Biotechnology and Bioengineering, Vol.67, No.2, 206-216, 2000
Facilitated downstream processing of a histidine-tagged protein from unclarified E-coli homogenates using immobilized metal affinity expanded-bed adsorption
The facilitated downstream processing of an intracellular, polyhistidine-tagged protein, glutathione S-transferase [GST-(His)(6)], direct from unclarified E. coli homogenates using expanded beds of STREAMLINE chelating, has been investigated. A series of pilot experiments were used to develop preparative-scale separations of GST-(His)(6), initially in packed and then in expanded beds. Packed beds of Ni2+-loaded STREAMLINE chelating proved to have the highest 5% dynamic capacity for GST-(His)(6), of 357 U mL(-1) (36 mg mL(-1)). When using immobilized Cu2+ or Zn2+, metal ion transfer was observed from the iminodiacetate ligands to the high-affinity chelator, GST-(His)(6). The subsequent metal affinity precipitation of this homodimer resulted in operational problems. An equilibrium adsorption isotherm demonstrated the high affinity of GST-(His)(6) for immobilized Ni2+, with a q(m) of 695 U mL(-1) (70 mg mL(-1)) and a K-d of 0.089 U mL(-1) (0.0089 mg mL(-1)). Ni2+-loaded STREAMLINE chelating was therefore selected to purify GST-(His)(6) from unclarified E. coli homogenate, resulting in an eluted yield of 80% and a 3.34-fold purification. The high dynamic capacity in the expanded mode of 357 U mL(-1) (36 mg mL(-1)) demonstrates that this specific interaction was not affected by the presence of E. coli cell debris. (C) 2000 John Wiley & Sons, Inc.
Keywords:RECOMBINANT PROTEINS;FLUIDIZED-BED;LACTATE-DEHYDROGENASE;MONOCLONAL-ANTIBODIES;ENGINEERING PROTEINS;FUSION-PROTEIN;T4LYSOZYME;PURIFICATION;CHROMATOGRAPHY;PRECIPITATION