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

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                             <h5>Current clamp</h5>
 
                             <h5>Current clamp</h5>
 
                                         <ul>
 
                                         <ul>
                                             <li>When trying to measure an oscillation in the cell membrane, you cannot use voltage-clamp, since this technique doesn't allow the cell to change its membrane potential. We used current-clamp instead. Here, you can inject a pre-defined current into the cell which allows you to see how the membrane potential of the cell responds to the current. When a cell oscillates by itself, the membrane potential will oscillate while injecting 0 current. However, we often needed to inject a small negative current (-300pA) into a cell to elicit an oscillation in an extracellular Krebs solution.</li>  
+
                                             <li>When trying to measure an oscillation in the cell membrane, you cannot use voltage-clamp, since this technique doesn't allow the cell to change its membrane potential. We used current-clamp instead. Here, you can inject a pre-defined current into the cell which allows you to see how the membrane potential of the cell responds to the current. When a cell oscillates by itself, the membrane potential will oscillate while injecting 0 current. However, we often needed to inject a small negative current (-300pA) into a cell to elicit an oscillation in a cell with an extracellular Krebs solution.</li>  
 
                                         </ul>
 
                                         </ul>
 
                     </div>
 
                     </div>

Revision as of 13:11, 4 September 2017

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


Electrophysiology


Calcium imaging


Intra- and extracellular buffers