Difference between revisions of "Team:TecCEM/Experiments"

 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol A / Chemocompetent cells
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Chemocompetent cell preparation
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol B / Cell transformation
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Chemocompetent cell transformation
 
                 <span class="caret"></span></button>
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol C / Annealing of oligonucleotides
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Annealing of oligonucleotides
 
                 <span class="caret"></span></button>
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol D / Plasmid digestion
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Plasmid digestion
 
                 <span class="caret"></span></button>
 
                 <span class="caret"></span></button>
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol E / Ligation
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Ligation
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol F / Lowry Method
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Lowry Method por protein quantification
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol G / Plasmid extraction
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Plasmid extraction
 
                 <span class="caret"></span></button>
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol H / SDS-PAGE
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">SDS-PAGE
 
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                             </tr>
 
                             </tr>
 
                             <tr>
 
                             <tr>
                                 <th></th>
+
                                 <th>H<sub>2</sub>O</th>
                                 <th></th>
+
                                <th>5.2 ml</th>
                                 <th></th>
+
                                <th>4.6 ml</th>
                                 <th></th>
+
                                <th>3.8 ml</th>
                                 <th></th>
+
                                <th>3.2 ml</th>
                                 <th></th>
+
                                <th>2.2 ml</th>
 +
                            </tr>
 +
                            <tr class = "parBackgroundColor">
 +
                                <th>Acrylamide/Bis-acrylamide (30%/0.8% w/v)</th>
 +
                                <th>2 ml</th>
 +
                                <th>2.6 ml</th>
 +
                                <th>3.4 ml</th>
 +
                                <th>4 ml</th>
 +
                                <th>5 ml</th>
 +
                            </tr>
 +
                            <tr>
 +
                                <th>1.5M Tris (pH 8.8)</th>
 +
                                 <th>2.6 ml</th>
 +
                                 <th>2.6 ml</th>
 +
                                 <th>2.6 ml</th>
 +
                                 <th>2.6 ml</th>
 +
                                 <th>2.6 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr class = "parBackgroundColor">
 
                             <tr class = "parBackgroundColor">
                                 <th></th>
+
                                 <th>10% w/v SDS</th>
                                 <th></th>
+
                                 <th>0.1 ml</th>
                                 <th></th>
+
                                 <th>0.1 ml</th>
                                 <th></th>
+
                                 <th>0.1 ml</th>
                                 <th></th>
+
                                 <th>0.1 ml</th>
                                 <th></th>
+
                                 <th>0.1 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr>
 
                             <tr>
                                 <th></th>
+
                                 <th>10% w/v ammonium persulfate</th>
                                 <th></th>
+
                                 <th>100 μl</th>
                                 <th></th>
+
                                 <th>100 μl</th>
                                 <th></th>
+
                                 <th>100 μl</th>
                                 <th></th>
+
                                 <th>100 μl</th>
                                 <th></th>
+
                                 <th>100 μl</th>
 
                             </tr>
 
                             </tr>
 
                             <tr class = "parBackgroundColor">
 
                             <tr class = "parBackgroundColor">
                                 <th></th>
+
                                 <th>TEMED</th>
                                 <th></th>
+
                                 <th>10 μl</th>
                                 <th></th>
+
                                 <th>10 μl</th>
                                 <th></th>
+
                                 <th>10 μl</th>
                                 <th></th>
+
                                 <th>10 μl</th>
                                 <th></th>
+
                                 <th>10 μl</th>
 
                             </tr>
 
                             </tr>
 
                         </table>
 
                         </table>
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                             <tr class = "parBackgroundColor">
 
                                 <th>H<sub>2</sub>O</th>
 
                                 <th>H<sub>2</sub>O</th>
                                 <th>2.975ml</th>
+
                                 <th>2.97 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr>
 
                             <tr>
                                 <th></th>
+
                                 <th>0.5 M Tris-HCl (pH 6.8)</th>
                                 <th></th>
+
                                 <th>1.25 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr class = "parBackgroundColor">
 
                             <tr class = "parBackgroundColor">
                                 <th></th>
+
                                 <th>10% w/v SDS</th>
                                 <th></th>
+
                                 <th>0.05 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr>
 
                             <tr>
                                 <th></th>
+
                                 <th>Acrylamide/Bis-acrylamide (30%/0.8% w/v)</th>
                                 <th></th>
+
                                 <th>0.67 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr class = "parBackgroundColor">
 
                             <tr class = "parBackgroundColor">
                                 <th></th>
+
                                 <th>10% w/v ammonium persulfate</th>
                                 <th></th>
+
                                 <th>0.05 ml</th>
 
                             </tr>
 
                             </tr>
 
                             <tr>
 
                             <tr>
                                 <th></th>
+
                                 <th>TEMED</th>
                                 <th></th>
+
                                 <th>0.005 ml</th>
 
