Latest revision as of 18:05, 26 October 2012

Team Trieste iGEM 2012

Week 2

More

Suicide System

Finally we got by synthesis the antimicrobial peptide LL 37 cathelicidin (BBa_K875009) in pEX-A plasmid and we amplified it through the transformation of DH5-alpha bacteria.
The positive colonies were then digested EcoRI/SpeI, the fragment was eluted from the gel and then cut it again with EcoRI, because the pEX-A plasmid has another EcoRI restriction site downstream our fragment.
Then we did a column purification of the fragment and we successfully cloned the LL 37 into the pSB1C3 linearized backbone to make it ready for a potential submission.
LL 37 -previously cut EcoRI/SpeI- was cloned upstream the TT_B0015 and the DH5alpha cells were transformed with the plasmid (LL 37-B0015). The positive colonies were inoculated and then cloned downstream the RBS_B0034.

We also cloned the T5LacOperator inside the pSB1C3 plasmid, making it ready for the submission.

Antibody

We cloned the synthetized DNA sequence rbs-pelB-SIP 54.6-6HIS upstream the double terminator B0015 and then we ligated successfully the whole fragment under T5LacO. We introduced the resulting plasmid into E. coli strain W3110 already transformed with plasmid p-REP 4 coding for T5Lac Repressor.

Cumate-Switch Regulation

We received the two plasmids that we had built and ordered. The first one contains the RBS - CymR - SV5 tag (730bp), the second one contains T5 promoter - Cumate operator (129 bp).

Contact us

For other information, write to:

igem2012@gmail.com

@@ Line 11: / Line 11: @@
 		    <div id="suicide" class="notebook_section">
 		    	<h2 class="notebook_title">Suicide System</h2>
-Finally we got by synthesis the antimicrobial peptide LL37 cathelicidin (BBa_K875009) in pEX-A plasmid and we amplified it through the transformation of DH5-alpha bacteria.</br>
+Finally we got by synthesis the antimicrobial peptide LL 37 cathelicidin (BBa_K875009) in pEX-A plasmid and we amplified it through the transformation of DH5-alpha bacteria.</br>
-</br>
 The positive colonies were then digested EcoRI/SpeI, the fragment was eluted from the gel and then cut it again with EcoRI, because the pEX-A plasmid has another EcoRI restriction site downstream our fragment.</br>
-</br>
 Then we did a column purification of the fragment and we successfully cloned the LL 37 into the pSB1C3 linearized backbone to make it ready for a potential submission.</br>
-</br>
-We LL 37 -previously cut EcoRI/SpeI- was cloned upstream the TT_B0015 and the DH5alpha cells were transformed with the plasmid (LL-37-B0015). The positive colonies were inoculated and then cloned downstream the RBS_B0034.</br>
+LL 37 -previously cut EcoRI/SpeI- was cloned upstream the TT_B0015 and the DH5alpha cells were transformed with the plasmid (LL 37-B0015). The positive colonies were inoculated and then cloned downstream the RBS_B0034.</br>
 </br>
 We also cloned the T5LacOperator inside the pSB1C3 plasmid, making it ready for the submission.
@@ Line 23: / Line 22: @@
 		    <div id="antibody" class="notebook_section">
 		    	<h2 class="notebook_title">Antibody</h2>
-We cloned the synthetized DNA sequence rbs-pelB-SIP 54.6-6HIS upstream the double terminator B0015 and then we ligated successfully the whole fragment under T5LacO. We introduced  the resulting plasmid into E. coli strain W3110 already transformed with plasmid p-REP 4 coding for T5Lac Repressor.
+We cloned the synthetized DNA sequence rbs-pelB-SIP 54.6-6HIS upstream the double terminator B0015 and then we ligated successfully the whole fragment under T5LacO. We introduced  the resulting plasmid into <i>E. coli</i> strain W3110 already transformed with plasmid p-REP 4 coding for T5Lac Repressor.
 		    </div>
 		    <div id="chassis" class="notebook_section">
-		    	<h2 class="notebook_title">Chassis</h2>
+		    	<h2 class="notebook_title">Cumate-Switch Regulation</h2>
 We received the two plasmids that we had built and ordered.
-The first one contains the RBS - CymR - SV5 tag (730bp), the second one contain T5 promoter - Cumate operator (129 bp).
+The first one contains the RBS - CymR - SV5 tag (730bp), the second one contains T5 promoter - Cumate operator (129 bp).
 		    </div>
                  </div>
@@ Line 35: / Line 34: @@
              	<ul id="sub_menu">
 		    <li><a href="https://2012.igem.org/Team:Trieste/notebook">Week 1</a></li>
-                     <li><a href="https://2012.igem.org/Team:Trieste/notebook2">Week 2</a></li>
+                     <li class="select"  ><a href="https://2012.igem.org/Team:Trieste/notebook2">Week 2</a></li>
                      <li><a href="https://2012.igem.org/Team:Trieste/notebook3">Week 3</a></li>
                      <li><a href="https://2012.igem.org/Team:Trieste/notebook4">Week 4</a></li>
@@ Line 46: / Line 45: @@
                      <li><a href="https://2012.igem.org/Team:Trieste/notebook11">Week 11</a></li>
                      <li><a href="https://2012.igem.org/Team:Trieste/notebook12">Week 12</a></li>
+                    <li><a href="https://2012.igem.org/Team:Trieste/notebooklast">Post European-Jamboree</a></li>
                  </ul>
                  <img src="https://static.igem.org/mediawiki/2012/b/b0/Team_trieste.jpg" alt="Team iGEM 2012" id="igem_team" />
@@ Line 55: / Line 55: @@
                      Follow us also:
 			<a href="https://www.facebook.com/IGEMUNITS?ref=ts" target="_blank"><img src="https://static.igem.org/mediawiki/2012/f/f4/Ico_fb.png" alt="Facebook" class="fb" /></a>
-                         <a href="https://twitter.com/igemunits" target="_blank"><img src="https://static.igem.org/mediawiki/2012/2/21/Ico_twitter.png" alt="twitter" class="tw" /></a>
+                         <a href="https://twitter.com/iGEMTrieste" target="_blank"><img src="https://static.igem.org/mediawiki/2012/2/21/Ico_twitter.png" alt="twitter" class="tw" /></a>
                      </div>
                  </div>