Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells

Olivero-Deibe, Natalia - Tomé Poderti, Lorena Magalí - Carrión, Federico - Bianchi, Sergio - Fló Díaz, Martín - Prieto Mena, Daniel - Rammauro, Florencia - Addiego, Andrés - Ibañez, Natalia - Portela, María Magdalena - Durán, Rosario - Berois, Mabel - Pritsch, Otto

Editor(es): Duus, Karen

Resumen:

Bovine leukemia virus (BLV) is an oncogenic deltaretrovirus that infects cattle worldwide. In Uruguay, it is estimated that more than 70% of dairy cattle are infected, causing serious economic losses due to decreased milk production, increased calving interval, and livestock losses due to lymphosarcoma. Several attempts to develop vaccine candidates that activate protective immune responses against BLV were performed, but up to date, there is no vaccine that ensures efficient protection and/or decreased viral transmission. The development and application of new vaccines that effectively control BLV infection represent amajor challenge for countries with a high prevalence of infection. In this study, we generated two Drosophila melanogaster S2 stable cell lines capable of producing BLV virus-like particles (BLV-VLPs). One of them, BLV-VLP1, expressed both Gag and Env wild-type (Envwt) full-length proteins, whereas BLV-VLP2 contain Gag together with a mutant form of Env non-susceptible to proteolytic maturation by cellular furin type enzymes (EnvFm).We showed that Envwt is properly cleaved by cellular furin, whereas EnvFm is produced as a full-length gp72 precursor, which undergoes some partial cleavage. We observed that said mutation does not drastically affect its expression or its entry into the secretory pathway of S2 insect cells. In addition, it is expressed on the membrane and retains significant structural motifs when expressed in S2 insect cells. Morphology and size of purified BLV-VLPs were analyzed by transmission electron microscopy and dynamic light scattering, showing numerous non-aggregated and approximately spherical particles of variable diameter (70–200 nm) as previously reported for retroviral VLPs produced using different expression systems. Furthermore, we identified two N-glycosylation patterns rich in mannose in EnvFm protein displayed on VLP2. Our results suggest that the VLPs produced in Drosophila S2 cells could be a potential immunogen to be used in the development of BLV vaccines that might contribute, in conjunction with other control strategies, to reduce the transmission of the virus.


Detalles Bibliográficos
2021
CSIC I+D 2014
ANII: ALI_1_2016_2_129851; POS_NAC_2015_1_109471
PEDECIBA-FOCEM: COF 03/11
CAP: BFPD_2020_1#28143834
Bovine leukemia virus (BLV)
Virus-like particles (VLP)
Furin cleavage site
Immunogens
Gag
Env
Retrovirus
Inglés
Universidad de la República
COLIBRI
https://hdl.handle.net/20.500.12008/31348
Acceso abierto
Licencia Creative Commons Atribución (CC - By 4.0)
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author Olivero-Deibe, Natalia
author2 Tomé Poderti, Lorena Magalí
Carrión, Federico
Bianchi, Sergio
Fló Díaz, Martín
Prieto Mena, Daniel
Rammauro, Florencia
Addiego, Andrés
Ibañez, Natalia
Portela, María Magdalena
Durán, Rosario
Berois, Mabel
Pritsch, Otto
author2_role author
author
author
author
author
author
author
author
author
author
author
author
author_facet Olivero-Deibe, Natalia
Tomé Poderti, Lorena Magalí
Carrión, Federico
Bianchi, Sergio
Fló Díaz, Martín
Prieto Mena, Daniel
Rammauro, Florencia
Addiego, Andrés
Ibañez, Natalia
Portela, María Magdalena
Durán, Rosario
Berois, Mabel
Pritsch, Otto
author_role author
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collection COLIBRI
dc.contributor.filiacion.none.fl_str_mv Olivero-Deibe Natalia, Instituto Pasteur (Montevideo)
Tomé Poderti Lorena Magalí, Instituto Pasteur (Montevideo)
Carrión Federico, Instituto Pasteur (Montevideo)
Bianchi Sergio, Instituto Pasteur (Montevideo)
Fló Díaz Martín, Instituo Pasteur (Montevideo)
Prieto Mena Daniel, IIBCE
Rammauro Florencia, Instituo Pasteur (Montevideo)
Addiego Andrés, Instituo Pasteur (Montevideo)
Ibañez Natalia, Instituo Pasteur (Montevideo)
Portela María Magdalena, Instituo Pasteur (Montevideo)
Durán Rosario, Instituo Pasteur (Montevideo)
Berois Mabel, Universidad de la República (Uruguay). Facultad de Ciencias. Instituto de Biología.
