Literature DB >> 21751387

Porcine parvovirus removal using trimer and biased hexamer peptides.

Caryn L Heldt1, Patrick V Gurgel, Lee-Ann Jaykus, Ruben G Carbonell.   

Abstract

Assuring the microbiological safety of biological therapeutics remains an important concern. Our group has recently reported small trimeric peptides that have the ability to bind and remove a model nonenveloped virus, porcine parvovirus (PPV), from complex solutions containing human blood plasma. In an effort to improve the removal efficiency of these small peptides, we created a biased library of hexamer peptides that contains two previously reported trimeric peptides designated WRW and KYY. This library was screened and several hexamer peptides were discovered that also removed PPV from solution, but there was no marked improvement in removal efficiency when compared to the trimeric peptides. Based on simulated docking experiments, it appeared that hexamer peptide binding is dictated more by secondary structure, whereas the binding of trimeric peptides is dominated by charge and hydrophobicity. This study demonstrates that trimeric and hexameric peptides may have different, matrix-specific roles to play in virus removal applications. In general, the hexamer ligand may perform better for binding of specific viruses, whereas the trimer ligand may have more broadly reactive virus-binding properties.
Copyright © 2012 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.

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Year:  2011        PMID: 21751387      PMCID: PMC4083586          DOI: 10.1002/biot.201000397

Source DB:  PubMed          Journal:  Biotechnol J        ISSN: 1860-6768            Impact factor:   4.677


  18 in total

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4.  The structure of porcine parvovirus: comparison with related viruses.

Authors:  Alan A Simpson; Benoît Hébert; Gail M Sullivan; Colin R Parrish; Zoltán Zádori; Peter Tijssen; Michael G Rossmann
Journal:  J Mol Biol       Date:  2002-02-01       Impact factor: 5.469

5.  Experimental and theoretical investigation of effect of spacer arm and support matrix of synthetic affinity chromatographic materials for the purification of monoclonal antibodies.

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6.  Properties of a new intravenous immunoglobulin (IGIV-C, 10%) produced by virus inactivation with caprylate and column chromatography.

Authors:  W Lebing; K M Remington; C Schreiner; H-I Paul
Journal:  Vox Sang       Date:  2003-04       Impact factor: 2.144

7.  Equilibrium adsorption of LDL and gold immunoconjugates to affinity membranes containing PEG spacers.

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Journal:  Biomaterials       Date:  2000-01       Impact factor: 12.479

8.  Normal-flow virus filtration: detection and assessment of the endpoint in bio-processing.

Authors:  Glen Bolton; Mark Cabatingan; Mike Rubino; Scott Lute; Kurt Brorson; Mark Bailey
Journal:  Biotechnol Appl Biochem       Date:  2005-10       Impact factor: 2.431

9.  Generic/matrix evaluation of SV40 clearance by anion exchange chromatography in flow-through mode.

Authors:  Sherrie Curtis; Kitty Lee; Gregory S Blank; Kurt Brorson; Yuan Xu
Journal:  Biotechnol Bioeng       Date:  2003-10-20       Impact factor: 4.530

10.  A colorimetric assay for viral agents that produce cytopathic effects.

Authors:  Caryn L Heldt; Raquel Hernandez; Usharani Mudiganti; Patrick V Gurgel; Dennis T Brown; Ruben G Carbonell
Journal:  J Virol Methods       Date:  2006-03-06       Impact factor: 2.014

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