Abstract EN:

During HIV-1 assembly, the viral protein R (Vpr) is incorporated into newly formed viral particles via an interaction with the C-terminal domain of the Gag polyprotein precursor Pr55Gag. Vpr has been implicated in the nuclear import of the viral DNA and subsequently in its transcription. In addition, Vpr can impact on the cell physiology by causing G2/M arrest and apoptosis. The 3D structure of Vpr was solved by NMR and is composed of three amphipathic α helices spanning residues surrounded by flexible N- and Cterminal sequences. Two loops spanning residues allow a mutual orientation of these helices, conferring a globular conformation to the protein and promoting the formation of a hydrophobic core with numerous hydrophobic amino acids scattered throughout Vpr. The goal of this PhD work was focused on the oligomerization properties of Vpr in a cellular environment and to establish the function of this oligomerization in the interaction between Vpr and Pr55Gag during HIV-1 assembly. To address this issue, HeLa cells were transfected with plasmids expressing eGFP- and mCherry-tagged Vpr and Pr55Gag-TC, the latter being visualized by biarsenical labeling reagents (FlAsH/ReAsH). These cells were studied by confocal microscopy, fluorescence lifetime imaging microscopy (FLIM) and fluorescence correlation spectroscopy (FCS). Our results show that Vpr-Vpr interactions take place mostly at or close to the nuclear envelope. This oligomerization and localization require Vpr’s central hydrophobic core. Indeed, point mutations disrupting that core drastically impaired both Vpr-Vpr interactions and Vpr specific localization at the nuclear rim. We further evidence that the Pr55Gag-Vpr complexes, imaged in cellulo, mainly accumulated at the plasma membrane and confirmed the importance of the two Pr55Gag(p6) motifs, 15FXFG18 and 41LXXLF45, for Pr55Gag-Vpr complex formation. We also report that Vpr oligomerization is crucial for Pr55Gag recognition. On the other hand, Pr55Gag-Vpr complexes are still formed when Pr55Gag bears mutations causing a defect in its multimerization. Moreover, when Vpr was co-expressed with Pr55Gag mutants diffusing inside the cytoplasm or present on the contrary in multivesicular structures, Vpr lost its specific location on the plasma membrane and was detected in the same cellular compartments as the Pr55Gag mutants. These findings suggest that Pr55Gag-Vpr recognition is most probably occurring already at their respective site of synthesis and thus seems to be an early step in Pr55Gag assembly.