Anomalous protein uptake during cation exchange chromatography

Approximately one-third of all proteins reported in the literature have a pI sufficiently high to be resolved by cation-exchange chromatography. This paper reports the preparation and use of new high-performance polymeric-bonded-phase cation-exchange columns. Starting from a very stable, covalently

## Abstract A new experimental set‐up for on‐line visualization of the intra‐particle uptake kinetics during packed bed chromatography has been designed and tested. Confocal laser scanning microscopy was used to analyze the dynamics of protein adsorption to porous stationary phases. In combination

## Abstract A stable poly(2‐carboxyethyl acrylate‐__co__‐poly(ethylene glycol) diacrylate) monolith was synthesized inside a 75‐μm id capillary by direct __in situ__ photo‐initiated polymerization in a binary porogenic solvent consisting of methanol and ethyl ether. The resulting monolith was evalu

## Abstract In the current research, a series of dextran‐grafted adsorbents were prepared using sulfopropyl and 4‐(1__H__‐imidazol‐1‐yl) aniline as chromatographic ligands for ion‐exchange (IEC) and mixed‐mode chromatography (MMC) to respectively investigate the influence of dextran layer on adsorp

## Abstract Confocal laser scanning microscopy (CLSM) is a method allowing in situ visualization of protein transport in porous chromatography resins. CLSM requires labeling a protein with a fluorescent probe. Recent work has shown that conjugation of the protein with fluorescent probes can lead to