| Literature DB >> 30618334 |
Gunasekaran Dhandapani1, Assaf Howard1, Thien Van Truong1, Thekke V Baiju2, Ellina Kesselman3, Noga Friedman4, Ellen Wachtel4, Mordechai Sheves4, Dganit Danino3, Irishi N N Namboothiri2, Guy Patchornik1.
Abstract
We introduce a new concept and potentially general platform for antibody (Ab) purification that does not rely on chromatography or specific ligands (e.g., Protein A); rather, it makes use of detergent aggregates capable of efficiently capturing Ab while rejecting hydrophilic impurities. Captured Ab are then extracted from the aggregates in pure form without co-extraction of hydrophobic impurities or aggregate dissolution. The aggregates studied consist of conjugated "Engineered-micelles" built from the nonionic detergent, Tween-20; bathophenanthroline, a hydrophobic metal chelator, and Fe2+ions. When tested in serum-free media with or without bovine serum albumin as additive, human or mouse IgGs were recovered with good overall yields (70-80%, by densitometry). Extraction of IgGs with 7 different buffers at pH 3.8 sheds light on possible interactions between captured Ab and their surrounding detergent matrix that lead to purity very similar to that obtained via Protein A or Protein G resins. Extracted Ab preserve their secondary structure, specificity and monomeric character as determined by circular dichroism, enzyme-linked immunosorbent assay and dynamic light scattering, respectively.Entities:
Keywords: Antibody purification; Chromatography; IgG; Protein A; Protein G
Mesh:
Substances:
Year: 2019 PMID: 30618334 PMCID: PMC6512930 DOI: 10.1080/19420862.2019.1565749
Source DB: PubMed Journal: MAbs ISSN: 1942-0862 Impact factor: 5.857