Abstract
BackgroundThe Gag polyprotein is a multifunctional regulator of retroviral replication and major structural component of immature virions. The nucleic acid chaperone (NAC) activity is considered necessary to retroviral Gag functions, but so far, NAC activity has only been confirmed for HIV-1 and RSV Gag polyproteins. The nucleocapsid (NC) domain of Gag is proposed to be crucial for interactions with nucleic acids and NAC activity. The major function of matrix (MA) domain is targeting and binding of Gag to the plasma membrane but MA can also interact with RNA and influence NAC activity of Gag. Here, we characterize RNA binding properties and NAC activity of HIV-2 MA and Gag, lacking p6 domain (GagΔp6) and discuss potential contribution of NC and MA domains to HIV-2 GagΔp6 functions and interactions with RNA.ResultsWe found that HIV-2 GagΔp6 is a robust nucleic acid chaperone. HIV-2 MA protein promotes nucleic acids aggregation and tRNALys3 annealing in vitro. The NAC activity of HIV-2 NC is affected by salt which is in contrast to HIV-2 GagΔp6 and MA. At a physiological NaCl concentration the tRNALys3 annealing activity of HIV-2 GagΔp6 or MA is higher than HIV-2 NC. The HIV-2 NC and GagΔp6 show strong binding to the packaging signal (Ψ) of HIV-2 RNA and preference for the purine-rich sequences, while MA protein binds mainly to G residues without favouring Ψ RNA. Moreover, HIV-2 GagΔp6 and NC promote HIV-2 RNA dimerization while our data do not support MA domain participation in this process in vitro.ConclusionsWe present that contrary to HIV-1 MA, HIV-2 MA displays NAC activity and we propose that MA domain may enhance the activity of HIV-2 GagΔp6. The role of the MA domain in the NAC activity of Gag may differ significantly between HIV-1 and HIV-2. The HIV-2 NC and MA interactions with RNA are not equivalent. Even though both NC and MA can facilitate tRNALys3 annealing, MA does not participate in RNA dimerization in vitro. Our data on HIV-2 indicate that the role of the MA domain in the NAC activity of Gag differs not only between, but also within, retroviral genera.Electronic supplementary materialThe online version of this article (doi:10.1186/s12977-016-0245-1) contains supplementary material, which is available to authorized users.
Highlights
The Gag polyprotein is a multifunctional regulator of retroviral replication and major structural compo‐ nent of immature virions
The nucleic acid chaperone (NAC) activity of HIV-1 Gag has been shown to depend on the NC domain, which is required for tRNALys3/viral RNA complex formation [14, 16, 17], whereas the MA domain can inhibit this process via RNA binding [17]
We recently reported that HIV-2 NC is an effective NAC, but its activity is limited by the structural stability of the nucleic acid molecule to a much greater degree than that of HIV-1 NC [29]
Summary
The Gag polyprotein is a multifunctional regulator of retroviral replication and major structural compo‐ nent of immature virions. The nucleic acid chaperone (NAC) activity is considered necessary to retroviral Gag func‐ tions, but so far, NAC activity has only been confirmed for HIV-1 and RSV Gag polyproteins. The retroviral Gag polyprotein is a major structural component of immature virions, and acts as multifunctional regulator of virus replication [1,2,3,4]. The NAC activity is considered necessary to anneal tRNALys but, so far, it has only been confirmed for HIV-1 and Rous sarcoma virus (RSV) Gag proteins in vitro [15,16,17,18]. We recently reported that HIV-2 NC is an effective NAC, but its activity is limited by the structural stability of the nucleic acid molecule to a much greater degree than that of HIV-1 NC [29]
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