Pritsch Otto, Instituo Pasteur (Montevideo)
dc.creator.editor.none.fl_str_mv Duus, Karen
dc.creator.none.fl_str_mv Olivero-Deibe, Natalia
Tomé Poderti, Lorena Magalí
Carrión, Federico
Bianchi, Sergio
Fló Díaz, Martín
Prieto Mena, Daniel
Rammauro, Florencia
Addiego, Andrés
Ibañez, Natalia
Portela, María Magdalena
Durán, Rosario
Berois, Mabel
Pritsch, Otto
dc.date.accessioned.none.fl_str_mv 2022-04-27T18:42:43Z
dc.date.available.none.fl_str_mv 2022-04-27T18:42:43Z
dc.date.issued.none.fl_str_mv 2021
dc.description.abstract.none.fl_txt_mv Bovine leukemia virus (BLV) is an oncogenic deltaretrovirus that infects cattle worldwide. In Uruguay, it is estimated that more than 70% of dairy cattle are infected, causing serious economic losses due to decreased milk production, increased calving interval, and livestock losses due to lymphosarcoma. Several attempts to develop vaccine candidates that activate protective immune responses against BLV were performed, but up to date, there is no vaccine that ensures efficient protection and/or decreased viral transmission. The development and application of new vaccines that effectively control BLV infection represent amajor challenge for countries with a high prevalence of infection. In this study, we generated two Drosophila melanogaster S2 stable cell lines capable of producing BLV virus-like particles (BLV-VLPs). One of them, BLV-VLP1, expressed both Gag and Env wild-type (Envwt) full-length proteins, whereas BLV-VLP2 contain Gag together with a mutant form of Env non-susceptible to proteolytic maturation by cellular furin type enzymes (EnvFm).We showed that Envwt is properly cleaved by cellular furin, whereas EnvFm is produced as a full-length gp72 precursor, which undergoes some partial cleavage. We observed that said mutation does not drastically affect its expression or its entry into the secretory pathway of S2 insect cells. In addition, it is expressed on the membrane and retains significant structural motifs when expressed in S2 insect cells. Morphology and size of purified BLV-VLPs were analyzed by transmission electron microscopy and dynamic light scattering, showing numerous non-aggregated and approximately spherical particles of variable diameter (70–200 nm) as previously reported for retroviral VLPs produced using different expression systems. Furthermore, we identified two N-glycosylation patterns rich in mannose in EnvFm protein displayed on VLP2. Our results suggest that the VLPs produced in Drosophila S2 cells could be a potential immunogen to be used in the development of BLV vaccines that might contribute, in conjunction with other control strategies, to reduce the transmission of the virus.
dc.description.es.fl_txt_mv Material complementario: https://www.frontiersin.org/articles/10.3389/fviro.2021.756559/full#supplementary-material
dc.description.sponsorship.none.fl_txt_mv CSIC I+D 2014
ANII: ALI_1_2016_2_129851; POS_NAC_2015_1_109471
PEDECIBA-FOCEM: COF 03/11
CAP: BFPD_2020_1#28143834
dc.format.extent.es.fl_str_mv 13 h
dc.format.mimetype.es.fl_str_mv application/pdf
dc.identifier.citation.es.fl_str_mv Olivero-Deibe, N., Tomé Poderti, L., Carrión, F., [y otros autores]. "Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells". Frontiers in Virology. [en línea] 2021, 1:756559. doi: 10.3389/fviro.2021.756559
dc.identifier.doi.none.fl_str_mv 10.3389/fviro.2021.756559
dc.identifier.issn.none.fl_str_mv 2673-818X
dc.identifier.uri.none.fl_str_mv https://hdl.handle.net/20.500.12008/31348
dc.language.iso.none.fl_str_mv en
eng
dc.publisher.es.fl_str_mv Frontiers Media
dc.relation.ispartof.es.fl_str_mv Frontiers in Virology, 2021, 1:756559
dc.rights.license.none.fl_str_mv Licencia Creative Commons Atribución (CC - By 4.0)
dc.rights.none.fl_str_mv info:eu-repo/semantics/openAccess
dc.source.none.fl_str_mv reponame:COLIBRI
instname:Universidad de la República
