Transfection (nonviral)

From 2008.igem.org

PrincetonLogo.gif

PRINCETON IGEM 2008

Home Project Overview Project Details Experiments Results Notebook
Parts Submitted to the Registry Modeling The Team Gallery




Transfection Protocol

Take media off of cells

Rinse with PBS

Put 1mL trypsin on cells. Trypsin will interfere with “sticky” extracellular proteins. When cells start to detach from gelatin, add 5mL media with serum in it. The serum in the media will stop the action of the trypsin.


In multiple-well plate:

Add 1mL media to each well


Count cells with henocytometer to determine concentration of cells.


Add DNA to wells.

Add blasticidin to wells at a one in 1000 volume factor.

Add 105 cells to each well. Shake up and down, side to side

Add 3ul Superfect to each well.