Difference between revisions of "Team:Uppsala/Experiments"
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<h2 class="text"> Experimental Procedures</h2> | <h2 class="text"> Experimental Procedures</h2> | ||
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<li><a href="#intro"> Introduction </a></li> | <li><a href="#intro"> Introduction </a></li> | ||
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| − | + | <h3 id="microfluidics">Microfluidics</h3> | |
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<h4>Transformation on chip:</h4> | <h4>Transformation on chip:</h4> | ||
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<li>Flush the cell channel with 2 mL of 75% ethanol with a syringe. Dry the cell channel with air. This cleaning step should be repeated after each transformation to avoid contamination. </li> | <li>Flush the cell channel with 2 mL of 75% ethanol with a syringe. Dry the cell channel with air. This cleaning step should be repeated after each transformation to avoid contamination. </li> | ||
Revision as of 13:54, 16 October 2016
Experimental Procedures
Microfluidics
Transformation on chip:
Preparing for cell transformation
- Set up chip by connecting 0.583mm tubes insulated with paper towels to the heat channels. Use bent metal connectors. Connect tubes to two peristaltic pumps; one for each heating channel. Place a syringe needle in the inlet of the transformation channel and a tube in its outlet. (See image of setup)
- Heat the chip by running water at 65°C and 300mL h-1 through the heating channels.
- Take out 50µL of CaCl2 competent cells from -80°C freezer and thaw them on ice for 5 min.
- Take 10µL of competent cells into a separate tube for negative control.
- Add 0.8µL of DNA (at a concentration of approximately 70 ng µL-1 ) to the remaining 40µL of cells. Incubate cell and DNA suspension for 20 min on ice.
- Flush the cell channel with 2 mL of 75% ethanol with a syringe. Dry the cell channel with air. This cleaning step should be repeated after each transformation to avoid contamination.
- For each transformation: pipette 6µL of cell and DNA suspension into the syringe connector on the chip.
- Push the suspension into the transformation channel by pushing air in with a syringe.
- Fill the transformation channel and heat shock the suspension for 45 sec.
- Push the cell suspension through and collect in an Eppendorf tube filled with 100µL SOB.
- Place the tube on ice immediately.
- Incubate for 1.5 h at 37°C and then spread on an agar plate with the appropriate antibiotic.
General procedures
