A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line

Widely used methods for quantification of human cytomegalovirus (HCMV) infection in cell culture such as immunoblotting or plaque reduction assays are generally restricted to low throughput and require time-consuming evaluation. Up to now, only few HCMV reporter cell lines have been generated to ove...

Descripción completa

Detalles Bibliográficos
Autores principales: Maier, Anna Katharina, Jung, Raimund, Villinger, Clarissa, Schubert, Axel, Walther, Paul, Sinzger, Christian, Lieber, Diana
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2017
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5217978/
https://www.ncbi.nlm.nih.gov/pubmed/28060895
http://dx.doi.org/10.1371/journal.pone.0169580
_version_ 1782492187958706176
author Maier, Anna Katharina
Jung, Raimund
Villinger, Clarissa
Schubert, Axel
Walther, Paul
Sinzger, Christian
Lieber, Diana
author_facet Maier, Anna Katharina
Jung, Raimund
Villinger, Clarissa
Schubert, Axel
Walther, Paul
Sinzger, Christian
Lieber, Diana
author_sort Maier, Anna Katharina
collection PubMed
description Widely used methods for quantification of human cytomegalovirus (HCMV) infection in cell culture such as immunoblotting or plaque reduction assays are generally restricted to low throughput and require time-consuming evaluation. Up to now, only few HCMV reporter cell lines have been generated to overcome these restrictions and they are afflicted with other limitations because permanently expandable cell lines are normally not fully permissive to HCMV. In this work, a previously existing epithelial cell line hosting a luciferase gene under control of a Varicella-zoster virus promoter was adopted to investigate HCMV infection. The cells were susceptible to different HCMV strains at infection efficiencies that corresponded to their respective degree of epithelial cell tropism. Expression of early and late viral antigens, formation of nuclear inclusions, release of infectious virus progeny, and focal growth indicated productive viral replication. However, viral release and spread occurred at lower levels than in primary cell lines which appears to be due to a malfunction of virion morphogenesis during the nuclear stage. Expression of the luciferase reporter gene was specifically induced in HCMV infected cultures as a function of the virus dose and dependent on viral immediate early gene expression. The level of reporter activity accurately reflected infection efficiencies as determined by viral antigen immunostaining, and hence could discriminate the cell tropism of the tested virus strains. As proof-of-principle, we demonstrate that this cell line is applicable to evaluate drug resistance of clinical HCMV isolates and the neutralization capacity of human sera, and that it allows comparative and simultaneous analysis of HCMV and human herpes simplex virus type 1. In summary, the permanent epithelial reporter cell line allows robust, rapid and objective quantitation of HCMV infection and it will be particularly useful in higher throughput analyses as well as in comparative analyses of different human herpesviruses.
format Online
Article
Text
id pubmed-5217978
institution National Center for Biotechnology Information
language English
publishDate 2017
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-52179782017-01-19 A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line Maier, Anna Katharina Jung, Raimund Villinger, Clarissa Schubert, Axel Walther, Paul Sinzger, Christian Lieber, Diana PLoS One Research Article Widely used methods for quantification of human cytomegalovirus (HCMV) infection in cell culture such as immunoblotting or plaque reduction assays are generally restricted to low throughput and require time-consuming evaluation. Up to now, only few HCMV reporter cell lines have been generated to overcome these restrictions and they are afflicted with other limitations because permanently expandable cell lines are normally not fully permissive to HCMV. In this work, a previously existing epithelial cell line hosting a luciferase gene under control of a Varicella-zoster virus promoter was adopted to investigate HCMV infection. The cells were susceptible to different HCMV strains at infection efficiencies that corresponded to their respective degree of epithelial cell tropism. Expression of early and late viral antigens, formation of nuclear inclusions, release of infectious virus progeny, and focal growth indicated productive viral replication. However, viral release and spread occurred at lower levels than in primary cell lines which appears to be due to a malfunction of virion morphogenesis during the nuclear stage. Expression of the luciferase reporter gene was specifically induced in HCMV infected cultures as a function of the virus dose and dependent on viral immediate early gene expression. The level of reporter activity accurately reflected infection efficiencies as determined by viral antigen immunostaining, and hence could discriminate the cell tropism of the tested virus strains. As proof-of-principle, we demonstrate that this cell line is applicable to evaluate drug resistance of clinical HCMV isolates and the neutralization capacity of human sera, and that it allows comparative and simultaneous analysis of HCMV and human herpes simplex virus type 1. In summary, the permanent epithelial reporter cell line allows robust, rapid and objective quantitation of HCMV infection and it will be particularly useful in higher throughput analyses as well as in comparative analyses of different human herpesviruses. Public Library of Science 2017-01-06 /pmc/articles/PMC5217978/ /pubmed/28060895 http://dx.doi.org/10.1371/journal.pone.0169580 Text en © 2017 Maier 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 (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Maier, Anna Katharina
Jung, Raimund
Villinger, Clarissa
Schubert, Axel
Walther, Paul
Sinzger, Christian
Lieber, Diana
A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line
title A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line
title_full A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line
title_fullStr A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line
title_full_unstemmed A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line
title_short A Luciferase Gene Driven by an Alphaherpesviral Promoter Also Responds to Immediate Early Antigens of the Betaherpesvirus HCMV, Allowing Comparative Analyses of Different Human Herpesviruses in One Reporter Cell Line
title_sort luciferase gene driven by an alphaherpesviral promoter also responds to immediate early antigens of the betaherpesvirus hcmv, allowing comparative analyses of different human herpesviruses in one reporter cell line
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5217978/
https://www.ncbi.nlm.nih.gov/pubmed/28060895
http://dx.doi.org/10.1371/journal.pone.0169580
work_keys_str_mv AT maierannakatharina aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT jungraimund aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT villingerclarissa aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT schubertaxel aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT waltherpaul aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT sinzgerchristian aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT lieberdiana aluciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT maierannakatharina luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT jungraimund luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT villingerclarissa luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT schubertaxel luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT waltherpaul luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT sinzgerchristian luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline
AT lieberdiana luciferasegenedrivenbyanalphaherpesviralpromoteralsorespondstoimmediateearlyantigensofthebetaherpesvirushcmvallowingcomparativeanalysesofdifferenthumanherpesvirusesinonereportercellline

Ejemplares similares