Hi
I need to lyse THP1 monocytes and then use western blotting to quantify the levels of certain proteins in the lysate. I tried lysing the cells with RIPA buffer, but the high detergent concentration was incompatable with running a gel. I then tried Lamberts Break buffer, but the total protein concentration of my lysare was extremely low (i.e. the cells didnt lyse).
Does anyone have any suggestions ass to how I can successfully lyse THP1s in a buffer that is compatable with SDS PAGE??
Thank you in advance!!
0
1 reply to this topic
#2
-
- Active Members
-
- 117 posts
Veteran
Posted 01 September 2011 - 06:26 AM
I dont think RIPA would interfere your gel run!! post your RIPA composition and also tell how it interferes in the running of lysate...
I dont know manythings, but i know what i should know!!