instacron:Universidad de la República
dc.subject.es.fl_str_mv Bovine leukemia virus (BLV)
Virus-like particles (VLP)
Furin cleavage site
Immunogens
Gag
Env
Retrovirus
dc.title.none.fl_str_mv Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
dc.type.es.fl_str_mv Artículo
dc.type.none.fl_str_mv info:eu-repo/semantics/article
dc.type.version.none.fl_str_mv info:eu-repo/semantics/publishedVersion
description Material complementario: https://www.frontiersin.org/articles/10.3389/fviro.2021.756559/full#supplementary-material
eu_rights_str_mv openAccess
format article
id COLIBRI_9b9a68d7e5f20891ce265a2f404a253c
identifier_str_mv Olivero-Deibe, N., Tomé Poderti, L., Carrión, F., [y otros autores]. "Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells". Frontiers in Virology. [en línea] 2021, 1:756559. doi: 10.3389/fviro.2021.756559
2673-818X
10.3389/fviro.2021.756559
instacron_str Universidad de la República
institution Universidad de la República
instname_str Universidad de la República
language eng
language_invalid_str_mv en
network_acronym_str COLIBRI
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publishDate 2021
reponame_str COLIBRI
repository.mail.fl_str_mv mabel.seroubian@seciu.edu.uy
repository.name.fl_str_mv COLIBRI - Universidad de la República
repository_id_str 4771
rights_invalid_str_mv Licencia Creative Commons Atribución (CC - By 4.0)
spelling Olivero-Deibe Natalia, Instituto Pasteur (Montevideo)Tomé Poderti Lorena Magalí, Instituto Pasteur (Montevideo)Carrión Federico, Instituto Pasteur (Montevideo)Bianchi Sergio, Instituto Pasteur (Montevideo)Fló Díaz Martín, Instituo Pasteur (Montevideo)Prieto Mena Daniel, IIBCERammauro Florencia, Instituo Pasteur (Montevideo)Addiego Andrés, Instituo Pasteur (Montevideo)Ibañez Natalia, Instituo Pasteur (Montevideo)Portela María Magdalena, Instituo Pasteur (Montevideo)Durán Rosario, Instituo Pasteur (Montevideo)Berois Mabel, Universidad de la República (Uruguay). Facultad de Ciencias. Instituto de Biología.Pritsch Otto, Instituo Pasteur (Montevideo)2022-04-27T18:42:43Z2022-04-27T18:42:43Z2021Olivero-Deibe, N., Tomé Poderti, L., Carrión, F., [y otros autores]. "Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells". Frontiers in Virology. [en línea] 2021, 1:756559. doi: 10.3389/fviro.2021.7565592673-818Xhttps://hdl.handle.net/20.500.12008/3134810.3389/fviro.2021.756559Material complementario: https://www.frontiersin.org/articles/10.3389/fviro.2021.756559/full#supplementary-materialBovine leukemia virus (BLV) is an oncogenic deltaretrovirus that infects cattle worldwide. In Uruguay, it is estimated that more than 70% of dairy cattle are infected, causing serious economic losses due to decreased milk production, increased calving interval, and livestock losses due to lymphosarcoma. Several attempts to develop vaccine candidates that activate protective immune responses against BLV were performed, but up to date, there is no vaccine that ensures efficient protection and/or decreased viral transmission. The development and application of new vaccines that effectively control BLV infection represent amajor challenge for countries with a high prevalence of infection. In this study, we generated two Drosophila melanogaster S2 stable cell lines capable of producing BLV virus-like particles (BLV-VLPs). One of them, BLV-VLP1, expressed both Gag and Env wild-type (Envwt) full-length proteins, whereas BLV-VLP2 contain Gag together with a mutant form of Env non-susceptible to proteolytic maturation by cellular furin type enzymes (EnvFm).We showed that Envwt is properly cleaved by cellular furin, whereas EnvFm is produced as a full-length gp72 precursor, which undergoes some partial cleavage. We observed that said mutation does not drastically affect its expression or its entry into the secretory pathway of S2 insect cells. In addition, it is expressed on the membrane