Team:Groningen/protocols/Transformation EC

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Latest revision as of 15:11, 27 September 2013

E. coli transformation protocol

Materials:

LB plates with selection markers (antibiotics, inducers,…)
LB broth
Eppendorf tubes (preferably 2 ml)
Spreaders
DNA to be transformed

Reaction procedure:

Prepare plates with the correct antibiotic selection marker.
Prechill the eppendorf tubes on ice.
Remove a tube of frozen competent E. coli (DH5α) cells from the storage (-80°C freezer) and thaw it on ice (about 5 minutes). Mix the cells by gently flicking the tube. Avoid excessive pipetting, as the competent cells are extremely fragile.
Carefully transfer 50 μl of cells into each tube prepared in Step 2.
Add 10 μl ligation reaction to the competent cells.
Gently flick the tubes to mix and place them on ice for 30 minutes.
Heat-shock the cells for 60 seconds in a water bath at 42°C (do not shake and make sure the content of the tube is all at the bottom).
Immediately return the tubes to ice for 2 minutes.
Add 1 ml LB broth (RT) to the reaction mixture.
Incubate at 37°C for 1 hour with shaking (~150 rpm).
Centrifuge the tubes at 14000 rpm for 1 min.
Empty the tube until about 200 μl supernatant is left.
Resuspend the pellet in the supernatant.
Plate 200 μl of each transformation culture on LB agar plates with the correct resistant marker.
Incubate the plates overnight (16–24 hours) at 37°C.
Afterwards the plates can be stored at 4°C.

@@ Line 22: / Line 22: @@
 <div class="mainContent">
-<h2>E. Coli transformation protocol</h2>
+<h2><i>E. coli</i> transformation protocol</h2>
-<h3>Materials:</h3>
+<h5>Materials:</h5>
 <ul type="square">
 <li>LB plates with selection markers (antibiotics, inducers,…)</li>
@@ Line 32: / Line 32: @@
 </ul>
-<h3>Steps:</h3>
+<p>
+<h5>Reaction procedure:</h5>
 <ol>
 <li>Prepare plates with the correct antibiotic selection marker.</li>
 <li>Prechill the eppendorf tubes on ice.</li>
-<li>Add 10μl ligation reaction to a sterile tube.</li>
+<li>Remove a tube of frozen competent <i>E. coli </i>(DH5&#945;) cells from the storage (-80°C freezer) and thaw it on ice (about 5 minutes). Mix the cells by gently flicking the tube. Avoid excessive pipetting, as the competent cells are extremely fragile.</li>
-<li>Remove a tube of frozen competent cells from the storage (-80°C freezer) and thaw it on ice (about 5 minutes). Mix the cells by gently flicking the tube. Avoid excessive pipetting, as the competent cells are extremely fragile.</li>
+<li>Carefully transfer 50 μl of cells into each tube prepared in Step 2.</li>
-<li>Carefully transfer 50μl of cells into each tube prepared in Step 2.</li>
+<li>Add 10 μl ligation reaction to the competent cells.</li>
-<li>Add 10μl ligation reaction to the competent cells.</li>
 <li>Gently flick the tubes to mix and place them on ice for 30 minutes.</li>
 <li>Heat-shock the cells for 60 seconds in a water bath at 42°C (do not shake and make sure the content of the tube is all at the bottom).</li>
 <li>Immediately return the tubes to ice for 2 minutes.</li>
-<li>Add 1ml LB broth (RT) to the reaction mixture.</li>
+<li>Add 1 ml LB broth (RT) to the reaction mixture.</li>
-<li>Incubate for at 37°C 1 hour with shaking (~150rpm).</li>
+<li>Incubate at 37°C for 1 hour with shaking (~150 rpm).</li>
-<li>Centrifuge the tubes at 14000 rpm for 1min.</li>
+<li>Centrifuge the tubes at 14000 rpm for 1 min.</li>
-<li>Empty the tube until about 200μl supernatant is left.</li>
+<li>Empty the tube until about 200 μl supernatant is left.</li>
 <li>Resuspend the pellet in the supernatant.</li>
-<li>Plate 200μl of each transformation culture on LB agar plates with an ampicillin resistant marker.</li>
+<li>Plate 200 μl of each transformation culture on LB agar plates with the correct resistant marker.</li>
 <li>Incubate the plates overnight (16–24 hours) at 37°C.</li>
-<li>Afterwards plates can be stored at 4°C.</li>
+<li>Afterwards the plates can be stored at 4°C.</li>
 </ol>