                             </tr>                             
 
                             </tr>                             
 
                         </table>
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol I / Plasmid extraction
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Plasmid extraction with Monarch Miniprep Kit
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol J / DNA band purification
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">DNA band purification
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol K / Polymerase Chain Reaction
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Polymerase Chain Reaction
 
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Protocol L / Insect Medium
+
                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Schneider's Insect Medium preparation
 
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 +
                <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Sequencing Biobricks
 +
                <span class="caret"></span></button>
 +
                <div class="dropdown-menu">
 +
                    <h3>Sequencing Biobricks</h3>                   
 +
                    <object data="https://static.igem.org/mediawiki/2017/9/9b/TEC-CEM-Protocol_for_biobricks.pdf" type="application/pdf" width="100%" height="900px" internalinstanceid="11">
 +
                <p>It appears you don't have a PDF plugin for this browser.
 +
                    No biggie... you can <a href="https://static.igem.org/mediawiki/2017/9/9b/TEC-CEM-Protocol_for_biobricks.pdf">click here to
 +
                download the PDF file.</a></p> 
 +
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                <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">BSLA SiRNA confirmation protocol
 +
                <span class="caret"></span></button>
 +
                <div class="dropdown-menu">
 +
                    <h3>BSLA SiRNA confirmation protocol</h3>                   
 +
                    <ol><h4>Steps</h4>
 +
                        <li>Transform BSLA devices in HT115</li>
 +
                        <li>Culture a blue colony of HT115 with BSLA devices for 2 days in liquid medium</li>
 +
                        <li>Extract RNA (Without using RNAse)</li>
 +
                        <li>Quantify the RNA samples</li>
 +
                        <li>Prepare a hybridization buffer (30 mM Na2HPO4 pH 8, 0.3 M NaCl, 10 mM EDTA)</li>
 +
                        <li>Place 16 μL fo the hybridization buffer in a 0.6 ml microtube and then add 4 μL of oligos (100 μM)</li>
 +
                        <li>Add 2 μg of RNA sample</li>
 +
                        <li>Mix the samples with the micropipette</li>
 +
                        <li>Incubate the samples at 94°C for 5 minutes</li>
 +
                        <li>Incubate the samples at 42°C for 60 minutes</li>
 +
                        <li>Add 20 units of exonuclease 1</li>
 +
                        <li>Incubate at 37°C for 30 minutes</li>
 +
                        <li>Place the samples in ice or store they at -80°C until its use</li>
 +
                        <li>Run a non-denaturing gel</li>
 +
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                     <h3>RFP characterization curve for DH5a strain</h3>                   
 
                     <h3>RFP characterization curve for DH5a strain</h3>                   
 
                     <ol><h4>IPTG induction</h4>
 
                     <ol><h4>IPTG induction</h4>
                         <li>Prepare the seed culture d by resuspending an isolated colony of transformed Escherichia coli DH5a+BBa_J04450 in 10 mL of liquid LB broth with chloramphenicol (25μg/mL) and incubate it at 37°C overnight.
+
                         <li>Prepare the seed culture by resuspending an isolated colony of transformed Escherichia coli DH5a+BBa_J04450 in 10 mL of liquid LB broth with chloramphenicol (25μg/mL) and incubate it at 37°C overnight.
 
                         </li>  
 
                         </li>  
 
                         <li>Inoculate 100 mL of LB + CAM (25μg/mL) with 1 ml of the seed culture and incubate at 37°C and 260 RPM until the OD reaches 0.6.</li>
 
                         <li>Inoculate 100 mL of LB + CAM (25μg/mL) with 1 ml of the seed culture and incubate at 37°C and 260 RPM until the OD reaches 0.6.</li>
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                 <button class="btn btn-primary dropdown-toggle responsiveImage" type="button" data-toggle= "dropdown">Extraction of DNA from filter paper
 
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                     <h3>GENSCRIPT</h3>                                  
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                     <h3>Extraction of DNA from filter paper</h3>
 +
                    <ol><h4>Steps</h4>
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                        <li>Cut out the area of the filter with spotted cDNA (circle marked on the paper).</li>
 +
                        <li>Put the piece of paper in a sterile microtube.</li>
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                        <li>Apply 75 µl of Water Molecular Biology Grade.</li>
 +
                        <li>Vortex 30 seconds.</li>
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                        <li>Centrifuge 1 min to elute the DNA and pellet the solution and paper.</li>
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                        <li> Store the solution toghether with the filter paper at 4°C.</li>
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                        <li>Transform E. coli with 1 µl of the plasmid DNA.</li>
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                    </ol>                               
 
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                     <h3>Establishment of Diaphorina citri primary cell culture</h3>  
 
