Abstract
The GagPol protein of HIV-1 harbors viral enzymes, such as protease (PR), reverse transcriptase, and integrase, that are all crucial for virion infectivity. Previous studies have suggested that expression of GagPol alone does not produce viral particles and that the budding defect is caused by the presence of the Pol region. However, it has remained unknown why GagPol fails to produce viral particles. We show here that HIV-1 GagPol is incapable of membrane binding and subsequent particle assembly. Our confocal data indicated that, despite full N-myristoylation, GagPol protein failed to target plasma membrane with diffuse distribution in the cytoplasm. Membrane flotation analysis confirmed these findings. Progressive C-terminal truncation of GagPol to give GagPR allowed for plasma membrane targeting but still not for particle production. Conversely, the C-terminal addition of a noncognate protein, such as ß-galactosidase or 4 tandem GFP, to Gag impaired the membrane affinity, indicating that the Pol region, a large extension to Gag, inhibits membrane binding in the context of GagPol. The addition of the 10 N-terminal amino acids of Fyn kinase [Fyn(10)], a tight membrane-binding signal, conferred plasma membrane targeting on GagPol, but the Fyn(10)GagPol did not produce viral particles. The defect in particle budding was not rescued by the introduction of the PTAP motif, which is responsible for a late stage of viral particle budding. Rather, electron microscopy suggested that the budding defect of GagPR occurred at an early stage of particle morphogenesis. Our data, which were consistent with previous observations, demonstrate the defects of GagPol in membrane binding and particle assembly.
Highlights
The human immunodeficiency virus type 1 (HIV-1) genome contains three major genes, gag, pol, and env, that encode the viral structural protein Gag, enzymatic polyprotein Pol, and envelope protein Env, respectively
To examine the defect of HIV-1 GagPol in particle assembly, we used the PR-inactive version of pNL43 derivatives, in which the gag and pol frames were placed into the same reading frame by deleting the frameshifting signal
HeLa cells were transfected with these GagPol constructs, and their particle production abilities were examined by Western blotting using antiHIV-1 p24 antibody (Fig. 1B)
Summary
The human immunodeficiency virus type 1 (HIV-1) genome contains three major genes, gag, pol, and env, that encode the viral structural protein Gag, enzymatic polyprotein Pol, and envelope protein Env, respectively. The gag gene is translated into a Gag precursor protein that is subsequently cleaved into the p17/matrix (MA), p24/capsid (CA), p7/nucleocapsid (NC), and p6 domains by HIV-1 protease during virion maturation. The Gag protein is a driving force for retroviral particle assembly This process consists of several distinct but mutually interdependent steps, including the membrane targeting and multimerization of Gag as well as the pinching off of budded particles from the membrane. A number of studies indicate that HIV-1 Gag primarily targets the plasma membrane, where particle assembly and budding occur [21,22,23,24,25,26], Gag can initiate assembly in endosomes and be transported to the cell surface [27,28,29,30,31,32,33,34]
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