Hydrophobic interaction chromatography for purification of monoPEGylated RNase A
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2012-06-15Metadata
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Mayolo-Deloisa, Karla
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Hydrophobic interaction chromatography for purification of monoPEGylated RNase A
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Abstract
The chromatographic methods used for the purification of PEGylated proteins are mainly Size Exclusion
(SEC) and Ion Exchange Chromatography (IEX). Although the PEGylation affects the protein hydrophobicity,
Hydrophobic Interaction Chromatography (HIC) has not been extensively applied for the separation of
these proteins. Purification of monoPEGylated Ribonuclease A (RNase A) using HIC is studied in this work.
The products of the PEGylation reaction of RNase A with 20 kDa methoxy-poly(ethylene glycol) were separated
using three resins with different degrees of hydrophobicity: Butyl, Octyl and Phenyl sepharose.
The effects of resin type, concentration and salt type (ammonium sulphate or sodium chloride), and gradient
length on the separation performance were evaluated. Yield and purity were calculated using the
plate model. Under all conditions assayed the native protein was completely separated from PEGylated
species. The best conditions for the purification of monoPEGylated RNase A were: Butyl sepharose, 1 M
ammonium sulphate and 35 column volumes (CVs); this resulted in a yield as high as 85% with a purity
of 97%. The purity of monoPEGylated RNase A is comparable to that obtained when the separation is performed
using SEC, but the yield increases from 65% with SEC to ∼85% with HIC. This process represents
a viable alternative for the separation of PEGylated proteins.
General note
Artículo de publicación ISI
Patrocinador
financial support of Tecnológico
de Monterrey, Bioprocess research chair (Grant CAT161)
and CONACyT (Grant 53654). Karla Mayolo-Deloisa thanks CONACyT
for the Joint Fellowship 27470 (Beca-Mixta 2010).
Identifier
URI: https://repositorio.uchile.cl/handle/2250/126133
DOI: DOI: 10.1016/j.chroma.2012.03.079
ISSN: 0021-9673
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Journal of Chromatography A, 1242 (2012) 11– 16
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