                     <h3>Establishment of Diaphorina citri primary cell culture</h3>  
 
                     <ol><h4>Steps</h4>
 
                     <ol><h4>Steps</h4>
                         <li>Collect 50 Diaphorina Citri, keep them in ice.</li>
+
                         <li>Collect 50 Diaphorina citri and keep in ice.</li>
                         <li>Pick one with sterile tweezers.</li>
+
                         <li>Pick each with sterile tweezers.</li>
                         <li>Wash in .11% sodium hypochloride for 10 seconds.</li>
+
                         <li>Wash in .11% sodium hypochlorite for 10 seconds.</li>
 
                         <li>Wash in 75% of ethanol for 30 seconds.</li>
 
                         <li>Wash in 75% of ethanol for 30 seconds.</li>
 
                         <li>Wash in sterile H20MiliQ water for 20 seconds.</li>
 
                         <li>Wash in sterile H20MiliQ water for 20 seconds.</li>
                         <li>Place the diaphorina in an sterile petri dish under a stereoscopic microscope.</li>
+
                         <li>Place on an sterile petri dish under a stereoscopic microscope.</li>
                         <li>Take the insect by the head with the tweezers then slowly remove the lower abdomen.</li>
+
                         <li>Grab the head of the insect with tweezers then slowly remove the lower abdomen. If removed slowly, green strings will appear indicating the digestive tract. In order to avoid contamination, remove completely.</li>
                        <ol>
+
                         <li>Collect the removed digestive tracts and place in a separate container.</li>
                            <li>If removed slowly the green strings will appear, this might be its stomach its colon in order to avoid contamination remove it, it is number 2 in the image.</li>
+
                         <li>Collect the head and rest of the body and place in a microtube.</li>
                        </ol>
+
                        <p>For the digestive tract:</p>
                         <li>Leave the abdomens in the petri dish, number 3 in the image.</li>
+
                         <li>Place a Corning 10 μm cell strain filter over a sterile 50 mL Falcon Tube and place the material in it.</li>
                         <li>Collect the diaphorina head and upper body in a microtube.</li>
+
                         <li>Using a 5 ml syringe plunger, grind the tissue until it is completely homogenous.</li>
                         <li>Place a Corning 10 μm cell strain filter over a sterile 50 mL Falcon Tube, place the abdomens.</li>
+
                         <li>Add 500 ul of Hank's Salt Solution.</li>
                         <li>Using a 5ml syringe plunger grind the tissue until it is completely homogenous.</li>
+
                         <li>Add 500ul of Hanks Salts.</li>
+
 
                         <li>Keep grinding the remains.</li>
 
                         <li>Keep grinding the remains.</li>
                         <li>Add another 500ul of Hanks Salts.</li>
+
                         <li>Add another 500ul of Hank's Salt Solution.</li>
                         <li>Open a second 50mL Falcon Tube and place a 40 μm Corning cell strain filter was used to filter the previous liquid.</li>
+
                         <li>In a different 50mL Falcon Tube, place a 40 μm Corning cell strain filter and filter the previously obtained solution.</li>
                         <p>*For the rest of the body:</p>
+
                        <li>Add 300 uL of Schneider's Insect medium and place on a cell culture plate.</li>
 +
                         <p>For the rest of the body:</p>
 
                         <li>Centrifuge at 250 g for 5 minutes.</li>
 
                         <li>Centrifuge at 250 g for 5 minutes.</li>
                         <li>Remove the supernatant with a micropipette and place the bodies on a 10 μm cell strain filter.</li>
+
                         <li>Remove the supernatant with a micropipette and place on a 10 μm cell strain filter.</li>
 
                         <li>Grind with a syringe plunger until homogeneous.</li>
 
                         <li>Grind with a syringe plunger until homogeneous.</li>
 
                         <li>Wash the filter with 400 uL of Hank’s Salt Solution.</li>
 
                         <li>Wash the filter with 400 uL of Hank’s Salt Solution.</li>
                         <li>Transfer the filtered liquid to a 40 μm cell strain filter and add 200 uL of Hank’s salt solution.</li>
+
                         <li>Transfer the filtered liquid to a 40 μm cell strain filter and add 200 uL of Hank’s Salt Solution.</li>
 
                         <li>Centrifuge the filtered liquid at 250 g for 10 minutes.</li>
 
                         <li>Centrifuge the filtered liquid at 250 g for 10 minutes.</li>
 
                         <li>Add the supernatant to a cell culture plate well, then resuspend the pellet in 300 uL of Schneider’s Insect medium and add to a different well.</li>
 
                         <li>Add the supernatant to a cell culture plate well, then resuspend the pellet in 300 uL of Schneider’s Insect medium and add to a different well.</li>
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            <h1 class = "titleUbuntu">Project Development</h1>
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Latest revision as of 18:05, 1 November 2017

IGEM_TECCEM

Experiments

Protocols

Experiments

IGEM_TECCEM