Hi everybody,
I'm currently expressing proteins in and extracting from bacteria. The procedure is that I pellet the bacteria from bioreactor, resuspend in buffer (50 mM Tris/HCl, pH 8.0; 1M NaCl; 5% glycerol; 1 mM EDTA), pellet and once again.
Then I add the buffer again approx. in ratio 1:1 to the cells. And resuspend and then I lyse them with BioLogics model 3000MP ultrasonic homogenizer (with probe) with the following setting: 49 % intensity; 6 s ON; 9 s OFF for 5 minutes in total.
Because I usually have > 200 ml of the cell suspension, I lyse ~25ml at once, colled the lysed cells together and then go two more rounds; i.e. I lyse it three times, but not at once.
Then I pellet cell debris (and obviously undisrupted cells) and take away the supernatant.
The problem is, that when I resuspend these pellets again and lyse them once again (well, three times), I recover additional activity.
So my two questions are:
1) Does the cell density affect the efficiency of the cell lysis by ultrasound? If I diluted the cells more, would be the lysis more efficient?
2) is the cell lysis affected by the volume I use? I was told not to lyse more than 30 ml at once. I found an article, but there they had sonic bath and the volume was in range 100-700 ul.
Thank you