Team:Wageningen UR/Project/DevicesSetup
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(→Custom fluidic device designed by Team Wageningen UR to measure oscillations) |
(→Custom fluidic device designed by Team Wageningen UR to measure oscillations) |
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Because it is not necessary for our system to have a flow going over the wells we eventually only used bottom flow, as depicted in figure 5. Our resulting setup enabled us to bottom feed our bacteria, this is depicted in figure 6. This allowed the measurements to be taken continuously for various hours, as nutrients could diffuse through the bottom of the wells. Measurements were taken with the use of our LEGO robot (see [https://2011.igem.org/Team:Wageningen_UR/Project/DevicesFunFacts fun facts]). | Because it is not necessary for our system to have a flow going over the wells we eventually only used bottom flow, as depicted in figure 5. Our resulting setup enabled us to bottom feed our bacteria, this is depicted in figure 6. This allowed the measurements to be taken continuously for various hours, as nutrients could diffuse through the bottom of the wells. Measurements were taken with the use of our LEGO robot (see [https://2011.igem.org/Team:Wageningen_UR/Project/DevicesFunFacts fun facts]). | ||
- | [[File:Micro-dish2_device_WUR.png| | + | [[File:Micro-dish2_device_WUR.png|270px]] [[File:Bottom_feed_WUR.png|470px|right]] |
- | '''Fig.5 (Top)''' | + | '''Fig.5 (Top)''' ''Using microdish with bottom flow'' |
'''Fig.6 (Right)''' ''Applying bottom feeding to keep the cells in the wells alive'' | '''Fig.6 (Right)''' ''Applying bottom feeding to keep the cells in the wells alive'' | ||
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- | During our plate reader experiments we observed oscillatory behavior of transformed ''E.coli'' containing the [[Team:Wageningen_UR/Project/CompleteProject1Description# | + | During our plate reader experiments we observed oscillatory behavior of transformed ''E.coli'' containing the [[Team:Wageningen_UR/Project/CompleteProject1Description#3._Designs| streamlined construct]]. This suggested oscillations could occur even without applying any flow over the wells. Letting the [[Team:Wageningen_UR/Project/ModelingProj1#Writing_a_modeling_tool_in_Matlab| modeling tool]] iterate over a range of cell densities while keeping the flow rate constant at 0 confirmed that [[Team:Wageningen_UR/Project/ModelingProj1#Preliminary_conclusions_for_our_system| oscillations could occur]] at high cell densities. Therefore the measurements were taken without applying any flow. |
[[File:Measuring_GFP_WUR.jpg|500px|center]] | [[File:Measuring_GFP_WUR.jpg|500px|center]] | ||
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For the experiments, an overnight culture of the cells containing our construct was spun down and resuspended in PBS. The resuspended culture was inoculated in the device and left in the chamber to settle down for a while. Since the bacteria were bottom fed with LB as seen in the setup section in [[Team:Wageningen_UR/Project/DevicesSetup#Controlling_cell_growth| figure 6]], only the bacteria which settled down in the wells survived, while the bacteria in PBS starved to death. This is shown in the short video below. The pictures were taken every ten minutes. | For the experiments, an overnight culture of the cells containing our construct was spun down and resuspended in PBS. The resuspended culture was inoculated in the device and left in the chamber to settle down for a while. Since the bacteria were bottom fed with LB as seen in the setup section in [[Team:Wageningen_UR/Project/DevicesSetup#Controlling_cell_growth| figure 6]], only the bacteria which settled down in the wells survived, while the bacteria in PBS starved to death. This is shown in the short video below. The pictures were taken every ten minutes. | ||
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- | '''Fig. | + | '''Fig.9''' ''Microdish with ptetGFP inoculum in PBS (left) and cells in wells after removal of the PBS (right)'' |
- | For the experiment depicted above, the PBS was removed before all the cells died. The procedure varied depending on how well the bacteria settled down in the wells. They were left to grow in the device for an additional night and the measurements were then taken in a 10 minute interval during the next day. This was done for two reasons: for one the chamber had to be completely dried out before measurements could be taken, otherwise the remaining liquid would condense through the heat of the light and blur the pictures. The second reason was that - as mentioned before - [[Team:Wageningen_UR/Project/ModelingProj1# | + | For the experiment depicted above, the PBS was removed before all the cells died. The procedure varied depending on how well the bacteria settled down in the wells. They were left to grow in the device for an additional night and the measurements were then taken in a 10 minute interval during the next day. This was done for two reasons: for one the chamber had to be completely dried out before measurements could be taken, otherwise the remaining liquid would condense through the heat of the light and blur the pictures. The second reason was that - as mentioned before - [[Team:Wageningen_UR/Project/ModelingProj1#Preliminary_conclusions_for_our_system| our modeling]] suggested that - when applying no flow - the oscillations would only occur when starting with a high cell density. |
Latest revision as of 02:15, 22 September 2011