Team:EPF-Lausanne/Notebook/19 July 2012

From 2012.igem.org

Revision as of 21:47, 19 July 2012 by Mcheraka (Talk | contribs)

Contents

Morning: Cell counting and sampling

Cell counting Given our cell density we used a 12x dilution (table). We transfered 6 samples of cells into a 96 well plate, added Trypan blue and analysed each sample with Countess.

[table with results] Western Blot sampling

Protocol (add to separate page):

  1. Centrifugation of the cell samples at 2500xg for 10min. Discard the supernatant (vacuum).
  2. Washing: Resuspend the pellet in PBS1x, centrifuge at 2500xg for 10min, discard supernatant.
  3. Add at least 1mL PER-M Reagent for 100mg (~100µl) of cell pellet. Pipette up and down to suspend.
  4. Shake gently for 10min.
  5. Remove cell bedris by centrifugation: ~1400xg for 15min
  6. Transfer the supernatant into new tubes for analysis or storage.
  • Samples where taken from odd numbered tubes : 1,3,5,7.
  • We used 300µl of M-PER Reagent based on the size of our pellets.
  • Maximum centrifugation was 10'600xg.


Protocol: None

Forgot to insert protocol.


Comments

For samples 3 and 5 we had to repeat step 5 (centrifugation to remove cell debris) because the cell pellet got aspired in the pipette while trying to transfer the supernantant into fresh tubes.

Afternoon: Cell lysates

Protocol: None

Forgot to insert protocol.


Comments
Retrieved from "http://2012.igem.org/Team:EPF-Lausanne/Notebook/19_July_2012"