Impact of asymmetrical flow field-flow fractionation on protein aggregates stability

Carmen R M Bria; S Kim Ratanathanawongs Williams

doi:10.1016/j.chroma.2016.08.037

Impact of asymmetrical flow field-flow fractionation on protein aggregates stability

J Chromatogr A. 2016 Sep 23:1465:155-64. doi: 10.1016/j.chroma.2016.08.037. Epub 2016 Aug 16.

Authors

Carmen R M Bria¹, S Kim Ratanathanawongs Williams²

Affiliations

¹ Laboratory for Advanced Separations Technologies, Department of Chemistry, Colorado School of Mines, Golden, CO 80401, USA.
² Laboratory for Advanced Separations Technologies, Department of Chemistry, Colorado School of Mines, Golden, CO 80401, USA. Electronic address: krwillia@mines.edu.

PMID: 27575921
DOI: 10.1016/j.chroma.2016.08.037

Abstract

The impact of asymmetrical flow field-flow fractionation (AF4) on protein aggregate species is investigated with the aid of multiangle light scattering (MALS) and dynamic light scattering (DLS). The experimental parameters probed in this study include aggregate stability in different carrier liquids, shear stress (related to sample injection), sample concentration (during AF4 focusing), and sample dilution (during separation). Two anti-streptavidin (anti-SA) IgG1 samples composed of low and high molar mass (M) aggregates are subjected to different AF4 conditions. Aggregates suspended and separated in phosphate buffer are observed to dissociate almost entirely to monomer. However, aggregates in citric acid buffer are partially stable with dissociation to 25% and 5% monomer for the low and high M samples, respectively. These results demonstrate that different carrier liquids change the aggregate stability and low M aggregates can behave differently than their larger counterparts. Increasing the duration of the AF4 focusing step showed no significant changes in the percent monomer, percent aggregates, or the average Ms in either sample. Syringe-induced shear related to sample injection resulted in an increase in hydrodynamic diameter (dh) as measured by batch mode DLS. Finally, calculations showed that dilution during AF4 separation is significantly lower than in size exclusion chromatography with dilution occurring mainly at the AF4 channel outlet and not during the separation. This has important ramifications when analyzing aggregates that rapidly dissociate (<∼2s) upon dilution as the size calculated by AF4 theory may be more accurate than that measured by online DLS. Experimentally, the dhs determined by online DLS generally agreed with AF4 theory except for the more well retained larger aggregates for which DLS showed smaller sizes. These results highlight the importance of using AF4 retention theory to understand the impacts of dilution on analytes.

Keywords: Field-Flow fractionation; Focusing; Light scattering; Protein aggregates stability; Sample dilution; Shear stress.

MeSH terms

Chromatography, Gel
Dynamic Light Scattering
Fractionation, Field Flow*
Immunoglobulin G / chemistry*
Immunoglobulin G / isolation & purification
Protein Aggregates / physiology*
Protein Stability
Shear Strength

Substances

Immunoglobulin G
Protein Aggregates