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dc.contributor.author
Banerjee, Indranil
dc.contributor.author
Yamauchi, Yohei
dc.contributor.author
Helenius, Ari
dc.contributor.author
Horvath, Peter
dc.date.accessioned
2018-08-23T12:33:48Z
dc.date.available
2017-06-10T19:49:51Z
dc.date.available
2018-08-23T12:33:48Z
dc.date.issued
2013-07-12
dc.identifier.issn
1932-6203
dc.identifier.other
10.1371/journal.pone.0068450
en_US
dc.identifier.uri
http://hdl.handle.net/20.500.11850/70157
dc.identifier.doi
10.3929/ethz-b-000070157
dc.description.abstract
Influenza A virus (IAV) represents a worldwide threat to public health by causing severe morbidity and mortality every year. Due to high mutation rate, new strains of IAV emerge frequently. These IAVs are often drug-resistant and require vaccine reformulation. A promising approach to circumvent this problem is to target host cell determinants crucial for IAV infection, but dispensable for the cell. Several RNAi-based screens have identified about one thousand cellular factors that promote IAV infection. However, systematic analyses to determine their specific functions are lacking. To address this issue, we developed quantitative, imaging-based assays to dissect seven consecutive steps in the early phases of IAV infection in tissue culture cells. The entry steps for which we developed the assays were: virus binding to the cell membrane, endocytosis, exposure to low pH in endocytic vacuoles, acid-activated fusion of viral envelope with the vacuolar membrane, nucleocapsid uncoating in the cytosol, nuclear import of viral ribonucleoproteins, and expression of the viral nucleoprotein. We adapted the assays to automated microscopy and optimized them for high-content screening. To quantify the image data, we performed both single and multi-parametric analyses, in combination with machine learning. By time-course experiments, we determined the optimal time points for each assay. Our quality control experiments showed that the assays were sufficiently robust for high-content analysis. The methods we describe in this study provide a powerful high-throughput platform to understand the host cell processes, which can eventually lead to the discovery of novel anti-pathogen strategies.
en_US
dc.format
application/pdf
en_US
dc.language.iso
en
en_US
dc.publisher
PLOS
dc.rights.uri
http://creativecommons.org/licenses/by/3.0/
dc.title
High-Content Analysis of Sequential Events during the Early Phase of Influenza A Virus Infection
en_US
dc.type
Journal Article
dc.rights.license
Creative Commons Attribution 3.0 Unported
ethz.journal.title
PLoS ONE
ethz.journal.volume
8
en_US
ethz.journal.issue
7
en_US
ethz.journal.abbreviated
PLoS ONE
ethz.pages.start
e68450
en_US
ethz.size
9 p.
en_US
ethz.version.deposit
publishedVersion
en_US
ethz.identifier.wos
ethz.publication.place
San Francisco, CA
ethz.publication.status
published
en_US
ethz.leitzahl
03495 - Helenius, Ari
en_US
ethz.leitzahl
ETH Zürich::00002 - ETH Zürich::00012 - Lehre und Forschung::00007 - Departemente::02020 - Dep. Chemie und Angewandte Biowiss. / Dep. of Chemistry and Applied Biosc.::02534 - Institut für Pharmazeutische Wiss. / Institute of Pharmaceutical Sciences::09780 - Yamauchi, Yohei / Yamauchi, Yohei
ethz.leitzahl.certified
03495 - Helenius, Ari
ethz.leitzahl.certified
ETH Zürich::00002 - ETH Zürich::00012 - Lehre und Forschung::00007 - Departemente::02020 - Dep. Chemie und Angewandte Biowiss. / Dep. of Chemistry and Applied Biosc.::02534 - Institut für Pharmazeutische Wiss. / Institute of Pharmaceutical Sciences::09780 - Yamauchi, Yohei / Yamauchi, Yohei
ethz.date.deposited
2017-06-10T19:51:39Z
ethz.source
ECIT
ethz.identifier.importid
imp593650db2cd1f52242
ethz.ecitpid
pub:111044
ethz.eth
yes
en_US
ethz.availability
Open access
en_US
ethz.rosetta.installDate
2017-07-15T09:17:15Z
ethz.rosetta.lastUpdated
2024-02-02T05:46:05Z
ethz.rosetta.versionExported
true
ethz.COinS
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