Purification of a recombinant baculovirus of Autographa californica M nucleopolyhedrovirus by ion exchange membrane chromatography

dc.citation.doi10.1016/j.jviromet.2012.03.031en_US
dc.citation.epage124en_US
dc.citation.issue2en_US
dc.citation.jtitleJournal of Virological Methodsen_US
dc.citation.spage117en_US
dc.citation.volume183en_US
dc.contributor.authorGrein, Tanja A.
dc.contributor.authorMichalsky, Ronald
dc.contributor.authorLópez, Maria Vega
dc.contributor.authorCzermak, Peter
dc.contributor.authoreidpczermaken_US
dc.contributor.authoreidrm83en_US
dc.date.accessioned2012-07-05T19:15:32Z
dc.date.available2012-07-05T19:15:32Z
dc.date.issued2012-08-01
dc.date.published2012en_US
dc.description.abstractSignificant progress in the application of viral vectors for gene delivery into mammalian cells and the use of viruses as biopesticides requires downstream processing that can satisfy application-specific demands on performance. In the present work the stability and ion exchange membrane chromatography of a recombinant of Autographa californica M nucleopolyhedrovirus is studied. To adjust the degree of purification the effect of ionic conductivity or pH on the viral infectivity was assessed (0.77-78.00 mS/cm, pH 3-8). Infectivity decreased rapidly by several orders of magnitude at below 5 mS/cm (i.e., 0.49 MPa osmotic pressure change) or at below pH 5.5 (rationalized with particle aggregation). The virus was concentrated and purified via adsorption (0.2-1.1 x 10[superscript]16 pfu/m[superscript]3 chromatographic bed volume, 0.6-1.1 x 10[superscript]12 pfu/m[superscript]2 membrane area facing the incident fluid flow) and elution at pH 6.1 and 6.35 mS/cm from three strong anion exchange membranes. Virus recovery and concentration in accord with the volume reduction were obtained using a polyether sulfone-based membrane with quaternary ammonium ligands. The level of host cell protein (down to below the detection limit) and suspended DNA (below 93 pg DNA per 106 pfu) are reported for each membrane employed, for the purpose of comparability, under equal adsorption or elution conditions respectively.en_US
dc.description.versionArticle (author version)
dc.identifier.urihttp://hdl.handle.net/2097/13980
dc.relation.urihttp://doi.org/10.1016/j.jviromet.2012.03.031en_US
dc.subjectGene therapyen_US
dc.subjectPesticideen_US
dc.subjectBaculovirusen_US
dc.subjectIon exchange membrane chromatographyen_US
dc.subjectConductivityen_US
dc.subjectpHen_US
dc.titlePurification of a recombinant baculovirus of Autographa californica M nucleopolyhedrovirus by ion exchange membrane chromatographyen_US
dc.typeTexten_US

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Figure 1: Schematic setup of virus production and one-step virus concentration and purification.
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Figure 2: Infectivity of virus dispersions and absorbance at 595 nm vs. pH. A line was added to guide the eye. Error bars are one standard deviation.
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Figure 3: Infectivity (instantaneously or after 24 h storage) vs. ionic conductivity in the liquid phase. Lines were added to guide the eye. Error bars reflect the average uncertainty reported previously for the assay quantifying viral infectivity (see 2.2).
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Figure 4: Separation of AcMNPV using three different anion exchange membranes. All fractions are 1 ml. Eluate I contains 0.15 mol/l NaCl, eluate II contains 0.5 mol/l NaCl. The acronyms of the tested membrane materials are given at 2.6. Error bars are one standard deviation for samples analyzed in triplicate.

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