Difference between revisions of "Team:UPMC-Paris/Experiments"
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<div align="center" style="margin: 10px 0px 10px; border:10px groove black;" onClick="ShowHide(compet)"><h3>Competent Cells</h3></div> | <div align="center" style="margin: 10px 0px 10px; border:10px groove black;" onClick="ShowHide(compet)"><h3>Competent Cells</h3></div> | ||
<div id="compet" style="display: none;"> | <div id="compet" style="display: none;"> | ||
| − | < | + | <h3>Preparation of Bacillus subtilis competent cells</h3> |
<ol><li>Streak out the strain to be made competent on an LB agar plate as a large patch and incubate overnight at 30°C</li> | <ol><li>Streak out the strain to be made competent on an LB agar plate as a large patch and incubate overnight at 30°C</li> | ||
<li>The following morning scrape the cell growth off the plate and use to inoculate fresh, pre-warmed, SpC medium (20 ml) to give an OD600 reading of about 0.5. </li> | <li>The following morning scrape the cell growth off the plate and use to inoculate fresh, pre-warmed, SpC medium (20 ml) to give an OD600 reading of about 0.5. </li> | ||
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<div align="center" style="margin: 10px 0px 10px; border:10px groove black;" onClick="ShowHide(cellprep)"><h3> Transformation</h3></div> | <div align="center" style="margin: 10px 0px 10px; border:10px groove black;" onClick="ShowHide(cellprep)"><h3> Transformation</h3></div> | ||
<div id="cellprep" style="display: none;"> | <div id="cellprep" style="display: none;"> | ||
| − | < | + | <h3>Cells Preparation :</h3> |
<ol><li>Thaw competent cells rapidly by immersing frozen tubes in a 37°C water bath</li> | <ol><li>Thaw competent cells rapidly by immersing frozen tubes in a 37°C water bath</li> | ||
<li>Immediately, add one volume of SpII + EGTA to the Thawed cells; mix gently </li> | <li>Immediately, add one volume of SpII + EGTA to the Thawed cells; mix gently </li> | ||
<li>In a sterile test tube add competent cell (0.2~0.5 ml) to the DNA solution (<0.1 ml) and incubate in a roller drum at 37.</li> | <li>In a sterile test tube add competent cell (0.2~0.5 ml) to the DNA solution (<0.1 ml) and incubate in a roller drum at 37.</li> | ||
| − | <li>Dilute the transformed cells as appropriate in T base containing 0.5% glucose and plate immediately onto selective media. </li | + | <li>Dilute the transformed cells as appropriate in T base containing 0.5% glucose and plate immediately onto selective media. </li> |
| − | + | <img src="https://static.igem.org/mediawiki/igem.org/d/d3/Transfo_pic_1.png" width="400px"/> | |
| − | < | + | <h3>Digestion :</h3> |
| − | + | <li>Select restriction enzymes to digest your plasmid. Determine an appropriate reaction buffer by reading the instructions for your enzyme. </li> | |
<p>In a 1.5mL tube combine the following:</p> | <p>In a 1.5mL tube combine the following:</p> | ||
<li>DNA </li> | <li>DNA </li> | ||
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<li>Incubate tube at appropriate temperature (usually 37°C) for 1 hour. </li> | <li>Incubate tube at appropriate temperature (usually 37°C) for 1 hour. </li> | ||
<li>Always follow the manufacturer’s instructions. </li> | <li>Always follow the manufacturer’s instructions. </li> | ||
| − | <li>To visualize the results of your digest, conduct gel electrophoresis</li | + | <li>To visualize the results of your digest, conduct gel electrophoresis</li> |
<h3>Vector Preparation :</h3> | <h3>Vector Preparation :</h3> | ||
<p>Combine the following in a PCR or Eppendorf tube:</p> | <p>Combine the following in a PCR or Eppendorf tube:</p> | ||
| − | + | <li>25ng Vector DNA</li> | |
<li>75ng Insert DNA</li> | <li>75ng Insert DNA</li> | ||
<li>Ligase Buffer (1μL/10μL reaction for 10X buffer, and 2μL/10μL reaction for 5X buffer)</li> | <li>Ligase Buffer (1μL/10μL reaction for 10X buffer, and 2μL/10μL reaction for 5X buffer)</li> | ||
Revision as of 12:06, 14 October 2016
