Team:Aix-Marseille/Notebook ChassisConstruct

From 2014.igem.org

(Difference between revisions)

Revision as of 00:49, 12 October 2014

Week 7 : 08/11/2014 ➡ 08/17/2014

We have control if the insert of FRT-Kan-FRT is in the gene sdaBC and CheA by PCR.

#	DNA Template	Primers Name	Weight of amplified DNA
180	Genomic DNA of W3110	CheA_up CheA_down	1700
181	CheA-	CheA_up CheA_down	1500
182	Genomic DNA of W3110	sdaBC_up sdaBC_down	3100
183	sdaBC- KanR	sdaBC_up sdaBC_down	1500
184	sdaBC- KanR + pCP20	sdaBC_up sdaBC_down	1500

CheA- control is unsuccessful, we see a weight of amplification for #180 and #181 of 1700bp the gene FRT-Kan-FRT isn't insert in cheA.

>SdaBC- control have a problem we don't have amplification for #182 to #184.

Results not shown.

We made a PCR with new oligo to control mutants.

#	DNA Template	Primers Name	Weight of amplified DNA
185	Genomic DNA of W3110	CheA_check_up CheA_check_down	1700
186	CheA-	CheA_check_up CheA_check_down	1500
187	Genomic DNA of W3110	sdaBC_check_up sdaBC_check_down	3100
188	sdaBC- KanR	sdaBC_check_up sdaBC_check_down	1500
189	sdaBC- KanR + pCP20	sdaBC_check_up sdaBC_check_down	1500
190	Genomic DNA of W3110	FRT_up sdaBC_check_down	0
191	sdaBC- KanR	FRT_up sdaBC_check_down	1600
192	sdaBC- KanR + pCP20	FRT_up sdaBC_check_down	1600

Second control of CheA- show us the gene FRT-Kan-FRT isn't in the gene cheA

SdaBC control have an other problem with amplification

Results not shown.

We made a gradient PCR 55° to 65° with oligo sdaBC_checkdo/FRTup and W3110 sdaBC- strain and W3110 Wild type.

No amplification shown by the electrophoresis for all these PCR.

Results not shown

Week 8 : 08/18/2014 ➡ 08/24/2014

We made Q5 PCR with oligo 1-2 and 3-4 on pKD4 template for prepare new transformation sdaBC and cheA respectively #293 and #294. After we supress the template pKD4 with
We purified PCR products #293 thanks to Macherey Nagel PCR Clean up Kit.

293 22.65 ng.mL^-1

We made 2 new PCR on transformed strains. With specific hybridation temperature.

#	DNA Template	Primers Name	Weight of amplified DNA	Hybridation Temperature
300A	CheA-	CheA_check_up CheA_check_down	1500	55°C
301A	sdaBC- KanR	FRT_up sdaBC_check_down	1600	50°C

We made a PCR with new oligo to control mutants.

#	DNA Template	Primers Name	Weight of amplified DNA
185	Genomic DNA of W3110	CheA_check_up CheA_check_down	1700
186	CheA-	CheA_check_up CheA_check_down	1500
187	Genomic DNA of W3110	sdaBC_check_up sdaBC_check_down	3100
188	sdaBC- KanR	sdaBC_check_up sdaBC_check_down	1500
189	sdaBC- KanR + pCP20	sdaBC_check_up sdaBC_check_down	1500
190	Genomic DNA of W3110	FRT_up sdaBC_check_down	0
191	sdaBC- KanR	FRT_up sdaBC_check_down	1600
192	sdaBC- KanR + pCP20	FRT_up sdaBC_check_down	1600

After the electrophoresis, we can confirm The strain sdaBC- KanR is successful. We select 3 strains with electrophoresis control

C.23 and C.33 are contaminated. So we select C.43, C.53 and C.63.

We prepare seven starter of W3110 sdaBC- KanR strain with Kan50.

We realize day 7 of Lambda Red protocol on W3110 sdaBC- pCP20 strain.

We realize day 8 of Lambda Red protocol on W3110 sdaBC- strain.

Week 9 : 08/25/2014 ➡ 08/31/2014

We realize day 9 of Lambda Red protocol on W3110 sdaBC- strain, and day 2 of Lambda Red protocol on W3110 sdaBC- strain with #294 PCR product

We realize day 3 of Lambda Red protocol on W3110 sdaBC- strain CheA- KanR.
Check the construction 200(2) (RBS B0034 + RFP E1010) by digestion.

7µL E1010 (control) (500ng)
36µL H2O
5µ NEB Buffer 2.1
1µL XbaI
1µL EcoRI

2µL 200(2) (500ng)
36µL H2O
5µ NEB Buffer 2.1
1µL XbaI
1µL EcoRI

Incubation 53' at 37°C. Then, inactivation of enzymes 25' at 80°C.

It is difficult to see if 200(2) possesses the RBS. The plasmid 200(2) is sent to sequencing and it's OK.

We realize day 4 of Lambda Red protocol on W3110 sdaBC- strain CheA- KanR. strain.

We realize day 5 of Lambda Red protocol on W3110 sdaBC- CheA- KanR strain.

@@ Line 81: / Line 81: @@
-  <div class="container">
-    <h1>Notebook: Chassis Construction</h1>
-    <br><br>
-    <div id="stop_top"></div>
-    <div class="row" style="position:relative;" id="notebook-row">
-      <div class="col-md-9" id="notes"><!-- NOTES -->
                     <!-- ======= WEEK 7 ======= -->
@@ Line 438: / Line 431: @@
                    <li>
                      <p>We realize day 3 of Lambda Red protocol on W3110 sdaBC- strain CheA- KanR.</p>
+                  </li>
+                  <li>
+                    <p>Check the construction 200(2) (RBS B0034 + RFP E1010) by digestion.</p>
+                    <p>7µL E1010 (control) (500ng)<br>36µL H2O<br>5µ NEB Buffer 2.1<br>1µL XbaI<br>1µL EcoRI</p>
+                    <br>
+                    <p>2µL 200(2) (500ng)<br>36µL H2O<br>5µ NEB Buffer 2.1<br>1µL XbaI<br>1µL EcoRI</p>
+                    <p>Incubation 53' at 37°C. Then, inactivation of enzymes 25' at 80°C.</p>
+                    <div class="media notes-media">
+                      <img class="https://static.igem.org/mediawiki/2014/e/e7/AMU_Team-0826.png" style="width:350px">
+                      <div class="media-body">
+                        <p>It is difficult to see if 200(2) possesses the RBS. The plasmid 200(2) is sent to sequencing and it's OK.</p>
+                      </div>
+                    </div>
                    </li>
                  </ul>

Team:Aix-Marseille/Notebook ChassisConstruct

From 2014.igem.org

Revision as of 00:49, 12 October 2014

Week 7 : 08/11/2014 ➡ 08/17/2014

Week 8 : 08/18/2014 ➡ 08/24/2014

Week 9 : 08/25/2014 ➡ 08/31/2014

Week 7 08/11/14 → 08/17/14

Week 8 08/18/14 → 08/24/14

Week 9 08/25/14 → 08/31/14

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