Difference between revisions of "Team:KU Leuven/Protocols"

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                                            <li> Calcium imaging is a scientific technique which can be used to measure and follow the calcium ions inside and/or outside the cell. We used a specific dye (Fura2-AM) to follow the calcium ions by the rate of fluorescence. For our project, we only used the calcium imaging for testing whether there were oscillations or not and what potassium concentrations (in a krebs buffer) were needed. We did not mathematically analyse the data we received. We only used it as a criteria for the patch clamp.</li>
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                             <h2><b>Preparation of imaging</b></h2>
 
                             <h2><b>Preparation of imaging</b></h2>
 
                                     <h5><b>Fura-2, AM</b> (MW: 1001,9)</h5>
 
                                     <h5><b>Fura-2, AM</b> (MW: 1001,9)</h5>
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                                             <li>To load cells (1 well): add 2 μl of Fura-2 to 1 ml of medium (2μM work solution)</li>
 
                                             <li>To load cells (1 well): add 2 μl of Fura-2 to 1 ml of medium (2μM work solution)</li>
 
                                             <li>Incubate cells for 30 minutes before measurement</li>
 
                                             <li>Incubate cells for 30 minutes before measurement</li>
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Revision as of 17:59, 12 October 2017

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Protocols

In the lab, we used different experimental procedures. There are protocols for the wet and bacterial lab, for the cell culture lab and for the electrophysiology lab.

Cell Culture


Wet Lab


Patch Clamp


Calcium imaging


Intra- and extracellular buffers