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lostandconfused

Member Since 16 Jul 2012
Offline Last Active Jul 17 2012 08:58 AM
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Protein Concentration from Bacterial Lysates: Help!

16 July 2012 - 07:20 AM

I hope I'm posting this in the correct section. I am a masters student in a new lab (i.e. the first student) in a new lab where the PI shows little interest in my project other than getting it done as soon as possible. I've run SDS-Page bacterial lysates that I've made using the following protocol:
  • Grow bacteria ~18 hours on LB plates, grow @ 37C
  • The next day, add 1x PBS to the LB plates and mix with the bacteria to make a bacterial solution.
  • Dilute the bacterial solution with 1xPBS to get 1 mL of bacterial suspensions with an OD600 ~ 0.5 and 0.35.
  • Take 1 mL suspensions and centrifuge for 10K RPM for 5 minutes.
  • Remove the 1xPBS and leave the pellet
  • Add 200 uL of Sample buffer and Lysis buffer each (total of 400 uL) vortex well.
  • Take the new solution and boil for 10 minutes and store at 4C
  • Load 35 uL of this solution into 12% SDS-Page Gels of 1.5mm thickness.
These were the protocols outlined with little rhyme or reason and I followed them, but I would get fairly good bands when doing my SDS-Page and Western blots. After challenged with antibody, I wanted to identify certain proteins from my western blots (run with nitrocellulose), but I am not sure which step I would go about doing a Bradford or BCA assay to identify how much initial protein concentration I've been using. Any help would be greatly appreciated.

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