Utilization of cellulose microcapillary tubes as a model system for culturing and viral infection of mammalian cells

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dc.contributor.author Venter, Eudri
dc.contributor.author Van der Merwe, Christiaan F.
dc.contributor.author Van Staden, Vida
dc.date.accessioned 2012-12-12T10:17:12Z
dc.date.available 2012-12-12T10:17:12Z
dc.date.issued 2012-10
dc.description.abstract Cryofixation by high-pressure freezing (HPF) and freeze substitution (FS) gives excellent preservation of intracellular membranous structures, ideal for ultrastructural investigations of virus infected cells. Conventional sample preparation methods of tissue cultured cells can however disrupt the association between neighbouring cells or of viruses with the plasma membrane, which impacts upon the effectiveness whereby virus release from cells can be studied. We established a system for virus infection and transmission electron microscopy preparation of mammalian cells that allowed optimal visualisation of membrane release events. African horse sickness virus (AHSV) is a non-enveloped virus that employs two different release mechanisms from mammalian cells, i.e. lytic release through a disrupted plasma membrane and a non-lytic buddingtype release. Cellulose microcapillary tubes were used as support layer for culturing Vero cells. The cells grew to a confluent monolayer along the inside of the tubes and could readily be infected with AHSV. Sections of the microcapillary tubes proved easy to manipulate during the HPF procedure, showed no distortion or compression, and yielded well preserved cells in their native state. There was ample cell surface area available for visualisation, which allowed detection of both types of virus release at the plasma membrane at a significantly higher frequency than when utilising other methods. The consecutive culturing, virus infection and processing of cells within microcapillary tubes therefore represent a novel model system for monitoring intracellular virus life cycle and membrane release events, specifically suited to viruses that do not grow to high titres in tissue culture. en_US
dc.description.uri http://onlinelibrary.wiley.com/journal/10.1002/(ISSN)1097-0029 en_US
dc.identifier.citation Venter, E, Van der Merwe, CF & Van Staden, V 2012, 'Utilization of cellulose microcapillary tubes as a model system for culturing and viral infection of mammalian cells', Microscopy Research and Technique, vol. 75, no. 10, pp. 1452-1459. en_US
dc.identifier.issn 1059-910X (print)
dc.identifier.issn 1097-0029 (online)
dc.identifier.other 10..1002/jemt.22111
dc.identifier.uri http://hdl.handle.net/2263/20777
dc.language.iso en en_US
dc.publisher Wiley en_US
dc.rights © 2012 Wiley Periodicals, Inc.. This is a preprint of an article published in Microscopy Research and Techniques available online at: http://onlinelibrary.wiley.com/journal/10.1002/(ISSN)1097-0029. en_US
dc.subject Transmission electron microscopy en_US
dc.subject High-pressure freezing (HPF) en_US
dc.subject African horsesickness virus (AHSV) en_US
dc.title Utilization of cellulose microcapillary tubes as a model system for culturing and viral infection of mammalian cells en_US
dc.type Preprint Article en_US


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