Difference between revisions of "Team:Munich/Parts"

Latest revision as of 03:47, 2 November 2017


Parts
Our team created new BioBricks for expressing and purifying the Cas13a protein used in our CascAID system and BioBricks for investigation of degradation tags with GFP.
Lwa Cas13a To express the core piece of our project, Cas13a, we cloned the protein sequence - in this set of biobricks for the version of Leptotrichia Wadei- into a psB1C3-backbone and fused it with several elements of our part collection. By equipping the Cas13a with a T7-promoter, a Tphi-Terminator , N-terminal 6xHis/Twin-strep tag for affinity-chromatography and Sumo tag for increased solubility, we created our favorite Biobrick: BBa_K2323004, customized for expression and purification of Lwa Cas13a. Other, more basic versions of this construct we submitted are BBa_K2323000 and BBa_K2323001. The results gained by the use of our purified Cas13a enzymes is described in readouts.
TEV protease To independently provide a tool for the removal of the affinity tag for our other Cas13a versions from Lsh and Lbu, we improved BBa_K1319004, submitted by the Aachen team 2014, coding for Tobacco Etch Virus-(TEV) protease by inserting the sequence for an N-termianl 6xHis Tag, creating BBa_K2323002. This way we were able to express and purify the protease ourselves and could also show that it posesses high cleavage activity with this improved BioBrick.This BioBrick will be useful for any future iGEM using proteins in a cell-free system.
Degradation Tags We created a library of GFP-containing constructs fused to different degradation tags which are targeted by the ClpP machinery of E. coli. The degradation tags for BBa_K2323003, BBa_K2323006, BBa_K232300, BBa_K2323008, and BBa_K2323009 were pdt2E, ASV, LAA, LVA, and pdt2B, respectively. Further, the constructs were put under control of a pTet promoter to make them inducable by aTc. After induction of protein expression in cell culure and stopping the translation with Chloramphenicol, the reaction rate of degradation for the different tags was measured (Figure 1). Figure 1: First order kinetics of degradation for different protein-degradation tags. Since these tags promote degradation at different rates which are described here and in more detail on the respective registry page, this degradation tag library can be used by future teams for creation and fine-tuning of bacterial systems.

<groupparts>iGEM17 Munich</groupparts>

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-<img id="TopPicture" width="960" src="https://static.igem.org/mediawiki/2017/b/be/T--Munich--FrontPagePictures_Attributions.jpg">
+<img id="TopPicture" width="960" src="https://static.igem.org/mediawiki/2017/6/6e/T--Munich--FrontPagePictures_Parts.jpg">
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-<font size=7 color=#51a7f9><b style="color: #51a7f9">Composite Parts</b></font>
+<font size=7 color=#51a7f9><b style="color: #51a7f9">Parts</b></font>
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 		<p class="introduction">
-	Thanks to advances in molecular biology and biochemistry, scientists have been able to consistently detect lower and lower concentration of molecules<sup><a class="myLink" href="#ref_1">1</a></sup>, to the point that single molecules can be reliably recognized with methods such as polymerase chain reaction (PCR)<sup><a class="myLink" href="#ref_2">2</a></sup>, fluorescence in situ hybridization (FISH)<sup><a class="myLink" href="#ref_3">3</a></sup> and enzyme-linked immunosorbent assays (ELISA)<sup><a class="myLink" href="#ref_4">4</a></sup>. This has opened doors for synthetic biology to create better and more accurate diagnostic tests that use biomarkers like nucleic acids and proteins as targets<sup><a class="myLink" href="#ref_5">5</a>,<a class="myLink" href="#ref_6">6</a></sup>. Through such advances, the field of molecular diagnostics developed. Unfortunately, current standard methods require expensive equipment or trained personnel, which generally limits their usability to hospitals or laboratories. Recently, there has been a push to develop new tests that fuse the reliability of standard methods with affordable platforms such as lab-on-a-chip or paper strips  to overcome this restrictions<sup><a class="myLink" href="#ref_7">7-9</a></sup>. We wanted to help close this gap and set out to engineer a diagnosis principle for the detection of a wide array of targets that could be used without difficult-to-meet technical requirements.
+	Our team created new BioBricks for expressing and purifying the Cas13a protein used in our CascAID system and BioBricks for investigation of degradation tags with GFP.
+</td>
+</tr>
+<tr><td colspan=6 align=center valign=center>
+<h3>Lwa Cas13a</h3>
+	<p>To express the core piece of our project, Cas13a, we cloned the protein sequence - in this set of biobricks for the version of Leptotrichia Wadei- into a psB1C3-backbone and fused it with several elements of our part collection.
+	By equipping the Cas13a with a T7-promoter, a Tphi-Terminator , N-terminal 6xHis/Twin-strep tag for affinity-chromatography and Sumo tag for increased solubility, we created our favorite Biobrick: <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323001">BBa_K2323004</a>, customized for expression and purification of Lwa Cas13a.
+	Other, more basic versions of this construct we submitted are BBa_K2323000 and BBa_K2323001.
+	The results gained by the use of our purified Cas13a enzymes is described in <a class="myLink" href="https://2017.igem.org/Team:Munich/Readouts">readouts</a>. </p>
+<tr><td colspan=6><h3>TEV protease</h3>
+	<p> To independently provide a tool for the removal of the affinity tag for our other Cas13a versions from Lsh and Lbu, we improved BBa_K1319004, submitted by the Aachen team 2014, coding for Tobacco Etch Virus-(TEV) protease by inserting the sequence for an N-termianl 6xHis Tag, creating <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323002">BBa_K2323002</a>. This way we were able to express and purify the protease ourselves and could also show that it posesses high cleavage activity with this <a class="myLink" href="https://2017.igem.org/Team:Munich/Improve">improved BioBrick</a>.This BioBrick will be useful for any future iGEM using proteins in a cell-free system.</p>
+</td></tr>
+<tr><td colspan=6><h3>Degradation Tags</h3>
+	 <p>We created a library of GFP-containing constructs fused to different degradation tags which are targeted by the ClpP machinery of <i>E. coli</i>. The degradation tags for <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323003">BBa_K2323003</a>, <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323006">BBa_K2323006</a>, <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323007">BBa_K232300</a>, <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323008">BBa_K2323008</a>, and <a class="myLink" href="http://parts.igem.org/Part:BBa_K2323009">BBa_K2323009</a> were pdt2E, ASV, LAA, LVA, and pdt2B, respectively.
+Further, the constructs were put under control of a pTet promoter to make them inducable by aTc.
+After induction of protein expression in cell culure and stopping the translation with Chloramphenicol, the reaction rate of degradation for the different tags was measured <b>(Figure 1)</b>. </p>
+	</div>
+<div class="captionPicture">
+<img height=400 src="https://static.igem.org/mediawiki/parts/4/4c/17-10-30_overview.png">
+<p>
+<b>Figure 1</b>: First order kinetics of degradation for different protein-degradation tags.
+</p>
+</div>
+ 	<p> Since these tags promote degradation at different rates which are described here and in more detail on the respective  <a class="myLink" href="http://parts.igem.org/wiki/index.php?title=Part:BBa_K2323003">registry page</a>, this degradation tag library can be used by future teams for creation and fine-tuning of bacterial systems.
                  </p>
 	</td>
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 </table>
-</section>
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