p><strong>This year, the Grenoble-EMSE-LSU iGEM team has developed a bioelectronic device enabling the population control of a bacterial culture with light:  Talk’E. Coli.</strong><br><br>
+
<p><strong>This year, the Grenoble-EMSE-LSU iGEM team has developed a bioelectronic device enabling the population control of a bacterial culture with light:  Talk’E. coli.</strong><br><br>
                                 In general, bacteria are among the fastest growing and most widespread organisms on Earth. They can thrive in nearly every environment or ecosystem, and some can even reach a doubling time of only 10min [1]. Even though bacterial growth conforms to quite simple mathematical laws, many parameters of this process are far from being fully understood. Unraveling these genotypic and phenotypic processes represents an important challenge in current public health issues. Conceptually, we have developed a biological system that will enable researchers to <a>monitor and control cellular growth with light</a>. Such an undertaking could be of great interest for improving the understanding of bacterial functions, especially in regards to characterizing cellular populations and the defense mechanisms involved with oxidative stress responses.<br><br>
                                 In general, bacteria are among the fastest growing and most widespread organisms on Earth. They can thrive in nearly every environment or ecosystem, and some can even reach a doubling time of only 10min [1]. Even though bacterial growth conforms to quite simple mathematical laws, many parameters of this process are far from being fully understood. Unraveling these genotypic and phenotypic processes represents an important challenge in current public health issues. Conceptually, we have developed a biological system that will enable researchers to <a>monitor and control cellular growth with light</a>. Such an undertaking could be of great interest for improving the understanding of bacterial functions, especially in regards to characterizing cellular populations and the defense mechanisms involved with oxidative stress responses.<br><br>
                                 Light allows for precise machine-to-cell and cell-to-machine communication in both time and space and was thus elected to <a>interface a biological cell culture to our electronic device</a>.</p>
                                 Light allows for precise machine-to-cell and cell-to-machine communication in both time and space and was thus elected to <a>interface a biological cell culture to our electronic device</a>.</p>
Line 37: Line 37:
                                 [1] L. Elsgaard and D. Prieur, Hydrothermal vents in Lake Tanganyika harbor spore-forming thermophiles with extremely rapid growth, <em>Journal of Great Lakes Research</em>, March 2011.<br>
                                 [1] L. Elsgaard and D. Prieur, Hydrothermal vents in Lake Tanganyika harbor spore-forming thermophiles with extremely rapid growth, <em>Journal of Great Lakes Research</em>, March 2011.<br>
                                 [2] M.E. Bulina et al., A genetically encoded photosensitizer, <em>Nature Biotechnology</em>, January 2006.<br>
                                 [2] M.E. Bulina et al., A genetically encoded photosensitizer, <em>Nature Biotechnology</em>, January 2006.<br>
-
                                 [3] J.J. Tabor et al., Multichromatic Control of Gene Expression in Escherichia coli, <em>Journal of Molecular Biology</em>, 2011.<br>
+
                                 [3] J.J. Tabor et al., Multichromatic Control of Gene Expression in <em>Escherichia coli</em>, <em>Journal of Molecular Biology</em>, 2011.<br>
                                 [4] K.E. McGinness et al., Engineering Controllable Protein Degradation, <em>Molecular Cell</em>, June 2006.
                                 [4] K.E. McGinness et al., Engineering Controllable Protein Degradation, <em>Molecular Cell</em>, June 2006.

Revision as of 08:58, 14 August 2013

Grenoble-EMSE-LSU, iGEM


Grenoble-EMSE-LSU, iGEM

Retrieved from "http://2013.igem.org/Team:Grenoble-EMSE-LSU"