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Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles

We have previously described a new family of mutant adenoviruses carrying different combinations of attB/attP sequences from bacteriophage PhiC31 flanking the Ad5 packaging domain. These novel helper viruses have a significantly delayed viral life cycle and a severe packaging impairment, regardless...

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Autores principales: Alba, Raul, Cots, Dan, Ostapchuk, Philomena, Bosch, Assumpcio, Hearing, Patrick, Chillon, Miguel
Formato: Texto
Lenguaje:English
Publicado: Public Library of Science 2011
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3097180/
https://www.ncbi.nlm.nih.gov/pubmed/21611162
http://dx.doi.org/10.1371/journal.pone.0019564
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author Alba, Raul
Cots, Dan
Ostapchuk, Philomena
Bosch, Assumpcio
Hearing, Patrick
Chillon, Miguel
author_facet Alba, Raul
Cots, Dan
Ostapchuk, Philomena
Bosch, Assumpcio
Hearing, Patrick
Chillon, Miguel
author_sort Alba, Raul
collection PubMed
description We have previously described a new family of mutant adenoviruses carrying different combinations of attB/attP sequences from bacteriophage PhiC31 flanking the Ad5 packaging domain. These novel helper viruses have a significantly delayed viral life cycle and a severe packaging impairment, regardless of the presence of PhiC31 recombinase. Their infectious viral titers are significantly lower (100–1000 fold) than those of control adenovirus at 36 hours post-infection, but allow for efficient packaging of helper-dependent adenovirus. In the present work, we have analyzed which steps of the adenovirus life cycle are altered in attB-helper adenoviruses and investigated whether these viruses can provide the necessary viral proteins in trans. The entry of attB-adenoviral genomes into the cell nucleus early at early timepoints post-infection was not impaired and viral protein expression levels were found to be similar to those of control adenovirus. However, electron microscopy and capsid protein composition analyses revealed that attB-adenoviruses remain at an intermediate state of maturation 36 hours post-infection in comparison to control adenovirus which were fully mature and infective at this time point. Therefore, an additional 20–24 hours were found to be required for the appearance of mature attB-adenovirus. Interestingly, attB-adenovirus assembly and infectivity was restored by inserting a second packaging signal close to the right-end ITR, thus discarding the possibility that the attB-adenovirus genome was retained in a nuclear compartment deleterious for virus assembly. The present study may have substantive implications for helper-dependent adenovirus technology since helper attB-adenovirus allows for preferential packaging of helper-dependent adenovirus genomes.
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spelling pubmed-30971802011-05-24 Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles Alba, Raul Cots, Dan Ostapchuk, Philomena Bosch, Assumpcio Hearing, Patrick Chillon, Miguel PLoS One Research Article We have previously described a new family of mutant adenoviruses carrying different combinations of attB/attP sequences from bacteriophage PhiC31 flanking the Ad5 packaging domain. These novel helper viruses have a significantly delayed viral life cycle and a severe packaging impairment, regardless of the presence of PhiC31 recombinase. Their infectious viral titers are significantly lower (100–1000 fold) than those of control adenovirus at 36 hours post-infection, but allow for efficient packaging of helper-dependent adenovirus. In the present work, we have analyzed which steps of the adenovirus life cycle are altered in attB-helper adenoviruses and investigated whether these viruses can provide the necessary viral proteins in trans. The entry of attB-adenoviral genomes into the cell nucleus early at early timepoints post-infection was not impaired and viral protein expression levels were found to be similar to those of control adenovirus. However, electron microscopy and capsid protein composition analyses revealed that attB-adenoviruses remain at an intermediate state of maturation 36 hours post-infection in comparison to control adenovirus which were fully mature and infective at this time point. Therefore, an additional 20–24 hours were found to be required for the appearance of mature attB-adenovirus. Interestingly, attB-adenovirus assembly and infectivity was restored by inserting a second packaging signal close to the right-end ITR, thus discarding the possibility that the attB-adenovirus genome was retained in a nuclear compartment deleterious for virus assembly. The present study may have substantive implications for helper-dependent adenovirus technology since helper attB-adenovirus allows for preferential packaging of helper-dependent adenovirus genomes. Public Library of Science 2011-05-18 /pmc/articles/PMC3097180/ /pubmed/21611162 http://dx.doi.org/10.1371/journal.pone.0019564 Text en Alba 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
Alba, Raul
Cots, Dan
Ostapchuk, Philomena
Bosch, Assumpcio
Hearing, Patrick
Chillon, Miguel
Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles
title Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles
title_full Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles
title_fullStr Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles
title_full_unstemmed Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles
title_short Altering the Ad5 Packaging Domain Affects the Maturation of the Ad Particles
title_sort altering the ad5 packaging domain affects the maturation of the ad particles
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3097180/
https://www.ncbi.nlm.nih.gov/pubmed/21611162
http://dx.doi.org/10.1371/journal.pone.0019564
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