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HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells

HIV-1 replication commences inside the cone-shaped viral capsid, but timing, localization, and mechanism of uncoating are under debate. We adapted a strategy to visualize individual reverse-transcribed HIV-1 cDNA molecules and their association with viral and cellular proteins using fluorescence and...

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Autores principales: Müller, Thorsten G, Zila, Vojtech, Peters, Kyra, Schifferdecker, Sandra, Stanic, Mia, Lucic, Bojana, Laketa, Vibor, Lusic, Marina, Müller, Barbara, Kräusslich, Hans-Georg
Formato: Online Artículo Texto
Lenguaje:English
Publicado: eLife Sciences Publications, Ltd 2021
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8169111/
https://www.ncbi.nlm.nih.gov/pubmed/33904396
http://dx.doi.org/10.7554/eLife.64776
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author Müller, Thorsten G
Zila, Vojtech
Peters, Kyra
Schifferdecker, Sandra
Stanic, Mia
Lucic, Bojana
Laketa, Vibor
Lusic, Marina
Müller, Barbara
Kräusslich, Hans-Georg
author_facet Müller, Thorsten G
Zila, Vojtech
Peters, Kyra
Schifferdecker, Sandra
Stanic, Mia
Lucic, Bojana
Laketa, Vibor
Lusic, Marina
Müller, Barbara
Kräusslich, Hans-Georg
author_sort Müller, Thorsten G
collection PubMed
description HIV-1 replication commences inside the cone-shaped viral capsid, but timing, localization, and mechanism of uncoating are under debate. We adapted a strategy to visualize individual reverse-transcribed HIV-1 cDNA molecules and their association with viral and cellular proteins using fluorescence and correlative-light-and-electron-microscopy (CLEM). We specifically detected HIV-1 cDNA inside nuclei, but not in the cytoplasm. Nuclear cDNA initially co-localized with a fluorescent integrase fusion (IN-FP) and the viral CA (capsid) protein, but cDNA-punctae separated from IN-FP/CA over time. This phenotype was conserved in primary HIV-1 target cells, with nuclear HIV-1 complexes exhibiting strong CA-signals in all cell types. CLEM revealed cone-shaped HIV-1 capsid-like structures and apparently broken capsid-remnants at the position of IN-FP signals and elongated chromatin-like structures in the position of viral cDNA punctae lacking IN-FP. Our data argue for nuclear uncoating by physical disruption rather than cooperative disassembly of the CA-lattice, followed by physical separation from the pre-integration complex.
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spelling pubmed-81691112021-06-04 HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells Müller, Thorsten G Zila, Vojtech Peters, Kyra Schifferdecker, Sandra Stanic, Mia Lucic, Bojana Laketa, Vibor Lusic, Marina Müller, Barbara Kräusslich, Hans-Georg eLife Cell Biology HIV-1 replication commences inside the cone-shaped viral capsid, but timing, localization, and mechanism of uncoating are under debate. We adapted a strategy to visualize individual reverse-transcribed HIV-1 cDNA molecules and their association with viral and cellular proteins using fluorescence and correlative-light-and-electron-microscopy (CLEM). We specifically detected HIV-1 cDNA inside nuclei, but not in the cytoplasm. Nuclear cDNA initially co-localized with a fluorescent integrase fusion (IN-FP) and the viral CA (capsid) protein, but cDNA-punctae separated from IN-FP/CA over time. This phenotype was conserved in primary HIV-1 target cells, with nuclear HIV-1 complexes exhibiting strong CA-signals in all cell types. CLEM revealed cone-shaped HIV-1 capsid-like structures and apparently broken capsid-remnants at the position of IN-FP signals and elongated chromatin-like structures in the position of viral cDNA punctae lacking IN-FP. Our data argue for nuclear uncoating by physical disruption rather than cooperative disassembly of the CA-lattice, followed by physical separation from the pre-integration complex. eLife Sciences Publications, Ltd 2021-04-27 /pmc/articles/PMC8169111/ /pubmed/33904396 http://dx.doi.org/10.7554/eLife.64776 Text en © 2021, Müller et al https://creativecommons.org/licenses/by/4.0/This article is distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use and redistribution provided that the original author and source are credited.
spellingShingle Cell Biology
Müller, Thorsten G
Zila, Vojtech
Peters, Kyra
Schifferdecker, Sandra
Stanic, Mia
Lucic, Bojana
Laketa, Vibor
Lusic, Marina
Müller, Barbara
Kräusslich, Hans-Georg
HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells
title HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells
title_full HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells
title_fullStr HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells
title_full_unstemmed HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells
title_short HIV-1 uncoating by release of viral cDNA from capsid-like structures in the nucleus of infected cells
title_sort hiv-1 uncoating by release of viral cdna from capsid-like structures in the nucleus of infected cells
topic Cell Biology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8169111/
https://www.ncbi.nlm.nih.gov/pubmed/33904396
http://dx.doi.org/10.7554/eLife.64776
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