Team:Paris Bettencourt/Notebook/Human Practice/Monday 12th August.html

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<h2>Phage Sensor</h2>
 
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<a href="https://2013.igem.org/Team:Paris_Bettencourt/Project/Phage_Sensor" target="_blank" class="tbnotelogo PSlogo"> ASDF </a>
 
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<div style="clear: both;"></div>
 
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<h3>Monday 12<sup>th</sup> August</h3>
 
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<p><b><em>
 
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Glycerol Stock, Miniprep, M13 plate test, Patches
 
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<b>Glycerol Stock</b>
 
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sSP018 - NEB with E1010<br>
 
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sSP017<br>
 
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sSP016<br>
 
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Take 1.5ml of ON culture + 500ul Glycerol (60%)<br>
 
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Freeze at -80°C<br>
 
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<br>
 
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<b>Miniprep</b><br>
 
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E1010<br>
 
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J04450<br>
 
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<br>
 
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1) Pellet 2x 9ml of liquid culture (4000rpm, 10 min)<br>
 
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2) Discard supernatant<br>
 
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3) resuspend the cells in 250ul of resuspension olution<br>
 
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4) add 250ul of lysis solution, mix by inverting 4-6 times<br>
 
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5) add 350ul of neutralization solution<br>
 
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4) centrifuge for 5 min<br>
 
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5) transfer supernatant to spin column<br>
 
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6) centrifuge for 1 min<br>
 
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7) discard flow through<br>
 
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8) add 500 ul wash solution and centrifuge for 1 min , discard flow through(repeat this step)<br>
 
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9) centrifuge for 1 min to remove left over liquid<br>
 
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10) transfer the column on a 1.5ml tube<br>
 
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11) add 50ul of elution buffer and incubate for 2 min<br>
 
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12) centrifuge for 2 min<br>
 
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13) Nanodrop the concentration and freeze at -20°<br>
 
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<br>
 
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J04450: ng/ul<br>
 
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E1010: ng/ul<br>
 
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<br>
 
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<br>
 
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<b>M13 plate test</b><br>
 
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1) 100 μ l of plating bacteria per tube<br>
 
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2) Prepare tenfold serial dilutions (10-6  to 10-9 ) of the bacteriophage stock in LB<br>
 
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3) Put 10 μ l/ 100 μ l of each dilution to the bacteria<br>
 
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4)  Mix the bacteriophage particles with the bacterial culture by vortexing gently.<br>
 
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5) Add 40 μ l of X-gal solution (working conc) and IPTG (working conc) solution to each of the tubes<br>
 
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6) Add 3ml of Agar to each tube and gently vortexing for 3 seconds<br>
 
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7) Pour the mixture onto  plates containing LB medium supplemented with 5 mM MgCl2 <br>
 
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8) Swirl the plate gently to ensure an even distribution of bacteria and agar.<br>
 
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9) Incubate them at 37°C.<br>
 
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<br>
 
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<b>Patches</b><br>
 
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check them and prepare new ones of those that haven’t been done yet<br>
 
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</div>
 
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</html>
 

Latest revision as of 17:28, 23 August 2013