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dc.contributor.authorNielsen S.U.
dc.contributor.authorBassendine M.F.
dc.contributor.authorBurt A.D.
dc.contributor.authorMartin C.
dc.contributor.authorPumeechockchai W.
dc.contributor.authorToms G.L.
dc.date.accessioned2021-04-05T04:32:23Z-
dc.date.available2021-04-05T04:32:23Z-
dc.date.issued2006
dc.identifier.issn0022538X
dc.identifier.other2-s2.0-33144465371
dc.identifier.urihttps://ir.swu.ac.th/jspui/handle/123456789/15042-
dc.identifier.urihttps://www.scopus.com/inward/record.uri?eid=2-s2.0-33144465371&doi=10.1128%2fJVI.80.5.2418-2428.2006&partnerID=40&md5=7d51cd7781491d946f78cf9e9dac86c4
dc.description.abstractHepatitis C virus (HCV) RNA circulates in the blood of persistently infected patients in lipoviroparticles (LVPs), which are heterogeneous in density and associated with host lipoproteins and antibodies. The variability and lability of these virus-host complexes on fractionation has hindered our understanding of the structure of LVP and determination of the physicochemical properties of the HCV virion. In this study, HCV from an antibody-negative immunodeficient patient was analyzed using three fractionation techniques, NaBr gradients, isotonic iodixanol, and sucrose gradient centrifugation. Iodixanol gradients were shown to best preserve host lipoprotein-virus complexes, and all HCV RNA was found at densities below 1.13 g/ml, with the majority at low density, ≤1.08 g/ml. Immunoprecipitation with polyclonal antibodies against human ApoB and ApoE precipitated 91.8% and 95.0% of HCV with low density, respectively, suggesting that host lipoprotein is closely associated with HCV in a particle resembling VLDL. Immunoprecipitation with antibodies against glycoprotein E2 precipitated 25% of HCV with low density, providing evidence for the presence of E2 in LVPs. Treatment of serum with 0.5% deoxycholic acid in the absence of salt produced HCV with a density of 1.12 g/ml and a sedimentation coefficient of 215S. The diameters of these particles were calculated as 54 nm. Treatment of serum with 0.18% NP-40 produced HCV with a density of 1.18 g/ml, a sedimentation coefficient of 180S, and a diameter of 42 nm. Immunoprecipitation analysis showed that ApoB remained associated with HCV after treatment of serum with deoxycholic acid or NP-40, whereas ApoE was removed from HCV with these detergents. Copyright © 2006, American Society for Microbiology. All Rights Reserved.
dc.subjectapolipoprotein B
dc.subjectapolipoprotein E
dc.subjectdeoxycholic acid
dc.subjectdetergent
dc.subjectiodixanol
dc.subjectlipoprotein
dc.subjectlow density lipoprotein
dc.subjectpolyclonal antibody
dc.subjectsodium bromide
dc.subjectvery low density lipoprotein
dc.subjectvirus RNA
dc.subjectarticle
dc.subjectclinical article
dc.subjectcontrolled study
dc.subjectdensity
dc.subjectdensity gradient
dc.subjectfractionation
dc.subjecthepatitis C
dc.subjectHepatitis C virus
dc.subjecthuman
dc.subjecthuman tissue
dc.subjectimmune deficiency
dc.subjectimmunoprecipitation
dc.subjectnonhuman
dc.subjectparticle size
dc.subjectpersistent infection
dc.subjectphysical chemistry
dc.subjectpriority journal
dc.subjectsedimentation
dc.subjectserum
dc.subjectsucrose gradient
dc.subjectvirion
dc.subjectvirus cell interaction
dc.subjectvirus load
dc.subjectvirus particle
dc.subjectApolipoproteins B
dc.subjectApolipoproteins E
dc.subjectBromides
dc.subjectCentrifugation, Density Gradient
dc.subjectCommon Variable Immunodeficiency
dc.subjectDeoxycholic Acid
dc.subjectDetergents
dc.subjectHepacivirus
dc.subjectHepatitis C Antibodies
dc.subjectHumans
dc.subjectImmunoprecipitation
dc.subjectLipoproteins, VLDL
dc.subjectMacromolecular Substances
dc.subjectPolyethylene Glycols
dc.subjectRNA, Viral
dc.subjectSodium Compounds
dc.subjectSucrose
dc.subjectTriiodobenzoic Acids
dc.subjectViral Envelope Proteins
dc.subjectHepatitis C virus
dc.titleAssociation between hepatitis C virus and very-low-density lipoprotein (VLDL)/LDL analyzed in iodixanol density gradients
dc.typeArticle
dc.rights.holderScopus
dc.identifier.bibliograpycitationJournal of Virology. Vol 80, No.5 (2006), p.2418-2428
dc.identifier.doi10.1128/JVI.80.5.2418-2428.2006
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