Team:TPHS SanDiego/Project

From 2013hs.igem.org

(Difference between revisions)
Line 43: Line 43:
<div class="col12-2" >
<div class="col12-2" >
<div align="justify">
<div align="justify">
-
<p style="font-family:Georgia;color:black;font-size:16px;">Our project focuses on promoter engineering. Our goal is to characterize a set of promoters (of our design) by moving the repressor and/or activator binding sites with respect to the -10 and -35 regions of the promoter. Ideally, we would like to show that by moving an activator binding site it can become a repressor and that by moving a repressor binding site it may become either irrelevant to transcription rate or even boost it. We also want to see if there is a steep decline in repressor/activator function as the binding site move along the promoter or if it is a gradual/linear change. We believe this project could have application to genetic circuits by allowing a single protein to either activate or repress a promoter depending on where the binding sites are placed on the promoter.</p>
+
<p style="font-family:Georgia;color:black;font-size:16px;">
 +
<h1>Overview</h1>
 +
Our project focuses on promoter engineering. Our goal is to characterize a set of promoters (of our design) by moving the repressor and/or activator binding sites with respect to the -10 and -35 regions of the promoter. Ideally, we would like to show that by moving an activator binding site it can become a repressor and that by moving a repressor binding site it may become either irrelevant to transcription rate or even boost it. We also want to see if there is a steep decline in repressor/activator function as the binding site move along the promoter or if it is a gradual/linear change. We believe this project could have application to genetic circuits by allowing a single protein to either activate or repress a promoter depending on where the binding sites are placed on the promoter.
 +
<h1>XBa1 Insertion</h1>
 +
 
 +
 
 +
 
 +
 
 +
 
 +
</p>
<p>
<p>
Line 50: Line 59:
&nbsp;
&nbsp;
</p>
</p>
-
<center>
 
-
<iframe src="https://docs.google.com/presentation/d/18V3cPgfWJIS7meO2SBBTGxSG1RrKxYvsg_Pxw9hB-2Q/embed?start=false&loop=false&delayms=3000" frameborder="0" width="900" height="500" allowfullscreen="true" mozallowfullscreen="true" webkitallowfullscreen="true"></iframe></center>
 
<div class="row-end" ></div>
<div class="row-end" ></div>

Revision as of 22:02, 21 June 2013

header
Mercury

Overview

Our project focuses on promoter engineering. Our goal is to characterize a set of promoters (of our design) by moving the repressor and/or activator binding sites with respect to the -10 and -35 regions of the promoter. Ideally, we would like to show that by moving an activator binding site it can become a repressor and that by moving a repressor binding site it may become either irrelevant to transcription rate or even boost it. We also want to see if there is a steep decline in repressor/activator function as the binding site move along the promoter or if it is a gradual/linear change. We believe this project could have application to genetic circuits by allowing a single protein to either activate or repress a promoter depending on where the binding sites are placed on the promoter.

XBa1 Insertion

     

Retrieved from "http://2013hs.igem.org/Team:TPHS_SanDiego/Project"