An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells

Recombinant virus-like particles (rVLPs) of flaviviruses are non-infectious particles released from cells expressing the envelope glycoproteins prM and E. Dengue virus rVLPs are recognized as a potential vaccine candidate, but large scale production of these particles is hindered by low yields and t...

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Main Authors: Nicha Charoensri, Amporn Suphatrakul, Rungtawan Sriburi, Thippawan Yasanga, Jiraphan Junjhon, Poonsook Keelapang, Utaiwan Utaipat, Chunya Puttikhunt, Watchara Kasinrerk, Prida Malasit, Nopporn Sittisombut
Format: Journal
Published: 2018
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http://cmuir.cmu.ac.th/jspui/handle/6653943832/53605
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Institution: Chiang Mai University
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spelling th-cmuir.6653943832-536052018-09-04T09:52:41Z An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells Nicha Charoensri Amporn Suphatrakul Rungtawan Sriburi Thippawan Yasanga Jiraphan Junjhon Poonsook Keelapang Utaiwan Utaipat Chunya Puttikhunt Watchara Kasinrerk Prida Malasit Nopporn Sittisombut Immunology and Microbiology Recombinant virus-like particles (rVLPs) of flaviviruses are non-infectious particles released from cells expressing the envelope glycoproteins prM and E. Dengue virus rVLPs are recognized as a potential vaccine candidate, but large scale production of these particles is hindered by low yields and the occurrence of cytopathic effects. In an approach to improve the yield of rVLPs from transfected insect cells, several components of a dengue serotype 2 virus prM. +. E expression cassette were modified and the effect of these modifications was assessed during transient expression. Enhancement of extracellular rVLP levels by simultaneous substitutions of the prM signal peptide and the stem-anchor region of E with homologous cellular and viral counterparts, respectively, was further augmented by codon optimization. Extensive formation of multinucleated cells following transfection with the codon-optimized expression cassette was abrogated by introducing an E fusion loop mutation. This mutation also helped restore the extracellular E levels affected negatively by alteration of a charged residue at the pr-M junction, which was intended to promote maturation of rVLPs during export. Optimized expression cassettes generated in this multiple add-on modification approach should be useful in the generation of stably expressing clones and production of dengue virus rVLPs for immunogenicity studies. © 2014 Elsevier B.V. 2018-09-04T09:52:41Z 2018-09-04T09:52:41Z 2014-09-01 Journal 18790984 01660934 2-s2.0-84902001370 10.1016/j.jviromet.2014.04.019 https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=84902001370&origin=inward http://cmuir.cmu.ac.th/jspui/handle/6653943832/53605
institution Chiang Mai University
building Chiang Mai University Library
country Thailand
collection CMU Intellectual Repository
topic Immunology and Microbiology
spellingShingle Immunology and Microbiology
Nicha Charoensri
Amporn Suphatrakul
Rungtawan Sriburi
Thippawan Yasanga
Jiraphan Junjhon
Poonsook Keelapang
Utaiwan Utaipat
Chunya Puttikhunt
Watchara Kasinrerk
Prida Malasit
Nopporn Sittisombut
An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
description Recombinant virus-like particles (rVLPs) of flaviviruses are non-infectious particles released from cells expressing the envelope glycoproteins prM and E. Dengue virus rVLPs are recognized as a potential vaccine candidate, but large scale production of these particles is hindered by low yields and the occurrence of cytopathic effects. In an approach to improve the yield of rVLPs from transfected insect cells, several components of a dengue serotype 2 virus prM. +. E expression cassette were modified and the effect of these modifications was assessed during transient expression. Enhancement of extracellular rVLP levels by simultaneous substitutions of the prM signal peptide and the stem-anchor region of E with homologous cellular and viral counterparts, respectively, was further augmented by codon optimization. Extensive formation of multinucleated cells following transfection with the codon-optimized expression cassette was abrogated by introducing an E fusion loop mutation. This mutation also helped restore the extracellular E levels affected negatively by alteration of a charged residue at the pr-M junction, which was intended to promote maturation of rVLPs during export. Optimized expression cassettes generated in this multiple add-on modification approach should be useful in the generation of stably expressing clones and production of dengue virus rVLPs for immunogenicity studies. © 2014 Elsevier B.V.
format Journal
author Nicha Charoensri
Amporn Suphatrakul
Rungtawan Sriburi
Thippawan Yasanga
Jiraphan Junjhon
Poonsook Keelapang
Utaiwan Utaipat
Chunya Puttikhunt
Watchara Kasinrerk
Prida Malasit
Nopporn Sittisombut
author_facet Nicha Charoensri
Amporn Suphatrakul
Rungtawan Sriburi
Thippawan Yasanga
Jiraphan Junjhon
Poonsook Keelapang
Utaiwan Utaipat
Chunya Puttikhunt
Watchara Kasinrerk
Prida Malasit
Nopporn Sittisombut
author_sort Nicha Charoensri
title An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
title_short An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
title_full An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
title_fullStr An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
title_full_unstemmed An optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
title_sort optimized expression vector for improving the yield of dengue virus-like particles from transfected insect cells
publishDate 2018
url https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=84902001370&origin=inward
http://cmuir.cmu.ac.th/jspui/handle/6653943832/53605
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