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dc.contributor.author
Pacesa, Martin
dc.contributor.author
Hendrickx, Rodinde
dc.contributor.author
Bieri, Manuela
dc.contributor.author
Flatt, Justin W.
dc.contributor.author
Greber, Urs F.
dc.contributor.author
Hemmi, Silvio
dc.date.accessioned
2017-11-07T12:54:11Z
dc.date.available
2017-10-06T02:08:51Z
dc.date.available
2017-11-07T12:52:11Z
dc.date.available
2017-11-07T12:54:11Z
dc.date.issued
2017-08-18
dc.identifier.issn
1743-422X
dc.identifier.other
10.1186/s12985-017-0822-5
en_US
dc.identifier.uri
http://hdl.handle.net/20.500.11850/190505
dc.identifier.doi
10.3929/ethz-b-000190505
dc.description.abstract
Background: Adenoviruses are common pathogens infecting animals and humans. They are classified based on serology, or genome sequence information. These methods have limitations due to lengthy procedures or lack of infectivity data. Adenoviruses are easy to produce and amenable to genetic and biochemical modifications, which makes them a powerful tool for biological studies, and clinical gene-delivery and vaccine applications. Antibodies directed against adenoviral proteins are important diagnostic tools for virus identification in vivo and in vitro, and are used to elucidate infection mechanisms, often in combination with genomic sequencing and type specific information from hyper-variable regions of structural proteins. Results: Here we describe a novel and readily useable method for cloning, expressing and purifying small fragments of hyper-variable regions 1-6 of the adenoviral hexon protein. We used these polypeptides as antigens for generating polyclonal rabbit antibodies against human adenovirus 3 (HAdV-B3), mouse adenovirus 1 (MAdV-1) and MAdV-2 hexon. In Western immunoblots with lysates from cells infected from thirteen human and three mouse viruses, these antibodies bound to homologous full-length hexon protein and revealed variable levels of cross-reactivity to heterologous hexons. Results from immuno-fluorescence and electron microscopy studies indicated that HAdV-B3 and MAdV-2 hexon antibodies recognized native forms of hexon. Conclusions: The procedure described here can in principle be applied to any adenovirus for which genome sequence information is available. It provides a basis for generating novel type-specific tools in diagnostics and research, and extends beyond the commonly used anti-viral antibodies raised against purified viruses or subviral components.
en_US
dc.format
application/pdf
dc.language.iso
en
en_US
dc.publisher
BioMed Central
en_US
dc.rights.uri
http://creativecommons.org/licenses/by/4.0/
dc.subject
Protein Purification
en_US
dc.subject
Immunoblotting
en_US
dc.subject
Electron Microscopy
en_US
dc.subject
Antibodies
en_US
dc.subject
Immunofluorescence
en_US
dc.subject
Virus Blocking
en_US
dc.subject
Neutralization
en_US
dc.subject
Adenovirus
en_US
dc.subject
Hexon
en_US
dc.title
Small-size recombinant adenoviral hexon protein fragments for the production of virus-type specific antibodies
en_US
dc.type
Journal Article
dc.rights.license
Creative Commons Attribution 4.0 International
ethz.journal.title
Virology Journal
ethz.journal.volume
14
en_US
ethz.journal.abbreviated
Virol. j.
ethz.pages.start
158
en_US
ethz.size
14 p.
en_US
ethz.version.deposit
publishedVersion
en_US
ethz.identifier.wos
ethz.identifier.scopus
ethz.publication.place
London
ethz.publication.status
published
en_US
ethz.date.deposited
2017-10-06T02:08:57Z
ethz.source
WOS
ethz.eth
yes
en_US
ethz.availability
Open access
en_US
ethz.rosetta.installDate
2017-11-07T12:52:18Z
ethz.rosetta.lastUpdated
2024-02-02T02:50:34Z
ethz.rosetta.versionExported
true
ethz.COinS
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