Team:INSA-Lyon/Parts

From 2014.igem.org

(Difference between revisions)

Latest revision as of 17:07, 17 October 2014

Curly'on - IGEM 2014 INSA-LYON

PARTS

5 biobricks have been constructed, thre for Nickel chelation, two for promoter characterization.

Biobricks for nickel chelation

The principal of the construction is shown in the figure below.

On a pSB1C3 backbone, two essential part have been assembled: a promoter and a reporter coding for CsgA.The promoter in this case is always the same: P70.However, the reporter is different for each construction.
The first CsgA is called CsgA WT, the sequence is exactly the same as we found in a wild type CsgA protein except one mutation in order to eliminate one restriction site. The construction is also called CsgA-WT.
The second CsgA is based on the same sequence but with a short sequence coding for a his tag(a peptide chain coding six histidines). This construction is called CsgA-His1.
The last CsgA is almost the same but with 2 his tag. This construction is called CsgA-His2.

@@ Line 12: / Line 12: @@
 			<div id="icones">
 				<ul>
-		<a href="https://2014.igem.org/Team:INSA-Lyon/Biology" class="hu-icon"><li class="iconmulti"  style="line-height:20px;  ">WETLAB SUMMARY</li></a>
+		<a href="https://2014.igem.org/Team:INSA-Lyon/Biology" class="hu-icon"><li class="iconmulti">WETLAB SUMMARY</li></a>
-		<a href="https://2014.igem.org/Team:INSA-Lyon/Results" class="hu-icon"><li class="iconmulti"  style="line-height:40px;  ">RESULTS</li></a>
+		<a href="https://2014.igem.org/Team:INSA-Lyon/Results" class="hu-icon"><li class="icon">RESULTS</li></a>
-		<a href="https://2014.igem.org/Team:INSA-Lyon/Notebook" class="hu-icon"><li class="iconmulti"  style="line-height:40px;  ">NOTEBOOK</li></a>
+		<a href="https://2014.igem.org/Team:INSA-Lyon/Notebook" class="hu-icon"><li class="icon">NOTEBOOK</li></a>
-		<a href="https://2014.igem.org/Team:INSA-Lyon/Parts" class="hu-icon"><li class="iconmulti"  style="line-height:40px;  ">PARTS</li></a>
+		<a href="https://2014.igem.org/Team:INSA-Lyon/Protocol" class="hu-icon"><li class="icon">PROTOCOLS</li></a>
-		<a href="https://2014.igem.org/Team:INSA-Lyon/DataPage" class="hu-icon"><li class="iconmulti"  style="line-height:40px;  ">DATA PAGE</li></a>
+		<a href="https://2014.igem.org/Team:INSA-Lyon/DataPage" class="hu-icon"><li class="icon">DATA PAGE</li></a>
 				</ul>
 			</div>
@@ Line 23: / Line 23: @@
 		<div id="presentation">
 	<p></p>
-		</div>
-<li><div align="justified">
+<li><div align="justify">
-<p>5 biobricks have been constructed, three for Nickel chelation, three for promoter characterization.</p></br></br></br><div>
+<p>5 biobricks have been constructed, thre for Nickel chelation, two for promoter characterization.</p></br>
 <b>Biobricks for nickel chelation</b></br></br>
-<p>The principal of the construction is shown in the figure below.</p></br></br></br>
+<p>The principal of the construction is shown in the figure below.</p></br></br></br></div>
 <li><div align="center">
 <img src= "https://static.igem.org/mediawiki/parts/6/63/1.JPG"></br>
-<li><div align="justified">
+<li><div align="justify">
-<p>On a pSB1C3 backbone, two essential part have been assembled: a promoter and a reporter coding for CsgA.The promoter in this case is always the same: P70.However, the reporter is different for each construction.<div>
+<p>On a pSB1C3 backbone, two essential part have been assembled: a promoter and a reporter coding for CsgA.The promoter in this case is always the same: P70.However, the reporter is different for each construction.</br>
+The first CsgA is called CsgA WT, the sequence is exactly the same as we found in a wild type CsgA protein except one mutation in order to eliminate one restriction site. The construction is also called CsgA-WT.</br>
+The second CsgA is based on the same sequence but with a short sequence coding for a his tag(a peptide chain coding six histidines). This construction is called CsgA-His1.</br>
+The last CsgA is almost the same but with 2 his tag. This construction is called CsgA-His2.</br>
-<li><div align="justified">
-<p>The first CsgA is called CsgA WT, the sequence is exactly the same as we found in a wild type CsgA protein except one mutation in order to eliminate one restriction site. The construction is also called CsgA.</p></br></br></br><div>
-<li><div align="justified">
-<p>The second CsgA is based on the same sequence but with a short sequence coding for a his tag(a peptide chain coding six histidines). This construction is called His1.</p></br></br></br><div>
-<li><div align="justified">
-<p>The last CsgA is almost the same but with 2 his tag. This construction is called His2.</p></br></br></br><div>
-<li><div align="justified">
-<p>5 biobricks have been constructed, three for Nickel chelation, three for promoter characterization.</p></br></br></br><div>
-<b>Biobrick for promoter characterization</b></br></br>
-<p>The principal of the construction is shown in the figure below.</p></br></br></br>
-<li><div align="center">
-<img src= "https://static.igem.org/mediawiki/parts/f/fb/2.png"></br>
-<li><div align="justified">
-<p>On a pKK backbone, two essential parts have been assembled: a promoter and a reporter.
-The reporter in this case is always the same: gfp. However, the promoter is different for each construction.<div>
-<li><div align="justified">
-<p>The first promoter is P70, sequence found in the Resgistry. This construction is called p70::gfp</p></br></br></br><div>
-<li><div align="justified">
-<p>The second promoter is PCurli, obtained from a PCR, sequence coding for the inter-genic regulation for curli production. This construction is called pcurli::gfp.</p></br></br></br><div>
 </div></li>
+</div>