Difference between revisions of "Team:Exeter/Interlab"

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<p id="pp"> Part two of the InterLab study was started on the 31/8. Overnight cultures were grown from glycerol stocks inside a 15ml falcon tube with 5ml of LB media and 5μl of chloramphenicol. </p>
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<p id="pp"> Part two of the InterLab study was started on the 31/8.Overnight cultures of the devices and controls were grown from glycerol stocks inside a 15ml falcon tube with 5ml of LB media and 5μl of chloramphenicol.</p>
  
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<p id="pp">An initial OD600 reading was taken using a cuvette reader. Inoculation calculations were then carried out and the cultures of the constructs were grown in new 15ml falcon tubes with 5ml of fresh LB and 5μl of chloramphenicol from a starting OD of 0.02 for 6 hours in a 37°C incubator.</p>
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<p id="pp">The measurements for fluorescence were taken using a BD FACSAria II and the calibration as well as measurement protocols were followed according to the 2016 InterLab Worksheet for Flow Cytometry that is available on the iGEM website. Adjustments were made to the side-scatter and forward scatter PMT voltages using negative control bacteria to centre the distribution, adjustments to FITC/GFP PMT voltage were made  using the positive control bacteria to align bell curve an order of magnitude below the upper end of the scale. 1,000 events were acquired from calibration beads and from each biological sample.</p>
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<p id="pp">An initial OD reading was taken using a cuvette reader. Inoculation calculations were then carried out and the cultures of the constructs were grown in new 15ml falcon tubes with 5ml of fresh LB and 5μl of chloramphenicol from a starting OD of 0.02 for 6 hours in a 37°C incubator. </p>
 
<p id="pp">An initial OD reading was taken using a cuvette reader. Inoculation calculations were then carried out and the cultures of the constructs were grown in new 15ml falcon tubes with 5ml of fresh LB and 5μl of chloramphenicol from a starting OD of 0.02 for 6 hours in a 37°C incubator. </p>
  

Revision as of 14:25, 19 October 2016