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| Line 3: |
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| | <h2>Notebook</h2> | | <h2>Notebook</h2> |
| − | | + | <p> Document the dates you worked on your project.</p> |
| − | <p><h1><strong>LB medium</strong></h1></p> | + | |
| − | <p>- Add the following components</p>
| + | |
| − | <table border="1" cellspacing="0" cellpadding="0">
| + | |
| − | <tbody>
| + | |
| − | <tr>
| + | |
| − | <td valign="top" width="109">
| + | |
| − | <p>NaCl</p>
| + | |
| − | </td>
| + | |
| − | <td valign="top" width="150">
| + | |
| − | <p>10 g</p>
| + | |
| − | </td>
| + | |
| − | </tr>
| + | |
| − | <tr>
| + | |
| − | <td valign="top" width="109">
| + | |
| − | <p>Yeast extract</p>
| + | |
| − | </td>
| + | |
| − | <td valign="top" width="150">
| + | |
| − | <p>5 g</p>
| + | |
| − | </td>
| + | |
| − | </tr>
| + | |
| − | <tr>
| + | |
| − | <td valign="top" width="109">
| + | |
| − | <p>Tryptone</p>
| + | |
| − | </td>
| + | |
| − | <td valign="top" width="150">
| + | |
| − | <p>10 g</p>
| + | |
| − | </td>
| + | |
| − | </tr>
| + | |
| − | <tr>
| + | |
| − | <td valign="top" width="109">
| + | |
| − | <p>H<sub>2</sub>O</p>
| + | |
| − | </td>
| + | |
| − | <td valign="top" width="150">
| + | |
| − | <p>Add to 1 L</p>
| + | |
| − | </td>
| + | |
| − | </tr>
| + | |
| − | </tbody>
| + | |
| − | </table>
| + | |
| − | <ul>
| + | |
| − | <li>To obtain solid media add 15g/L agar.</li>
| + | |
| − | </ul>
| + | |
| − | <p>- Autoclave at 121 <sup>o</sup>C for 20 min.</p>
| + | |
| − | <p>- The preferred antibiotic is added with the proper concentration (e.g Ampicilin is added to a final concentration of 100 µg/ml)</p>
| + | |
| − | <ul>
| + | |
| − | <li>To the liquid medium antibiotic is added upon usage.</li>
| + | |
| − | <li>For the preparation of agar plates antibiotic is added after autoclaving the media and cooling it to 60 <sup>o</sup>C. </li>
| + | |
| − | </ul>
| + | |
| − | | + | |
| − | <p> </p>
| + | |
| − | | + | |
| − | <p>
| + | |
| − | <h1><strong>Plasmid Extraction - using peqGOLD Plasmid Miniprep Kit I,
| + | |
| − | PEQLAB Technologies</strong></h1>
| + | |
| − | </p>
| + | |
| − | | + | |
| − | <p>
| + | |
| − | Select few TOP10/BL21 <em>E.coli</em> transformed colonies from the LB Amp plates containing the propagated transformed colonies and inoculate them into
| + | |
| − | liquid LB medium (5 ml) containing preferred antibiotic of desired concentration in each tube.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Incubate the LB tubes with the transformed colonies at 37ᵒC in a shaker for about 12 – 15 hours (overnight) with agitation (150 rpm).
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Extract the plasmids from the incubated LB cultures using the peqGOLD Plasmid Miniprep Kit I.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Centrifuge the culture at 10000 x g for 2 min to obtain the pellet and repeat the process until the culture is completely centrifuged. Store the pellet of
| + | |
| − | 1 ml of the culture at -20ᵒC for future use.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Resuspend the pellet in 250 µl of Solution I of the Kit (which is normally kept at 4ᵒC because of the RNase) and vortex until the pellet is resuspended.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Add 250 µl of Solution II to the resuspended mixture and gently mix by inverting and rotating the tubes 6 -10 times to obtain a cleared lysate. Incubate
| + | |
| − | the mixture for 2 min to obtain optimum results.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Add 350 µl of Solution III to the cleared lysate and gently mix by inverting the tubes 6 -10 times until a flocculent white precipitate is formed.
