Revision as of 16:19, 17 September 2015

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Protocol Cell-free expression

How to perform a Luciferase assay

material: Luciferase Reaction Mix, Dilution Reagent, Luciferse DNA, Cell-free expression Mix
duration: Preparation 20 min + running time

To characterize a reaction, the luciferase plasmid was added to the expression mix and the expression is run using desired conditions (standard: 2 h at 37°C, no shaking). Afterwards, the reaction is stopped by putting it on ice. Inside a well of a 96-well microplate, 20 µl of the reaction are mixed with 20 µl of dilution reagent, creating a 1:2 dilution. If a 1:4 dilution is demanded, 20 µl of the first dilution are added to another 20 µl dilution reagent, otherwise they are discard-ed. 50 µl of the luciferase assay reagent is added to the reaction only seconds before the measurement is started. The microplate reader is set to perform a full spectrum emission scan (400 - 700 nm) of each well. Because of the kinetic temperature dependency of luciferase, it was minded to perform every scan at 25°C.

The Reaction Reagent tends to get contaminated so regular preparation is necessary

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-<td class="col0">TRIS-phosphate, pH 7.8 </td><td class="col1"> 25M</td>
+<td class="col0">TRIS-phosphate, pH 7.8 </td><td class="col1"> 25 M</td>
 </tr>
 <tr class="row2">
-<td class="col0"> DTT </td><td class="col1"> 2mM </td>
+<td class="col0"> DTT </td><td class="col1"> 2 mM </td>
 </tr>
 <tr class="row3">
-<td class="col0"> EDTA </td><td class="col1"> 2mM </td>
+<td class="col0"> EDTA </td><td class="col1"> 2 mM </td>
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 </tr>
 <tr class="row6">
-<td class="col0"> BSA </td><td class="col1"> 1mg/ml </td>
+<td class="col0"> BSA </td><td class="col1"> 1 mg/ml </td>
 </tr>
 </table></div>