ApoB is large protein, ~550KDa. I searched the literature and most of the published articles brifely described the prosedure of IP. They added SDS in lysis buffer and lyzed the cells overnight to dissolve ApoB. I followed these key points but got poor IP of ApoB. After centrifugation of the cell lysis, the supernatant was cloudy and I found ApoB existed in the undissolved part in the supernatant. Dose anyone have an idea to increase the solubility of large protein in cell lysis? Dose ultrasonication work?
Thomas Fungwe
See attached protocol. It worked for me well. The antibody you use has to be specific for B48 or B100, and for humans or rodents. Good luck.
Thomas
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