Following cell entry, HIV-1 capsids enter the nucleus by passage through nuclear pores and reach nuclear speckles with subsequent uncoating of the reverse-transcribed genome and its integration into speckle-associated chromatin domains. Here, we characterized the ultrastructure of HIV-1 subviral complexes in nuclei of primary monocyte-derived macrophages and cell lines using live-cell imaging, super-resolution microscopy, and correlative light and electron tomography in the absence and presence of capsid-targeting inhibitors Lenacapavir and PF74. Capsid-like structures containing viral DNA, as well as broken capsids, clustered in nuclear speckles and were displaced from speckles by drug treatment. This was accompanied by alteration of the nuclear capsid structure, with electron-dense protrusions emanating from the narrow end of capsid cones and exposure of integration-competent genomic HIV-1 DNA. Our data indicate that synthesis of genomic dsDNA can be completed inside the closed HIV-1 capsid, and speckle-associated factors could regulate genome uncoating. This may ensure that genome uncoating occurs at optimal sites for integration into transcriptionally active chromatin. The results also shed further light on the mechanism of action of Lenacapavir.
Lenacapavir-induced capsid damage uncovers HIV-1 genomes emanating from nuclear speckles.
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作者:Müller Thorsten G, Klaus Severina, Zila Vojtech, Lucic Bojana, Penzo Carlotta, Nopper Svenja L, Golani Gonen, Anders-Ãsswein Maria, Sonntag-Buck Vera, Heuser Anke-Mareil, Schwarz Ulrich S, Laketa Vibor, Lusic Marina, Müller Barbara, Kräusslich Hans-Georg
| 期刊: | EMBO Journal | 影响因子: | 8.300 |
| 时间: | 2026 | 起止号: | 2026 Jan;45(2):449-470 |
| doi: | 10.1038/s44318-025-00652-5 | ||
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