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Evaluation of recent Protein A stationary phase innovations for capture of biotherapeutics.

J Chromatogr A. 2018; 
Pabst TM, Thai J, Hunter AK.
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Proteins, Expression, Isolation and Analysis A C C EP T E D M A N U S C RIP T MabSelect SuRe MabSelect SuRe LX MabSelect SuRe pcc MabSelect PrismA Amsphere A3 AF-rProtein A HC- 650F KanCap A KCA KanCap A 3G KCA3G Eshmuno A EshA Praesto AP AP Monofinity A MonoA MabSpeed rP202 rP202 a Not disclosed by the manufacturer Cellulose Cellulose Polyvinylether Agarose Agarose polymethacrylate Kaneka Kaneka EMD Merck Purolite Genscript Mitsubishi GE Healthcare JSR Life Sciences Tosoh Biosciences polymethacrylate MSS LX PCC PrismA A3 650F Agarose polymethacrylate GE Healthcare Agarose Alkaline stabilize d Yes Yes Yes Yes Yes Yes Yes Yes Yes Yes Yes Yes (μm) 85 85 50 ~60 50 45 65-85 65-85 ~50 85 ~90 45 B (4) B (6) - a C (6) C (5) - a C (5) - a - a C (- a) Intraparticle porosity 0. Get A Quote

摘要

We describe a comprehensive evaluation of 12 Protein A stationary phases for capture of biotherapeutics. We first examine the morphological properties of the stationary phases using a variety of orthogonal techniques including electron microscopy, particle sizing, pressure-flow behavior, and isocratic pulse response. A panel of nine proteins spanning a wide range of structures and biochemical properties was then used to assess equilibrium uptake, mass transport, dynamic binding capacity, and elution pH. Process performance and product quality were also examined under realistic bioprocess conditions using clarified mammalian cell culture broth. Equilibrium isotherms were found to be highly favorable, with equili... More

關鍵詞

Affinity chromatography; Antibody; Bioprocessing; Dynamic binding capacity; Protein A
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