Team:Groningen/Template/MODULE/Notebook/secretion/week9

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Latest revision as of 00:46, 18 October 2014

September 29 - October 5

Obtaining the anti-Pseudomonas aeruginosa system with Three-A assembly

Extra amounts of dspB, ssUSP45DspB with His-tag, aiiA, ssUSP45aiiA with His-tag, pLAS, the RBS, the double terminator, pSB2k3 vector, pSB1C3 vector and pSB1A3 vector were miniprepped to be used for the assembly

aiiA, dspB, ssUSP45DspB with His-tag and ssUSP45aiiA with His-tag were digested with XbaI and PstI, and the RBS was cut with EcoRI and SpeI

These were eventually ligated for 3 hours into pSB2K3 and transformed into E. coli NEB cells

Name assembly	Upstream part	Downstream part	Backbone
A1’	RBS	aiiA	pSB2K3
A2’	RBS	dspB	pSB2K3
A3’	RBS	dspB+HIS	pSB2K3
A4’	RBS	aiiA+HIS	pSB2K3

After growing them for 1 day, colony PCR was done on the correct clones, these were inoculated for plasmid extraction

Then A1’, A4’ was digested with XbaI and PstI. A2’ and A3’ was cut with EcoRI and SpeI. Then ligated

Name assembly	Upstream part	Downstream part	Backbone
A1”	RBS + aiiA	Double terminator	pSB1A3
A2”	pLAS	RBS + dspB	pSB1A3
A3”	pLAS	RBS + dspB+HIS	pSB1A3
A4”	RBS + aiiA+HIS	Double terminator	pSB1A3

After doing growing analyzing and miniprepping the correct clones, A1” and A3”was cut with EcoRI and SpeI. A2” and A4” was cut with XbaI and PstI and ligated afterwards

Name assembly	Upstream part	Downstream part	Backbone
A1”’	pLAS+RBS+dspB	RBS+aiiA+Dterm	pSB1C3
A2”’	pLAS+RBS+dspB+HIS>	RBS+aiiA+HIS+Dterm	pSB1C3

