Team:Calgary/Notebook/Protocols/decatecholization
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- | <h2>GC | + | <h2>GC-MS Catechol Assay</h2> |
- | In order to identify if the PetroBrick or <i>Micrococcus</i> was capable of further reducing catechol products, GC | + | In order to identify if the PetroBrick or <i>Micrococcus</i> was capable of further reducing catechol products, GC-MS was used. |
<ol> | <ol> | ||
<li>Grow overnight cultures of the PetroBrick in LB at 37<sup>o</sup>C and <i>xylE</i> construct, or <i>Microccus</i> in yeast tryptone broth at 26<sup>o</sup>C. | <li>Grow overnight cultures of the PetroBrick in LB at 37<sup>o</sup>C and <i>xylE</i> construct, or <i>Microccus</i> in yeast tryptone broth at 26<sup>o</sup>C. |
Revision as of 02:10, 4 October 2012
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Catechol Assay in E. coli Cells
This assay is used to verify that catechol 2,3-dioxygenase (XylE) is converting catechol to the yellow compound 2-hydroxymuconic semialdehyde (2-HMS). For this procedure we used to the newly constructed XylE part. This part contains the TetR promoter the XylE gene and its native rbs site:
- Grow up 2 ml overnight cultures in LB.
- Spin the cultures down and keep the supernatant.
- Bring the supernatant to a concentration of 0.1 M of Catechol by using a 1M catechol stock solution.
- The colour of the supernatant should change to bright yellow very quickly (in about 30 seconds).
GC-MS Catechol Assay
In order to identify if the PetroBrick or Micrococcus was capable of further reducing catechol products, GC-MS was used.- Grow overnight cultures of the PetroBrick in LB at 37oC and xylE construct, or Microccus in yeast tryptone broth at 26oC.
- Subculture into the micrococcus or PetroBrick broth respectively and set up cultures with and without xylE as well as the appropriate control.
- Note: Prior to mixing, xylE and PetroBrick cultures were spun down at 4000 RPM for 5 min at room temperature and washed with 2x volume LB, spun down again, and then resuspended to the original volume to remove antibiotics which they were initially cultured in.
- Add 10 mM catechol to each tube, mix well, and cover in tin foil.
- Culture the cells at the appropriate temperature for 72 hours.
- Sonicate samples for 1 min using a Misonix Cell Disrupter set to Dial 11.
- Add 5 mL of ethyl acetate, shake well, and spin down at 4000 RPM for 5 min. at 4oC.
- Add 1mL of the ethyl acetate to a tube and reduce the volume to 0.3mL through heating.
- Samples were dried using sodium sulfate if any water layer was present and modified using trimethyl sylyl reagent.
- Samples were ran onto the GC-MS (see protocol)