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 {{US_AFRL_CarrollHS}}
-{{US_AFRL_CarrollHS_Project_Background}}
+{{US_AFRL_CarrollHS_Content_Start}}
 <html>
+<style>
-<div class="column full_size">
+#content {
+    background: #FFF;
+}
-<h1>Experiments</h1>
-<p>Describe the research, experiments, and protocols you used in your iGEM project. These should be detailed enough for another team to repeat your experiments.</p>
-<p>
+.hero-image {
-Please remember to put all characterization and measurement data for your parts on the corresponding Registry part pages.
+    background-image: url("https://static.igem.org/mediawiki/2017/f/f4/US_AFRL_CarrollHS_Experiments.jpg");
-</p>
+}
+</style>
+<div class="hero-image">
+  <div class="hero-text">
+    <h1>Experiments</h1>
+    <p><b> </p></b>
+  </div>
 </div>
-<div class="column half_size">
+<div class="text">
-<h5>What should this page contain?</h5>
+<h2>Transformations</h2>
+<h3>BI21 Cells:</h3>
+<p>
+<ol>
+<li>Thaw 50 µL vial of BL21 cells on ice</li>
+<li>Inoculate 2µL DNA into 50µL BL21 cells</li>
 <ul>
-<li> Protocols </li>
+<li>incubate on ice for 30 minutes</li>
-<li> Experiments </li>
+<li>heat shock at 42℃ for 10 seconds</li>
-<li> Documentation of the development of your project </li>
+<li>incubate on ice for 5m</li>
 </ul>
+<li>Inoculate 250µL LB into vial</li>
+<ul>
+<li>incubate at 37℃ with shaking for 1.5 hours</li>
+</ul>
+<li>Plate 1x/9x</li>
+</ol>
+</p>
-</div>
+<h3>JM109 Cells:</h3>
+<p>
-<div class="column half_size">
+<ol>
-<h5>Inspiration</h5>
+<li>Thaw vial of JM109 cells on ice</li>
+<li>Label 14 mL Falcon tube & plane on ice</li>
+<li>Inoculate 50 µL JM109 cells into Falcon tube</li>
+<li>Inoculate 2µL DNA into 50µL JM109 cells</li>
 <ul>
-<li><a href="https://2014.igem.org/Team:Colombia/Protocols">2014 Colombia </a></li>
+<li>incubate on ice for 20m</li>
-<li><a href="https://2014.igem.org/Team:Imperial/Protocols">2014 Imperial </a></li>
+<li>heat shock at 42℃ for 45 seconds</li>
-<li><a href="https://2014.igem.org/Team:Caltech/Project/Experiments">2014 Caltech </a></li>
 </ul>
+<li>Inoculate 950µL LB into vial</li>
+<ul>
+<li>incubate at 37℃ with shaking for 1.5 hours</li>
+</ul>
+<li>Plate 1x/9x</li>
+</ol>
+</p>
+<br>
 </div>
-<div class="clear"></div>
+<div class="text2">
+<h2>Electrophoresis/Gel Protocols</h2>
+<h3>1% Agarose Electrophoresis Gel</h3>
+<ol>
+<li>Add 0.35 g agarose to 35 mL 1x TAE in 100mL conical flask</li>
+<li>Heat in microwave for 35 seconds</li>
+<li>Swirl and heat in microwave for 25 seconds</li>
+<li>Swirl and heat in microwave for 15 seconds</li>
+<li>Swirl and heat in microwave for 7 seconds</li>
+<li>Swirl and ensure no ‘floaties’ </li>
+<li>Cool outside of conical flask with water until ‘hand not’</li>
+<li>Pour into gel mold and add well comb</li>
+</ol>
-<div class="column half_size">
+<h3>Gel Extraction</h3>
+<ol>
+<li>Use ethanol-wiped scalpel to excise appropriate bands</li>
+<li>Mix and incubate at 50°C for 10 min</li>
+<ul>
+<li>Vortex every 2 mins until gel slice is completely dissolved</li>
+</ul>
+<li>Place nucleospin column into 2mL collection tube</li>
+<ul>
+<li>Add sample</li>
+<li>Centrifuge at 11,000 xg for 1 minute</li>
+<li>Discard throughflow and place column back in same tube</li>
+ </ul>
+<li>Add 700 mL Buffer NT3</li>
+<ul>
+<li>Centrifuge at 11,000 xg for 1 minute</li>
+<li>Discard throughflow and place column back in same tube</li>
+</ul>
+<li>Repeat step 4</li>
+<li>Centrifuge at 11,000 xg for another minute</li>
+<ul>
+<li>To remove buffer</li>
+<ul>
+<li>Discard throughflow</li>
+<li>Centrifuge at 11,00 xg for add minute</li>
+<li>Place column in a clean, labelled 1.5 mL tube </li>
+</ul>
+</ul>
+<li>Add 25 mL prewarmed (50°C) Buffer NE</li>
+<ul>
+<li>Incubate at 50°C for 5 min</li>
+<li>Centrifuge at 50 xg for 1 minute</li>
+<li>Centrifuge at 11,000 xg for 1 minute</li>
+</ul>
+</ol>
+<br>
+</div>
+<div class= "text">
+<h2>Plasmid Transformation Protocol</h2>
