Team:Liceo Eugenio Hostos/Experiments
Experiments & Protocols
Protocols
Bacterial transformation:
- place 1 ml of bacteria to ependolf tubes then put them for 5 min at 14000 to the centrifuga.
- discard liquid and leave the pellet, then we went back to step 1. Then we went back to throw the pellet. This was to get more crop.
- place 250 ul of resuspencion solution.
- place 250 ul of lisis.
- solution - place 10 ul of solution - alkaline protease, wait 5min
- place 350 ul of neutralizing solution and wait 10 min, centrifuge at 10 min and max velocidad.
- insert the sample 600 UL listed in a column and in a tube colector.
- remove lysate and reinsertamos column in the tube colector.
- centrifuge at max speed by 1 min.
- Add 750 ul of lavado.
- solution - return to step 10.
- we discard the excess and reinsertamos in the way.
- column - add 250ul solution of washing.
- centrifuge at max speed for 2 min
- transfer the column to a tube esteril.
- Add 80 ul of free water nucleasa.
- centrifuge at max speed by 1 min.
- keep the sample at - 20° C.
Purification plasmodio: