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Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication

Orbiviruses form the largest genus of the family Reoviridae consisting of at least 23 different virus species. One of these is the bluetongue virus (BTV) and causes severe hemorrhagic disease in ruminants, and is transmitted by bites of Culicoides midges. BTV is a non-enveloped virus which is releas...

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Autores principales: van Gennip, René G. P., van de Water, Sandra G. P., van Rijn, Piet A.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2014
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3896414/
https://www.ncbi.nlm.nih.gov/pubmed/24465709
http://dx.doi.org/10.1371/journal.pone.0085788
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author van Gennip, René G. P.
van de Water, Sandra G. P.
van Rijn, Piet A.
author_facet van Gennip, René G. P.
van de Water, Sandra G. P.
van Rijn, Piet A.
author_sort van Gennip, René G. P.
collection PubMed
description Orbiviruses form the largest genus of the family Reoviridae consisting of at least 23 different virus species. One of these is the bluetongue virus (BTV) and causes severe hemorrhagic disease in ruminants, and is transmitted by bites of Culicoides midges. BTV is a non-enveloped virus which is released from infected cells by cell lysis and/or a unique budding process induced by nonstructural protein NS3/NS3a encoded by genome segment 10 (Seg-10). Presence of both NS3 and NS3a is highly conserved in Culicoides borne orbiviruses which is suggesting an essential role in virus replication. We used reverse genetics to generate BTV mutants to study the function of NS3/NS3a in virus replication. Initially, BTV with small insertions in Seg-10 showed no CPE but after several passages these BTV mutants reverted to CPE phenotype comparable to wtBTV, and NS3/NS3a expression returned by repair of the ORF. These results show that there is a strong selection for functional NS3/NS3a. To abolish NS3 and/or NS3a expression, Seg-10 with one or two mutated start codons (mutAUG1, mutAUG2 and mutAUG1+2) were used to generate BTV mutants. Surprisingly, all three BTV mutants were generated and the respective AUG(Met)→GCC(Ala) mutations were maintained. The lack of expression of NS3, NS3a, or both proteins was confirmed by westernblot analysis and immunostaining of infected cells with NS3/NS3a Mabs. Growth of mutAUG1 and mutAUG1+2 virus in BSR cells was retarded in both insect and mammalian cells, and particularly virus release from insect cells was strongly reduced. Our findings now enable research on the role of RNA sequences of Seg-10 independent of known gene products, and on the function of NS3/NS3a proteins in both types of cells as well as in the host and insect vector.
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spelling pubmed-38964142014-01-24 Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication van Gennip, René G. P. van de Water, Sandra G. P. van Rijn, Piet A. PLoS One Research Article Orbiviruses form the largest genus of the family Reoviridae consisting of at least 23 different virus species. One of these is the bluetongue virus (BTV) and causes severe hemorrhagic disease in ruminants, and is transmitted by bites of Culicoides midges. BTV is a non-enveloped virus which is released from infected cells by cell lysis and/or a unique budding process induced by nonstructural protein NS3/NS3a encoded by genome segment 10 (Seg-10). Presence of both NS3 and NS3a is highly conserved in Culicoides borne orbiviruses which is suggesting an essential role in virus replication. We used reverse genetics to generate BTV mutants to study the function of NS3/NS3a in virus replication. Initially, BTV with small insertions in Seg-10 showed no CPE but after several passages these BTV mutants reverted to CPE phenotype comparable to wtBTV, and NS3/NS3a expression returned by repair of the ORF. These results show that there is a strong selection for functional NS3/NS3a. To abolish NS3 and/or NS3a expression, Seg-10 with one or two mutated start codons (mutAUG1, mutAUG2 and mutAUG1+2) were used to generate BTV mutants. Surprisingly, all three BTV mutants were generated and the respective AUG(Met)→GCC(Ala) mutations were maintained. The lack of expression of NS3, NS3a, or both proteins was confirmed by westernblot analysis and immunostaining of infected cells with NS3/NS3a Mabs. Growth of mutAUG1 and mutAUG1+2 virus in BSR cells was retarded in both insect and mammalian cells, and particularly virus release from insect cells was strongly reduced. Our findings now enable research on the role of RNA sequences of Seg-10 independent of known gene products, and on the function of NS3/NS3a proteins in both types of cells as well as in the host and insect vector. Public Library of Science 2014-01-20 /pmc/articles/PMC3896414/ /pubmed/24465709 http://dx.doi.org/10.1371/journal.pone.0085788 Text en © 2014 van Gennip et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
van Gennip, René G. P.
van de Water, Sandra G. P.
van Rijn, Piet A.
Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication
title Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication
title_full Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication
title_fullStr Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication
title_full_unstemmed Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication
title_short Bluetongue Virus Nonstructural Protein NS3/NS3a Is Not Essential for Virus Replication
title_sort bluetongue virus nonstructural protein ns3/ns3a is not essential for virus replication
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3896414/
https://www.ncbi.nlm.nih.gov/pubmed/24465709
http://dx.doi.org/10.1371/journal.pone.0085788
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