I have tried to purify some proteins from transient transfected mammlian cells, but I have encountered some problems, such as the lipid removal. I found it is difficult to get clear supernant without lipid, I tried ultracentrifuge, Ammonium sulphate precipitation.
The cell line I used is 293T.
Do you have some ideas to remove the lipid from the cell lysate?
Adam B Shapiro
When I used sucrose gradient ultracentrifugation to purify plasma membranes from CHO cells, the lipid always ended up floating at the very top (0% sucrose) and could be removed with a transfer pipette.
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