After transformation, the plasmids were isolated, and confirmed by sequencing

@@ Line 9: / Line 9: @@
 <div class="title">
-– 12 September
+September 29 - October 5
 </div>
@@ Line 18: / Line 18: @@
 <div class="text">
-<b>Goal:</b> analysis of the possible made Biobricks.
+Obtaining the anti-<i>Pseudomonas aeruginosa</i> system with Three-A assembly
 </div>
@@ Line 27: / Line 27: @@
 <div class="text">
-Because of the very low amount of gblocks given, a decision was made to do a PCR directly on the product itself, therefor multiplying it exponentially.
+Extra amounts of <i>dspB</i>, ssUSP45DspB with His-tag, <i>aiiA</i>, ssUSP45aiiA with His-tag, <i>pLAS</i>, the RBS, the double terminator, pSB2k3 vector, pSB1C3 vector and pSB1A3 vector were miniprepped to be used for the assembly
 </div>
@@ Line 36: / Line 36: @@
 <div class="text">
-All the O/N cultures were mini-prepped. The possible plasmids were cut with EcoRI and SpeI. After running on gel, the result showed us that 20 of the 40 clones contained all the Biobricks, though with a low yield of plasmids.
+<i>aiiA</i>, <i>dspB</i>, ssUSP45DspB with His-tag and ssUSP45aiiA with His-tag were digested with XbaI and PstI, and the RBS was cut with EcoRI and SpeI
 </div>
@@ Line 45: / Line 45: @@
 <div class="text">
-A new strategy of assembling has been prepared and primers for this strategy have been made.
+These were eventually ligated for 3 hours into pSB2K3 and transformed into <i>E. coli</i> NEB cells
+</div>
+<div class="hspacer">&nbsp;</div>
+<!-- PARAGRAPH SNIPPET END-->
+<!-- TABLE SNIPPET OPTIONAL START-->
+<table class="table">
+<tr>
+<th>Name assembly</th><th>Upstream part</th><th>Downstream part</th><th>Backbone</th>
+</tr>
+<tr>
+<td>A1’</td><td>RBS</td><td><i>aiiA</i></td><td>pSB2K3</td>
+</tr>
+<tr>
+<td>A2’</td><td>RBS</td><td><i>dspB</i></td><td>pSB2K3</td>
+</tr>
+<tr>
+<td>A3’</td><td>RBS</td><td><i>dspB+HIS</i></td><td>pSB2K3</td>
+</tr>
+<tr>
+<td>A4’</td><td>RBS</td><td><i>aiiA+HIS</i></td><td>pSB2K3</td>
+</tr>
+</table>
+<div class="hspacer">&nbsp;</div>
+<!-- TABLE SNIPPET OPTIONAL END-->
+<!-- PARAGRAPH SNIPPET START-->
+<div class="text">
+After growing them for 1 day, colony PCR was done on the correct clones, these were inoculated for plasmid extraction
 </div>
@@ Line 54: / Line 84: @@
 <div class="text">
-All the Biobricks were send for sequencing.
+Then A1’, A4’ was digested with XbaI and PstI. A2’ and A3’ was cut with EcoRI and SpeI. Then ligated
 </div>
@@ Line 60: / Line 90: @@
 <!-- PARAGRAPH SNIPPET END-->
+<!-- TABLE SNIPPET OPTIONAL START-->
+<table class="table">
+<tr>
+<th>Name assembly</th><th>Upstream part</th><th>Downstream part</th><th>Backbone</th>
+</tr>
+<tr>
+<td>A1”</td><td>RBS + <i>aiiA</i></td><td>Double terminator</td><td>pSB1A3</td>
+</tr>
+<tr>
+<td>A2”</td><td><i>pLAS</i></td><td>RBS + <i>dspB</i></td><td>pSB1A3</td>
+</tr>
+<tr>
+<td>A3”</td><td><i>pLAS</i></td><td>RBS + <i>dspB+HIS</i></td><td>pSB1A3</td>
+</tr>
+<tr>
+<td>A4”</td><td>RBS + <i>aiiA+HIS</i></td><td>Double terminator</td><td>pSB1A3</td>
+</tr>
+</table>
+<div class="hspacer">&nbsp;</div>
+<!-- TABLE SNIPPET OPTIONAL END-->
+<!-- PARAGRAPH SNIPPET START-->
+<div class="text">
+After doing growing analyzing and miniprepping the correct clones, A1” and A3”was cut with EcoRI and SpeI. A2” and A4” was cut with XbaI and PstI and ligated afterwards
+</div>
+<div class="hspacer">&nbsp;</div>
+<!-- PARAGRAPH SNIPPET END-->
+<!-- TABLE SNIPPET OPTIONAL START-->
+<table class="table">
+<tr>
+<th>Name assembly</th><th>Upstream part</th><th>Downstream part</th><th>Backbone</th>
+</tr>
+<tr>
+<td>A1”’</td><td><i>pLAS</i>+RBS+<i>dspB</i></td><td>RBS+<i>aiiA</i>+Dterm</td><td>pSB1C3</td>
+</tr>
+<tr>
+<td>A2”’</td><td><i>pLAS</i>+RBS+<i>dspB+HIS</i>></td><td>RBS+<i>aiiA+HIS</i>+Dterm</td><td>pSB1C3</td>
+</tr>
+</table>
+<div class="hspacer">&nbsp;</div>
+<!-- TABLE SNIPPET OPTIONAL END-->
+<!-- PARAGRAPH SNIPPET START-->
+<div class="text">
+After transformation, the plasmids were isolated, and confirmed by sequencing
+</div>
+<div class="hspacer">&nbsp;</div>
+<!-- PARAGRAPH SNIPPET END-->
 <div class="hspacer">&nbsp;</div>