+<ol>
+<li>Aliquot 1 ml media into 1.5 mL tubes</li>
+<ul>
+    <li>Place in 42°C waterbath</li>
+</ul>
+<li>Prechill labelled 14 mL round-bottom falcon tubes</li>
+<ul>
+   <li>Add mL cell culture to tube</li>
+   <li>Add appropriate amount of ligase rxh (2-2.5 L)</li>
+   <li>Incubate in nice for 20 minutes</li>
+</ul>
+<li>Heat shock cells by placing at 42℃ for 45 seconds in waterbath </li>
+<ul>
+   <li>Place on ice for 2 minutes</li>
+</ul>
+<li>Add 950 mL preheated media to each tube</li>
+<ul>
+<li>Incubate at 37℃ with 215 rpm shaking for 1.5 hr -> 20 minutes</li>
+</ul>
+</ol>
+<h3>Plating</h3>
+<ol>
+<li>Plate on LB-antibiotic plates</li>
+<ul>
+<li>Plate 100 ml for 1x transformation</li>
+<li>Plate 100 mL 9x centrifuge remaining transformation at 2000 xg for 5 minutes and resuspended pellet in 100 L media </li>
+</ol>
+</div>
+<div class="text2">
+<h2>Plates Protocol</h2>
+<ol>
+<li>Follow LB Agar Recipe </li>
+   <ul>
+   <li>Make sure to put stirring bar in water</li>
+   <li>Needed to make into homogenous gel</li>
+   <li>Needs to be sterile</li>
+   </ul>
+<li>Put into Autoclave </li>
+   <ul>
+   <li>Lid should not be too tight</li>
+   </ul>
+<li>Put in ice bath42°C</li>
+   <ul>
+   <li>Cool till not burning hand</li>
+   <li>Put on stirring plate</li>
+   </ul>
+<li>Put sterilized plates in Lamenia shield</li>
+<li>Using micropipette put .5 mL of chlor. And amp. agar solution</li>
+   <ul>
+   <li>1000x dilution</li>
+   <li>Amp. has to be defrosted in dark drawer</li>
+   </ul>
+<li>Pour solution into plates</li>
+   <ul>
+   <li>Thin layer fill bottom</li>
+   <li>Take lid slightly off to prevent condensation</li>
+<br>
+</div>
+<div class="text">
+<h2>QIA Prep Spin Mini Prep Kit</h2>
+<ol>
+<li>Example for 18 mL LB add</li>
+<ul>
+   <li>18 L20 mg/ L Kanamycin (antibiotic)</li>
+   <li>18 L 50 mg/ L ampicillin</li>
+</ul>
+<li>Aliquot 3.5 mL into labelled round bottom falcon tubes</li>
+<li>Using sterile toothpicks- pick a single colony forming unit (cfu) and inoculate tube</li>
+   <ul>
+   <li>Incubate overnight at 37°C with 215 rpm shaking</li>
+   </ul>
+<li>To 100 mL 60% glycerol stock, add 300mL overnight culture to appropriately labelled tube</li>
+   <ul>
+   <li>Store at -80°C</li>
+   </ul>
+<li>Pellet remaining cells by centrifugation in 1.5 mL tube at 13,2000 rpm for 1 min</li>
+   <ul>
+   <li>Discard supernatant and repeat</li>
+   </ul>
+<li>Resuspend pellet in Buffer P1 250 mL </li>
+   <ul>
+   <li>Add 250 L Buffer, P2 and mix by inverting 10x</li>
+   <li>Add 350 L Buffer N3 and immediately mix by inverting 10x</li>
+   </ul>
+<li>Centrifuge at 13, 200 rpm for 10 minute</li>
+<li>Pipet supernatant into labelled QIA prep spin column</li>
+   <ul>
+   <li>Centrifuge at 13, 200 rpm for 1 minute</li>
+   <li>Discard thoroughflow </li>
+   </ul>
+<li>Wash column by adding .5 mL Buffer PB *regular for low copy number plasmids*</li>
+   <ul>
+   <li>Centrifuge at 13, 200 rpm for 1 minute</li>
+   <li>Discard thoroughflow </li>
+   </ul>
+<li>Wash by adding .75 mL Buffer PE</li>
+   <ul>
+   <li>Centrifuge at 13, 200 rpm for 1 minute</li>
+   <li>Discard thoroughflow </li>
+   <li>Centrifuge for an addition minute to ensure removal of residual wash buffer</li>
+   </ul>
+<li>Place spin column in a clean, labelled 1.5 mL tube </li>
+   <ul>
+   <li>Add 50 LEB to center of column & let stand for 1 minute at room temperature</li>
+   <li>Centrifuge at 12,000 rpm for 1 minute</li>
+   <li>Store at -20℃</li>
+   </ul>
+</ol>
 </div>
-</html>
+</html>{{US_AFRL_CarrollHS_Content_End}}{{US_AFRL_CarrollHS_Nav}}

Difference between revisions of "Team:US AFRL CarrollHS/Experiments"

Latest revision as of 22:10, 1 November 2017

Experiments

Transformations

BI21 Cells:

JM109 Cells:

Electrophoresis/Gel Protocols

1% Agarose Electrophoresis Gel

Gel Extraction

Plasmid Transformation Protocol

Plating

Plates Protocol

QIA Prep Spin Mini Prep Kit