IGEM:IMPERIAL/2007/Notebook/2007-8-29: Difference between revisions

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==In Vitro Testing of viability of home-made cell extract and reaction buffer together with the commercially bought cell extract and pre-incubation mix with pTet at 37<sup>o</sup>C==
==Investigate the efficiency of a 1:1 mixture of commercial and homemade extract with pTet at 37<sup>o</sup>C==
This is to test if the commmercial cell extract and pre-incubation mix, if mixed in a ratio of 1:1 with the home made cell extract and reaction buffer, will produce sufficiently satisfying results to be used for carrying out the rest of the experiments for CELL BY DATE and INFECTOR DETECTOR.  
This is to test if the commmercial cell extract and pre-incubation mix, if mixed in a ratio of 1:1 with the home made cell extract and reaction buffer, will produce sufficiently satisfying results to be used for carrying out the rest of the experiments for CELL BY DATE and INFECTOR DETECTOR.  
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Revision as of 04:10, 6 September 2007

<calendar> name=iGEM:IMPERIAL/2007/Notebook date=2007/09/24 view=threemonths format=%name/%year-%month-%day weekstart=7 </calendar>

Investigate the efficiency of a 1:1 mixture of commercial and homemade extract with pTet at 37oC

This is to test if the commmercial cell extract and pre-incubation mix, if mixed in a ratio of 1:1 with the home made cell extract and reaction buffer, will produce sufficiently satisfying results to be used for carrying out the rest of the experiments for CELL BY DATE and INFECTOR DETECTOR.

Protocol can be found here under Phase 1-In vitro testing on the experimental design page.

Results can here under Results on the experimental design page. It was observed that fluorescense did not increase after 4 hours incubation.

Construction of pT7-GFP

  1. Insert and vector digests were run in a 1% agarose gel
    • 1. 20 μl insert digest
    • 2. 10 μl uncut insert
    • 3. 3 μl vector digest
    • 4. 3 μl uncut vector
    • 5. 1 kb DNA ladder
  2. Insert band was too faint to be cut out

Protocols can be found at Electrophoresis in the general protocols page

  1. Re-digested 15 μl of insert (thrice the previous amount)

Vesicles

Formation of Vesicles

With the suspensions prepared the day before, the following steps were taken:

  • 2ml of suspension was taken to prepare an interface according to protocol.
  • 25μl of 100x diluted GFP solution was used to prepare the emulsion; stirred gently with magnetic stirrer.

5 samples prepared:

  • Sample 1: 1ml of 50ml POPC/dodecane/GFP emulsion added over interface prepared with 2ml of POPC/dodecane suspension.
  • Sample 2: 1ml of 50ml DOPC/Span-80/Mineral Oil/GFP emulsion added over interface prepared with 2ml of DOPC/dodecane suspension.
  • Sample 3: 2ml of POPC/dodecane/GFP emulsion, with no previously prepared interface.
  • Sample 4: 2ml of 40ml DOPC/Span-80/Mineral Oil/GFP emulsion, with no previously prepared interface.
  • Sample 5: 2ml of 10ml DOPC/Span-80/Mineral Oil/GFP emulsion, with no previously prepared interface.

Samples 1 and 2 were centrifuged at 120x g. Samples 3, 4, and were not centrifuged.

All samples were left overnight.

Results
No samples were observed today.

Preparations
No preparations were made today.

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