Difference between revisions of "Team:Tuebingen/Results"

Revision as of 23:39, 18 September 2015

Experiments

Results

Design

Parts

Safety

Interlabstudy

Notebook

Collaboration

References

SynBio-Day

SchoolClass@lab

Theatre Freiburg

<

>

Mutagenisation of the RFC10 restriction sites and the ApaI restriction site in the backbone of the pRS plasmids were performed by mutagenesis PCR. Positive clones were screened by restriction analysis with the respective restriction enzymes (compare plasmid maps: link [project description pRS vectors]).

Then, the old multiple cloning site (MCS) was replaced by restriction digest (ApaI, SacI) and subsequent ligation of annealed oligonucleotides containing matching overhangs. Verification of successful replacement of the old MCS was performed by using a restriction site that was only present in the initial pRS MCS (SalI).

Figure 1: Schematic agarose gel showing the migration pattern of various pRS plasmids incubated with different restriction enzymes.

Figure 2: Restriction analysis of various pRS plasmid constructs.

In figure 1, a schematic agarose gel showing the migration pattern of the three pRS vectors when digested with different restriction enzymes is depicted. Figure 2 shows the restriction analysis of various pRS plasmid constructs. The used pRS vectors show the expected migration behaviour. Lane 3 in figure 2c shows an additional fragment at around 5 kb which indicates an incomplete digestion of the pRS316 plasmid. In summary, every RFC10 restriction site in the pRS plasmid backbones was removed and the MCS was replaced. Unfortunately, due to time constraints we were not able to insert a terminator.

@@ Line 2: / Line 2: @@
 <html>
-<h2> Project Results</h2>
+	<script type="text/javascript">
+		dias = ['pRS-Vectors', 'Dronpa-caged Cre', 'Cre Reporter', 'Sensor/Promotors'];
+	</script>
+	<div id="dia0" class="dia">
+<p>Mutagenisation of the RFC10 restriction sites and the ApaI restriction site in the backbone of the pRS plasmids were performed by mutagenesis PCR. Positive clones were screened by restriction analysis with the respective restriction enzymes (compare plasmid maps: link [project description pRS vectors]).</p>
+<p>Then, the old multiple cloning site (MCS) was replaced by restriction digest (ApaI, SacI) and subsequent ligation of annealed oligonucleotides containing matching overhangs. Verification of successful replacement of the old MCS  was performed by using a restriction site that was only present in the initial pRS MCS (SalI).</p>
+<img id="resultsprs1" style="max-width:100%;max-height:100%;display: block; margin-left: auto;margin-right: auto;" src="https://static.igem.org/mediawiki/2015/a/ad/Team_Tuebingen_pRS_Restriction.png"/>
+Figure 1: Schematic agarose gel showing the migration pattern of various pRS plasmids incubated with different restriction enzymes.
+<img id="resultsprs1" style="max-width:100%;max-height:100%;display: block; margin-left: auto;margin-right: auto;" src="https://static.igem.org/mediawiki/2015/d/de/Team_Tuebingen_pRS_restriction_wet.png"/>
+Figure 2: Restriction analysis of various pRS plasmid constructs.
+<p>In figure 1, a schematic agarose gel showing the migration pattern of the three pRS vectors when digested with different restriction enzymes is depicted. Figure 2 shows the restriction analysis of various pRS plasmid constructs. The used pRS vectors show the expected migration behaviour. Lane 3 in figure 2c shows an additional fragment at around 5 kb which indicates an incomplete digestion of the pRS316 plasmid. In summary, every RFC10 restriction site in the pRS plasmid backbones was removed and the MCS was replaced.
+Unfortunately, due to time constraints we were not able to insert a terminator.</p>
-<p>Here you can describe the results of your project and your future plans. </p>
+        </div>
-<h5>What should this page contain?</h5>
+	<div id="dia1" class="dia">
-<ul>
+        </div>
-<li> Clearly and objectively describe the results of your work.</li>
-<li> Future plans for the project </li>
-<li> Considerations for replicating the experiments </li>
-</ul>
-<h4> Project Achievements </h4>
-<p>You can also include a list of bullet points (and links) of the successes and failures you have had over your summer. It is a quick reference page for the judges to see what you achieved during your summer.</p>
-<ul>
-<li>A list of linked bullet points of the successful results during your project</li>
-<li>A list of linked bullet points of the unsuccessful results during your project. This is about being scientifically honest. If you worked on an area for a long time with no success, tell us so we know where you put your effort.</li>
-</ul>
-<h4>Inspiration</h4>
-<p>See how other teams presented their results.</p>
-<ul>
-<li><a href="https://2014.igem.org/Team:TU_Darmstadt/Results/Pathway">2014 TU Darmstadt </a></li>
-<li><a href="https://2014.igem.org/Team:Imperial/Results">2014 Imperial </a></li>
-<li><a href="https://2014.igem.org/Team:Paris_Bettencourt/Results">2014 Paris Bettencourt </a></li>
-</ul>
+	<div id="dia2" class="dia">
+        </div>
+	<div id="dia3" class="dia">
+        </div>
 </div>
 </html>