A Procedure for Human Pregnancy Zone Protein (and Human α2-Macroglobulin) Purification Using Hydrophobic Interaction Chromatography on Phenyl–Sepharose CL-4B Column

A Procedure for Human Pregnancy Zone Protein (and Human α2-Macroglobulin) Purification Using Hydrophobic Interaction Chromatography on Phenyl–Sepharose CL-4B Column

In the present work we describe a procedure for the purification of human pregnancy zone protein (PZP) from pooled late pregnancy plasma by using hydrophobic interaction chromatography (HIC) on a phenyl–Sepharose column. The HIC step allowed the complete isolation of haptoglobins and the partial sep...

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Bibliographic Details
Published in:Protein expression and purification Vol. 9; no. 3; pp. 399 - 406
Main Authors: Chiabrando, Gustavo, Bonacci, Gustavo, Sanchez, Cecilia, Ramos, Adrian, Zalazar, Fabian, Vides, Miguel Angel
Format: Journal Article
Language:English
Published: United States Elsevier Inc 01-04-1997
Subjects:
alpha-Macroglobulins - chemistry
alpha-Macroglobulins - isolation & purification
Chelating Agents
Chromatography, Agarose - methods
Electrophoresis, Polyacrylamide Gel
Female
Humans
Pregnancy
Pregnancy Proteins - chemistry
Pregnancy Proteins - isolation & purification
Protein Conformation
Sepharose - analogs & derivatives
Zinc
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Summary:In the present work we describe a procedure for the purification of human pregnancy zone protein (PZP) from pooled late pregnancy plasma by using hydrophobic interaction chromatography (HIC) on a phenyl–Sepharose column. The HIC step allowed the complete isolation of haptoglobins and the partial separation of human α2-macroglobulin (α2-M) from a protein fraction containing PZP previously obtained by a DEAE-Sephacel chromatography. Pure and native PZP, with a recovery of nearly 25% and biological activity of protease-binding, was obtained by two definitive final steps consisting of zinc-chelate and size-filtration chromatographies. Moreover, we further present an alternative procedure for the purification of α2-M from the same pregnancy plasma, based on the differential elution of PZP and α2-M from the HIC. This purification step gave rise to a highly purified product with a recovery of 10%. This differential elution could be explained by differences in surface hydrophobicity observed between both proteins. In addition, considering the different hydrophobic properties exhibited by native PZP and PZP–protease complexes, HIC on phenyl–Sepharose column could also be used for separating both conformational states of PZP.
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ISSN:1046-5928
1096-0279
DOI:10.1006/prep.1996.0680