| + | |
| − | Centrifuge at 10000 x g for 10 min at room temperature.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Transfer the clear supernatant to a fresh PerfectBind DNA Column in a 2 ml Collection Tube. Centrifuge the Column with the Collection Tube for 1 min at
| + | |
| − | 10000 x g at room temperature. Discard the flow-through liquid.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Add 500 µl of PW Plasmid buffer to the PerfectBind DNA Column in the Collection Tube and centrifuge for 1 min at 10000 x g. Discard the flow-through.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Add 750 µl of DNA Wash buffer to the PerfectBind DNA Column in the Collection tube and centrifuge for 1 min at 10000 x g. Discard the flow-through. Repeat
| + | |
| − | this step to obtain optimum results.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Place the PerfectBind DNA Column in the Collection tube and centrifuge for 2 min at 10000 x g to dry the column matrix. This step is essential to remove
| + | |
| − | ethanol from the column.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Place the PerfectBind DNA Column into a fresh 1.5 ml Eppendorf tube. Add 50 µl of pre-warmed sterile deionized water directly to the binding matrix in the
| + | |
| − | PerfectBind DNA Column and centrifuge for 1 min at 5000 x g to elute the DNA.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Discard the PerfectBind DNA Column and store the eluted plasmid DNA at -20ᵒC.
| + | |
| − | </p>
| + | |
| − | <p>
| + | |
| − | Check the concentration of the plasmids by using a NanoDrop and note down the values for future experiments.
| + | |
| − | </p>
| + | |
| − | | + | |
| − | | + | |
| − | <p> </p>
| + | |
| − | | + | |
| − | <p>
| + | |
| − | <h1><strong>Plasmid Extraction - using QIAprep Spin Miniprep Kit (QIAGEN)</strong></h1>
| + | |
| − | </p>
| + | |
| − | | + | |
| − | <p>This protocol describes the purification of plasmid DNA from 5 ml overnight cultures of <em>E. coli</em> grown in LB medium using the QIAprep Spin Miniprep Kit. (QIAGEN).</p>
| + | |
| − | <ul>
| + | |
| − | <li>Add the provided RNase A solution to buffer P1, mix, and store at 4 <sup>o</sup>C.</li>
| + | |
| − | <li>Add ethanol (96–100%) to Buffer PE before use.</li>
| + | |
| − | <li>All centrifugation steps are carried out at 17,900 x g (13,000 rpm) in a conventional table-top microcentrifuge at room temperature.</li>
| + | |
| − | </ul>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Add the proper antibiotic with the proper concentration to 5 ml LB medium (e.g Ampicilin is added to a final concentration of 100 µg/ml).</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Inoculate the medium with the desired <em>E.coli</em> strain and incubate overnight at 37 <sup>o</sup>C with agitation (150 rpm).</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Pellet the overnight culture by centrifugation at 8000 rpm (6800xg) for 3 min at room temperature.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Resuspend pelleted bacterial cells in 250 μl Buffer P1 and transfer it to a microcentrifuge tube.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Add 250 μl Buffer P2 and mix thoroughly by inverting the tube 4–6 times. Do not allow the lysis reaction to proceed for more than 5 min.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Add 350 μl Buffer N3 and mix immediately and thoroughly by inverting the tube 4–6 times.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Centrifuge for 10 min at 13,000 rpm (~17,900 x g) in a table-top microcentrifuge.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Apply the supernatant to the QIAprep spin column by decanting. Centrifuge 60 s. Discard the flow-through.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Wash the QIAprep spin column by adding 500 μl Buffer PB and centrifuging for 60 s. Discard the flow-through.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Wash QIAprep spin column by adding 750 μl Buffer PE and centrifuging for 30–60 s.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Discard the flow-through, and centrifuge for an additional 1 min to remove residual wash buffer.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- Place each QIAquick column in a clean 1.5 ml microcentrifuge tube.</p>
| + | |
| − | <p> </p>
| + | |
| − | <p>- To elute DNA, add 50 μl water (40 – 60 <sup>o</sup>C) to the center of the QIAquick membrane, let the column stand for 1 min, and then centrifuge for 1 min.</p>
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| | <h5>What should this page have?</h5> | | <h5>What should this page have?</h5> |
| Line 167: |
Line 12: |
| | <li>Mention who participated in what task.</li> | | <li>Mention who participated in what task.</li> |
| | </ul> | | </ul> |
| − | <p> Document the dates you worked on your project.</p>
| + | |
| | | | |
| | <h4>Inspiration</h4> | | <h4>Inspiration</h4> |
Notebook
Document the dates you worked on your project.
What should this page have?
- Chronological notes of what your team is doing.
- Brief descriptions of daily important events.
- Pictures of your progress.
- Mention who participated in what task.
Inspiration
You can see what others teams have done to organize their notes: