https://bridgeslab.sph.umich.edu/protocols/index.php?action=history&feed=atom&title=Purification_of_MBP_Fusion_ProteinsPurification of MBP Fusion Proteins - Revision history2026-05-17T05:30:31ZRevision history for this page on the wikiMediaWiki 1.45.1https://bridgeslab.sph.umich.edu/protocols/index.php?title=Purification_of_MBP_Fusion_Proteins&diff=544&oldid=prevDavebrid: wrote initial page2010-12-02T22:00:52Z<p>wrote initial page</p>
<p><b>New page</b></p><div>==Bacteria Production and Induction==<br />
*Express and induce protein in culture under appropriate conditions:<br />
#grow an overnight culture in ~25 mL LB/Amp (with Chloramphenicol if using Rosetta cells) from a colony <2 weeks post transformation.<br />
#add 5 mL overnight culture to 1L TB/Amp and grow at 37C<br />
#grow to OD600 of 0.6-1.0 and induce with 100 uM IPTG (the concentration of IPTG and duration of induction should be optimized for each protein)<br />
#let grow O/N at <25C (optimize induction time/temp for each protein, see [[Induction Conditions]]).<br />
#centrifuge cells 10 min at 9000 RPM to pellet bacteria freeze if stopping at this point.<br />
<br />
==Lysis and Purification==<br />
#Resuspend cells in ~20 mL lysis buffer (PBS + 0.1% B-ME and a PI tablet). Freeze in liquid nitrogen if not continuing with purification<br />
#French Press cells 2 x 15 000 psi (see French Press Protocol)<br />
#Centrifuge lysate at >15 000 RPM (i.e. 20,000RMP in JA25.5 at 4 degrees C) for 30 min to clarify<br />
#Add 1.0 mL amylose resin to 50 mL PBS (no PI) to prepare beads. Let sit for 30 min. to allow beads to settle or pellet beads for 5 min at 1000 RPM and remove buffer<br />
#Save a lysate sample (20 uL) and add clarified lysate to equilibrated beads<br />
#Incubate with rotation for 1h at 4C<br />
#Pellet beads (save sample of unbound protein) and wash 3 x 50 mL cold wash buffer being careful to not suck up beads<br />
#Pour into disposable column (BioRad # 732-6008) to collect beads. Wash with another 10 mL of PBS<br />
#Prepare elution buffer containing 10mM maltose in PBS(0.615g in 40mL PBS), adjust pH to between 7 and 8. <br />
#Elute with ~5 mL room temp. elution buffer, collecting 10 x ~0.5 mL fractions. Check fractions for protein with Bradford assay<br />
#Combine fractions with protein and dialyse O/N into 200 mL PBS in 50% glycerol (will concentrate sample ~4X) or other desired buffer<br />
#Measure protein concentration ([[Bradford Assay]] or [[Quantification by Absorbance at 280nm]]; concentrate if necessary and store at -20)<br />
#Analyze uninduced and induced cells (0.5 mL culture resuspended in 100 uL 2X SDS), lysate (5 uL in 2X), unbound (5 uL in 2X) and purified protein (0.5-10 ug) by SDS-PAGE<br />
[[Category:Protein Purification]]<br />
[[Category:MBP]]</div>Davebrid