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Characterization of polyclonal antibodies against the capsid proteins of Ljungan virus
University of Kalmar, School of Pure and Applied Natural Sciences.
University of Kalmar, School of Pure and Applied Natural Sciences.
University of Kalmar, School of Pure and Applied Natural Sciences.
Apodemus AB.
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2008 (English)In: Journal of Virological Methods, ISSN 0166-0934, E-ISSN 1879-0984, Vol. 150, no 1-2, p. 34-40Article in journal (Refereed) Published
Abstract [en]

Ljungan virus (LV) is a suspected human pathogen isolated from voles in Sweden and North America. To enable virus detection and studies of localization and activity of virion proteins, polyclonal antibodies were produced against bacterially expressed capsid proteins of the LV strain, 87-012G. Specific detection of proteins corresponding to viral antigens in lysates of LV infected cells was demonstrated by immunoblotting using each one of the generated polyclonal antibodies. In addition, native viral antigens present in cell culture infected with LV strains 87-012G or 145SLG were detected in ELISA and by immunofluorescence using the antibodies against the VP0 and VP1 proteins. The anti-VP3 antibody did not react with native proteins of the LV virion, suggesting that the VP3 is less potent in evoking humoral response and may have a less exposed orientation in the virus capsid. No activity of the antibodies was observed against the closely related human parechovirus type 1. The polyclonal antibody against the VP1 protein was further used for detection of LV infected myocytes in a mouse model of LV-induced myocarditis. Thus, polyclonal antibodies against recombinant viral capsid proteins enabled detection of natural LV virions by several different immunological methods.

Place, publisher, year, edition, pages
Elsevier, 2008. Vol. 150, no 1-2, p. 34-40
Keywords [en]
Parechovirus, Protein expression, Polyclonal antibodies, Virus detection, Immunodetection
National Category
Microbiology in the medical area
Research subject
Biomedical Sciences, Virology
Identifiers
URN: urn:nbn:se:hik:diva-928DOI: 10.1016/j.jviromet.2008.02.012PubMedID: 18403027OAI: oai:DiVA.org:hik-928DiVA, id: diva2:128032
Available from: 2008-12-11 Created: 2008-12-10 Last updated: 2018-01-13Bibliographically approved
In thesis
1. Ljungan Virus Replication in Cell Culture
Open this publication in new window or tab >>Ljungan Virus Replication in Cell Culture
2007 (English)Doctoral thesis, comprehensive summary (Other scientific)
Abstract [en]

Ljungan virus (LV) is a recently identified picornavirus of the genus Parechovirus. LV has been isolated from voles trapped in Sweden and also in the United States. LV infected small rodents may suffer from diabetes type 1 and type 2 like symptoms, myocarditis and encephalitis. LV has been proposed as a human pathogen, with indications of causing diabetes type 1, myocarditis and intrauterine fetal deaths.

In this thesis, cell culture adapted LV strains were utilised for development and adaptation of several basic methodological protocols to study the LV biology, e.g. real time PCR, highly specific antibodies and a reverse genetics system. These methods allowed detailed studies of this virus and how it interacts with the host cell. The genomic 5'-end was identified and modelling showed unique secondary structure folding of this region. The LV encodes an aphthovirus-like 2A protein with a DvExNPGP motif. This motif was found to mediate primary cleavage of the LV polyprotein in vitro and is proposed to constitute the carboxy terminus of the structural protein VP1 in LV. Rabbit polyclonal antibodies generated against recombinant structural proteins were used to verify that the LV virion is composed of the structural proteins VP0, VP1 and VP3. Cell culture studies showed that LV replicates to low titer with an absent or delayed cell lysis. LV is proposed to be able to spread by a, for picornaviruses, not previously demonstrated direct cell-to-cell transmission. All results taken together suggest a maintenance strategy of LV including low amounts of the LV genome and persistently infected hosts. Stability studies showed that the LV virion not only maintain activity in acidic and alkaline environments but also exhibit resistance to the commonly used disinfectant Virkon®.The results presented in this thesis show that LV has several unique properties, not previously observed for a picornavirus.

Place, publisher, year, edition, pages
Högskolan i Kalmar, 2007
Series
Dissertation series: University of Kalmar, Faculty of Natural Science, ISSN 1650-2779 ; 37
Keywords
Ljungan virus, picornavirus, parechovirus, 5' - RACE, 5' -end, infectious cDNA clone, real time PCR, virus purification, virion stability, disinfection, aphthovirus-like 2A
National Category
Microbiology in the medical area
Research subject
Ecology, Microbiology
Identifiers
urn:nbn:se:hik:diva-10 (URN)978-91-89584-70-9 (ISBN)
Public defence
2007-04-20, 09:30 (English)
Opponent
Supervisors
Available from: 2007-08-27 Created: 2007-08-27 Last updated: 2018-01-13Bibliographically approved

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Tolf, ConnyGullberg, MariaEdman, KjellLindberg, A Michael

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