Selective packaging of HIV-1 RNA genome is guided by the stability of 5′ untranslated region polyA stem

This review is an accompaniment to a Special Issue on “Retroviral RNA Processing”. It discusses post-transcriptional regulation of retroviruses, ranging from the ancient foamy viruses to more modern viruses, such as HIV-1, HTLV-1, Rous sarcoma virus, murine leukemia virus, mouse mammary tumor virus, and Mason-Pfizer monkey virus. This review is not comprehensive. However, it tries to address some of the major questions in the field with examples of how different retroviruses express their genes. It is amazing that a single primary RNA transcript can have so many possible fates: genomic RNA, unspliced mRNA, and up to 50 different alternatively spliced mRNAs. This review will discuss the sorting of RNAs for packaging or translation, RNA nuclear export mechanisms, splicing, translation, RNA modifications, and avoidance of nonsense-mediated RNA decay.

Section: Viral Rna Must Choose Between Packaging and Translation (Or ...mentioning

confidence: 99%

Section: Splicingmentioning

confidence: 99%

Retroviral RNA Processing

Beemon¹

2022

“…As discussed above, cell-based experiments have documented HIV TMG-cap engages NCBP3/CBP80 heterodimer for translation in a Rev/RRE-dependent manner [ 20 ]. Taken together, in-cellulo data, in-solution analyses and in silico modeling converge on the hypothesis that TSS heterogeneity modulates HIV translation control, as well as the short- and long-range interactions in the HIV 5′ UTR that regulate genome dimerization and packaging [ 68 , 175 , 176 ]. Future studies are warranted to document the TSS of the TMG-capped RNA.…”

Section: Issues Experimental Questions Closingmentioning

confidence: 84%

“…Analysis of the HIV-1 TSS initially identified guanosine-guanosine as the primary sequence at the 5′ end of HIV-1 in lymphocytes [ 65 , 66 , 67 ]. Recently, an adenosine at the HIV TSS was detected infrequently [ 68 ]. Thus, PCIF1 improbably contributes to HIV evasion of innate immune suppression directly [ 69 ].…”

Section: Hiv Precursor Rnas Enter Mutually Exclusive Rna-fate Pathway...mentioning

confidence: 99%

Anomalous HIV-1 RNA, How Cap-Methylation Segregates Viral Transcripts by Form and Function

Boris‐Lawrie

Singh

Osmer

et al. 2022

The acquisition of m7G-cap-binding proteins is now recognized as a major variable driving the form and function of host RNAs. This manuscript compares the 5′-cap-RNA binding proteins that engage HIV-1 precursor RNAs, host mRNAs, small nuclear (sn)- and small nucleolar (sno) RNAs and sort into disparate RNA-fate pathways. Before completion of the transcription cycle, the transcription start site of nascent class II RNAs is appended to a non-templated guanosine that is methylated (m7G-cap) and bound by hetero-dimeric CBP80-CBP20 cap binding complex (CBC). The CBC is a nexus for the co-transcriptional processing of precursor RNAs to mRNAs and the snRNA and snoRNA of spliceosomal and ribosomal ribonucleoproteins (RNPs). Just as sn/sno-RNAs experience hyper-methylation of m7G-cap to trimethylguanosine (TMG)-cap, so do select HIV RNAs and an emerging cohort of mRNAs. TMG-cap is blocked from Watson:Crick base pairing and disqualified from participating in secondary structure. The HIV TMG-cap has been shown to license select viral transcripts for specialized cap-dependent translation initiation without eIF4E that is dependent upon CBP80/NCBP3. The exceptional activity of HIV precursor RNAs secures their access to maturation pathways of sn/snoRNAs, canonical and non-canonical host mRNAs in proper stoichiometry to execute the retroviral replication cycle.

“…The catalytically inactive dimeric pS207–LysRS/tRNA complex is then recruited to sites of viral assembly via interactions with HIV-1 Gag [ 5 , 48 ]. The 5′UTR can adopt various monomeric and dimeric conformations, including a “kissing loop” dimer [ 49 , 50 , 51 , 52 , 53 , 54 ] ( Figure 6 , Step 2). The anticodon-like TLE of an HIV-1 gRNA dimer then competes for binding to pS207–LysRS resulting in an increase in dynamics of the gRNA in this region and release of the tRNA primer proximal to the PBS ( Figure 6 , Step 3).…”

Section: Discussionmentioning

confidence: 99%

Phosphomimetic S207D Lysyl–tRNA Synthetase Binds HIV-1 5′UTR in an Open Conformation and Increases RNA Dynamics

Cantara

Pathirage

Hatterschide

et al. 2022

Self Cite

Interactions between lysyl–tRNA synthetase (LysRS) and HIV-1 Gag facilitate selective packaging of the HIV-1 reverse transcription primer, tRNALys3. During HIV-1 infection, LysRS is phosphorylated at S207, released from a multi-aminoacyl–tRNA synthetase complex and packaged into progeny virions. LysRS is critical for proper targeting of tRNALys3 to the primer-binding site (PBS) by specifically binding a PBS-adjacent tRNA-like element (TLE), which promotes release of the tRNA proximal to the PBS. However, whether LysRS phosphorylation plays a role in this process remains unknown. Here, we used a combination of binding assays, RNA chemical probing, and small-angle X-ray scattering to show that both wild-type (WT) and a phosphomimetic S207D LysRS mutant bind similarly to the HIV-1 genomic RNA (gRNA) 5′UTR via direct interactions with the TLE and stem loop 1 (SL1) and have a modest preference for binding dimeric gRNA. Unlike WT, S207D LysRS bound in an open conformation and increased the dynamics of both the PBS region and SL1. A new working model is proposed wherein a dimeric phosphorylated LysRS/tRNA complex binds to a gRNA dimer to facilitate tRNA primer release and placement onto the PBS. Future anti-viral strategies that prevent this host factor-gRNA interaction are envisioned.