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-	<a href='https://2013.igem.org/Team:Evry/Protocoles/01' title='Vers la page française'> <img src='https://static.igem.org/mediawiki/2013/b/b9/Francais.jpg'/></a>	+	<a href='https://2013.igem.org/Team:Evry/Protocoles/03' title='Vers la page française'> <img src='https://static.igem.org/mediawiki/2013/b/b9/Francais.jpg'/></a>
-	<h1 align='center'> Competents cells </h1>	+	<h1 align='center'> Plasmid purification </h1>
-	First prepare the following solutions required to make competent cells:<br/>	+	<i>Protocole from Macherey-Nagel plasmid purification notebook</i><br><br>
-	Solution for 1M Cacl2:<br/>	+
-	Add 14,30g of CaCl2 into 100 ml desalted water<br/>	+
-	<br/>	+
-	Solution for 0,1M Cacl2:<br/>	+	<b>. Récupération des bactéries</b><br>
-	Add 50 mL of CaCl2 1M solution into 450 ml of desalted water<br/>	+	Set saturated E.coli LM culture into 2 mL tubes. Centrifuge at 11 000 x g for 30 secondes. Discard as much as supernatant as possible.<br><br>
-	<br/>	+
-	Solution for 0,1M Cacl2 + 15% glycerol:<br/>	+	<b>.Cell lysis</b> <br>
-	Add 50 mL of CaCl2 1M solution and 75 mL of glycerol 100% into 450 ml of desalted water<br/>	+	Add 250 μL Buffer A1 (resuspension buffer). Resuspend the cells with a vortex or a pipette.
-	</p>	+	<br>
-	<br/>	+	Add 250 μL Buffer A2 (lysis buffer). Mix gently by inverting the tube 6 - 8 times. Incubate at room temperature until lysate appears clear.<br>
-	<p>For 200 ml LB medium, add 400 µL of strain sample.<br/>	+	Add 300 μL Buffer A3 (neutralisation buffer). Mix thoroughly by inverting the tube 6 - 8 times .<br>
-	Let the bacteria grow until it reaches an OD between 0,3 and 0,35.<br/>	+
-	Once it reached the right OD, put the medium on ice for 30 minutes to slow down growth.<br/>	+	<b>. Clarification of lysate</b><br>
-	Split the 200 mL into 4x50 mL tubes then centrifuge at 3000 rpm for 5 minutes at 4°C and suppress supernatant afterwards.<br/>	+	Centrifuge at 11 000 x g for 5 minutes . Repeat this step until supernatant is not clear.<br><br>
-	Resuspend the cells with 5 mL of Cacl2 at 0,1M for each 50 mL tube.<br/>	+
-	Again, put the medium on ice for 30 minutes.<br/>	+	<b>.Bind ADN<br></b>
-	Centrifuge at 3000 rpm for 5 minutes at 4°C then suppress supernatant.<br/>	+	Place a NucleoSpin Plasmid Column in a Collection Tube of 2 mL et and set the supernatant from the last step. Centrifuge at 11 000 x g for 1 minute. Discard flow-through and place the column back into the collection tube.<br><br>
-	Resuspend the cells with 1 mL of Cacl2 at 0,1M + 15% glycerol for each 50 mL tube.<br/>	+
-	Split the total 4 mL into 40 tubes containing each 100 µL of concentrated cell solution. This step should be executed fast enough and on ice.<br/></p>	+	<b>. Wash membrane<br></b>
		+	Add 600 μL Buffer A4 (wash buffer) previously supplemented with ethanol. Centrifuge ar 11 000 x g for 1 minute. Discard flow-through and place the column back into an empty collection tube.<br>
		+
		+	<b>. Dry membrane<br></b>
		+	Centrifuge at 11 000 x g for 2 minutes and discard the collection tube.<br><br>
		+
		+	<b>. Elution de l'ADN<br></b>
		+	Place the column in a 1,5 mL and add 50 μL de Buffer AE (elution buffer). Incubate at room temperature and centrifuge at 11 000 x g for 1 minute.<br>
		+	Measure the concentration with nanodrop, then stock the tubes at -20°C<br>
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Revision as of 14:25, 30 July 2013

Plasmid purification

Protocole from Macherey-Nagel plasmid purification notebook

. Récupération des bactéries
Set saturated E.coli LM culture into 2 mL tubes. Centrifuge at 11 000 x g for 30 secondes. Discard as much as supernatant as possible.

.Cell lysis
Add 250 μL Buffer A1 (resuspension buffer). Resuspend the cells with a vortex or a pipette.
Add 250 μL Buffer A2 (lysis buffer). Mix gently by inverting the tube 6 - 8 times. Incubate at room temperature until lysate appears clear.
Add 300 μL Buffer A3 (neutralisation buffer). Mix thoroughly by inverting the tube 6 - 8 times .
. Clarification of lysate
Centrifuge at 11 000 x g for 5 minutes . Repeat this step until supernatant is not clear.

.Bind ADN
Place a NucleoSpin Plasmid Column in a Collection Tube of 2 mL et and set the supernatant from the last step. Centrifuge at 11 000 x g for 1 minute. Discard flow-through and place the column back into the collection tube.

. Wash membrane
Add 600 μL Buffer A4 (wash buffer) previously supplemented with ethanol. Centrifuge ar 11 000 x g for 1 minute. Discard flow-through and place the column back into an empty collection tube.
. Dry membrane
Centrifuge at 11 000 x g for 2 minutes and discard the collection tube.

. Elution de l'ADN
Place the column in a 1,5 mL and add 50 μL de Buffer AE (elution buffer). Incubate at room temperature and centrifuge at 11 000 x g for 1 minute.
Measure the concentration with nanodrop, then stock the tubes at -20°C