and retains significant structural motifs when expressed in S2 insect cells. Morphology and size of purified BLV-VLPs were analyzed by transmission electron microscopy and dynamic light scattering, showing numerous non-aggregated and approximately spherical particles of variable diameter (70–200 nm) as previously reported for retroviral VLPs produced using different expression systems. Furthermore, we identified two N-glycosylation patterns rich in mannose in EnvFm protein displayed on VLP2. Our results suggest that the VLPs produced in Drosophila S2 cells could be a potential immunogen to be used in the development of BLV vaccines that might contribute, in conjunction with other control strategies, to reduce the transmission of the virus.Submitted by Faget Cecilia (lfaget@fcien.edu.uy) on 2022-04-27T15:18:11Z No. of bitstreams: 2 license_rdf: 19875 bytes, checksum: 9fdbed07f52437945402c4e70fa4773e (MD5) fviro-01-756559.pdf: 2327856 bytes, checksum: d1fdf0ebb00f09139fd5fc1a7e9b9455 (MD5)Approved for entry into archive by Faget Cecilia (lfaget@fcien.edu.uy) on 2022-04-27T17:52:54Z (GMT) No. of bitstreams: 2 license_rdf: 19875 bytes, checksum: 9fdbed07f52437945402c4e70fa4773e (MD5) fviro-01-756559.pdf: 2327856 bytes, checksum: d1fdf0ebb00f09139fd5fc1a7e9b9455 (MD5)Made available in DSpace by Luna Fabiana (fabiana.luna@seciu.edu.uy) on 2022-04-27T18:42:43Z (GMT). No. of bitstreams: 2 license_rdf: 19875 bytes, checksum: 9fdbed07f52437945402c4e70fa4773e (MD5) fviro-01-756559.pdf: 2327856 bytes, checksum: d1fdf0ebb00f09139fd5fc1a7e9b9455 (MD5) Previous issue date: 2021CSIC I+D 2014ANII: ALI_1_2016_2_129851; POS_NAC_2015_1_109471PEDECIBA-FOCEM: COF 03/11CAP: BFPD_2020_1#2814383413 happlication/pdfenengFrontiers MediaFrontiers in Virology, 2021, 1:756559Las obras depositadas en el Repositorio se rigen por la Ordenanza de los Derechos de la Propiedad Intelectual de la Universidad de la República.(Res. Nº 91 de C.D.C. de 8/III/1994 – D.O. 7/IV/1994) y por la Ordenanza del Repositorio Abierto de la Universidad de la República (Res. Nº 16 de C.D.C. de 07/10/2014)info:eu-repo/semantics/openAccessLicencia Creative Commons Atribución (CC - By 4.0)Bovine leukemia virus (BLV)Virus-like particles (VLP)Furin cleavage siteImmunogensGagEnvRetrovirusExpression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cellsArtículoinfo:eu-repo/semantics/articleinfo:eu-repo/semantics/publishedVersionreponame:COLIBRIinstname:Universidad de la Repúblicainstacron:Universidad de la RepúblicaOlivero-Deibe, NataliaTomé Poderti, Lorena MagalíCarrión, FedericoBianchi, SergioFló Díaz, MartínPrieto Mena, DanielRammauro, FlorenciaAddiego, AndrésIbañez, NataliaPortela, María MagdalenaDurán, RosarioBerois, MabelPritsch, OttoDuus, KarenLICENSElicense.txtlicense.txttext/plain; charset=utf-84267http://localhost:8080/xmlui/bitstream/20.500.12008/31348/5/license.txt6429389a7df7277b72b7924fdc7d47a9MD55CC-LICENSElicense_urllicense_urltext/plain; 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- Universidad de la Repúblicafalse
spellingShingle Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
Olivero-Deibe, Natalia
Bovine leukemia virus (BLV)
Virus-like particles (VLP)
Furin cleavage site
Immunogens
Gag
Env
Retrovirus
status_str publishedVersion
title Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
title_full Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
title_fullStr Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
title_full_unstemmed Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
title_short Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
title_sort Expression, purification, and characterization of bovine leukemia virus-like particles produced in Drosophila S2 cells
topic Bovine leukemia virus (BLV)
Virus-like particles (VLP)
Furin cleavage site
Immunogens
Gag
Env
Retrovirus
url https://hdl.handle.net/20.500.12008/31348