Latest revision as of 10:38, 6 September 2013

Iron coli project

Notebook

Protocols

Primers

Weeks

Month	Week
Jun.	1	2
Jul.	3	4	5	6
Aug.	7	8	9	10	11
Sep.	12	13	14	15
Oct.	16	17	18	19	20

Homologous Recombination

Aim

Preparation

Be careful, all recombination protocols should be done at 30°C unless indicated otherwise !

Strain Preparation

Transform the PTKred Plasmid¹ with the strain of interest.
Start an over night culture with the strain transformed with PTKred at 30°C.
Dilute the overnight culture in a ratio of 1 mL/100 mL and add IPTG (isopropyl β-D-1-thiogalactopyranoside; final concentration of 2 mM) and Spectinomycin (60 mg/mL).
Grow up to OD600: 0.5 then make electrocompetent cells .

Integration

Prepare the PCR fragment to be integrated flanked by 50 bp genomic sequences.
Gel-purify the product and transform with the electrocompetent PTKred strain.
Recover in LB for 2 hours with IPTG.
After 2 hours incubation add the selective drug which should be inserted in the genom (for example kanamycin if you have kan R cassette inserted) and incubate overnight in liquid culture at 30°C.
Next day, culture should be very turbid or the recombination did not work. Plate streak 50 μL of the overnight culture on a plate containing selection drug which in this case is kanamycin and grow overnight at 30°C.
Next day pick a colony and make glycerol stocks

Elimination of PTKred plasmid

Inoculate the strain that you have made by Homologous Recombination in LB overnight with spectinomycin at 30°C.
Adding spectinomycin in this step ensures that the plasmid will not integrate in the genome in a rare occurrence.
Dilute 1/100 and grow at 42°C for 4 hours and then plate sreak 50 μL of the culture on LB plate at 42°C.
Next day, pick colonies and grid plate on LB then spectinomycin and grow at 37°C.

Flip Recombinase and Anti-biotic Resistance Gene

Transform a cured strain with PCP20 plasmid
Grow overnight in LB with Cam at 30°C overnight.
Dilute 1/100 and grow for 3 hours at 37°C.
Streak plate on LB plates and grow over night at 42°C.
Repeart the grid plating as in the following diagram:

AJouter image

Reference:

http://www.addgene.org/41062/

@@ Line 22: / Line 22: @@
 <p>
-Transform the PTKred Plasmid with the strain of interest.
+Transform the PTKred Plasmid<a href='http://www.addgene.org/41062/' target='_blank'><small><sup>1</small></sup></a> with the strain of interest.
 <br>Start an over night culture with the strain transformed with PTKred at 30°C.
@@ Line 28: / Line 28: @@
 <br>Dilute the overnight culture in a ratio of 1 mL/100 mL and add IPTG (isopropyl β-D-1-thiogalactopyranoside; final concentration of 2 mM) and Spectinomycin (60 mg/mL).
-<br>Grow up to OD600: 0.5 then make <a href="https://2013.igem.org/Team:Evry/Protocols/01">electrocompetent cells</a> .
+<br>Grow up to OD600: 0.5 then make <a href="https://2013.igem.org/Team:Evry/Protocols/01" target='_blank'>electrocompetent cells</a> .
 </p>
@@ Line 36: / Line 36: @@
 Prepare the PCR fragment to be integrated flanked by 50 bp genomic sequences.
-<br>Gel-purify the product and transform with the electrocompetent PTKred strain.
+<br><a href="https://2013.igem.org/Team:Evry/Protocols/11" target='_blank'>Gel-purify</a> the product and transform with the electrocompetent PTKred strain.
-<br>Recover in LB for 2 hours with IPTG and spectinomycin.
+<br>Recover in LB for 2 hours with IPTG.
-<br>After 2 hours incubation add the selective drug which should be inserted in the genome (for example kanamycin if you have kan R cassette inserted ) and incubate overnight in liquid culture at 30°C.
+<br>After 2 hours incubation add the selective drug which should be inserted in the genom (for example kanamycin if you have kan R cassette inserted) and incubate overnight in liquid culture at 30°C.
-<br>Next day, culture should be very turbid or the recombination did not work. Plate streak 50 μL of the overnight culture on a plate containing selection drug which in this case is Kanamycin and grow overnight at 30°C.
+<br>Next day, culture should be very turbid or the recombination did not work. Plate streak 50 μL of the overnight culture on a plate containing selection drug which in this case is kanamycin and grow overnight at 30°C.
-<br>Next Day pick a colony and make Glycerol stocks
+<br>Next day pick a colony and make glycerol stocks
 </p>
@@ Line 51: / Line 51: @@
 <p>
 Inoculate the strain that you have made by Homologous Recombination in LB overnight with spectinomycin at 30°C.
+<br>
 <i>Adding spectinomycin in this step ensures that the plasmid will not integrate in the genome in a rare occurrence.</i>
-<br>Dilute 1/100 and grow at <b>42°C</b> for 4 hours and then plate sreak 50 μL of the culture om LB plate at <b>42°C</b>.
+<br>Dilute 1/100 and grow at <b>42°C</b> for 4 hours and then plate sreak 50 μL of the culture on LB plate at <b>42°C</b>.
 <br>Next day, pick colonies and grid plate on LB then spectinomycin and grow at <b>37°C</b>.
 </p>
@@ Line 60: / Line 61: @@
-<p>Transform a cured strain with PCP20 plasmid
+<p>
+<a href="https://2013.igem.org/Team:Evry/Protocols/02" target='_blank'>Transform</a> a cured strain with PCP20 plasmid
 <br>Grow overnight in LB with Cam at 30°C overnight.
-<br>Dilute 1/100 and grow for 3hrs at <b>37°C</b>.
+<br>Dilute 1/100 and grow for 3 hours at <b>37°C</b>.
 <br>Streak plate on LB plates and grow over night at <b>42°C</b>.
-<br>Repeart the grid plating as in the diagram
+<br>Repeart the grid plating as in the following diagram:
 <h1> AJouter image</h1>
 </p>
+<div id="citation_box">
+ <p id="references">Reference:</p>
+ <ol>
+  <li>http://www.addgene.org/41062/</li>
+ </ol>
+</div>
 </div>

Team:Evry/Protocols/10

From 2013.igem.org