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Preparation of a high‐performance multi‐lectin affinity chromatography (HP‐M‐LAC) adsorbent for the analysis of human plasma glycoproteins
Author(s) -
Kullolli Majlinda,
Hancock William S.,
Hincapie Marina
Publication year - 2008
Publication title -
journal of separation science
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.72
H-Index - 102
eISSN - 1615-9314
pISSN - 1615-9306
DOI - 10.1002/jssc.200800233
Subject(s) - lectin , concanavalin a , jacalin , wheat germ agglutinin , chromatography , chemistry , affinity chromatography , glycoproteomics , glycoprotein , agglutinin , high performance liquid chromatography , glycan , biochemistry , enzyme , in vitro
Abstract We report on the preparation of an improved multi‐lectin affinity support for HPLC separations. We combined the selectivity of three different lectins: concanavalin A (ConA), wheat germ agglutinin (WGA), and jacalin (JAC). Each lectin was first covalently immobilized onto a polymeric matrix and then the three lectin media were combined in equal ratios. The beads were packed into a column to produce a mixed‐bed multi‐lectin HPLC column (high‐performance multi‐lectin affinity chromatography (HP‐M‐LAC)) for fast chromatographic affinity separations. The support was characterized with respect to kinetics of immobilization, ligand density, and binding capacity for human plasma glycoproteins. A high lectin density (15 mg/mL of beads) was found to be optimal for the binding of glycoproteins from human plasma. A single clinical sample can be fractionated in less than 10 min per run, making this a useful sample preparation tool for proteomics/glycoproteomics studies associated with disease abormalities.