Mutations in the HIV-1 envelope glycoprotein can broadly rescue blocks at multiple steps in the virus replication cycle

Duyne, Rachel Van; Kuo, Lili; Pham, Phuong Ngoc; Fujii, Ken; Freed, Eric O.

doi:10.1073/pnas.1820333116

Cited by 44 publications

(93 citation statements)

References 100 publications

(113 reference statements)

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“…Interestingly, dominant non-synonymous mutations in env were observed in both selection groups (A541V, Q550H, and S144R in the Nelfinavir selection group, and N302Y, D547G, and Q550H in the PAV206 selection group in Fig 7A, B). One of these mutations, A541V (observed at Nelfinavir P29 in Fig 7A, B) was recently shown to confer broad escape from defects in virus replication defects caused by either virus mutations or antiretroviral drugs, most likely by increasing cell-to-cell transmission in T cell lines (45). The other dominant non-synonymous env mutations observed in our two selection groups are likely to also be in this general category.…”

Section: Resultsmentioning

confidence: 99%

“…Additionally, a second set of mutations was observed in PAV206 and Nelfinavir. These mutations were in env , are not drug-specific, and have been shown to confer global replication advantage most likely by increasing cell-to-cell transmission in T cell lines (45). The modest resistance observed in the PAV206 selection experiment (allowing virus replication in a PAV206 concentration 8X higher than the EC50) is likely explained by non-dominant cyclophilin A binding loop polymorphisms and the env mutations that may have been emerging.…”

Section: Discussionmentioning

confidence: 99%

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Identification of an antiretroviral small molecule that appears to be a host-targeting inhibitor of HIV-1 assembly

Reed

Solas²,

Kitaygorodskyy³

et al. 2020

Preprint

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Given the projected increase in multidrug resistant HIV-1, there is an urgent need for development of antiretrovirals that act on virus life-cycle stages that are not targeted by antiretrovirals currently in use. Host-targeting drugs are of particular interest because they can offer a high barrier to resistance. Here we report identification of two related small molecules that inhibit HIV-1 late events, a stage of the HIV-1 life cycle for which potent and specific inhibitors are lacking. This chemotype was discovered using cell-free protein synthesis and assembly systems that recapitulate intracellular host-catalyzed viral capsid assembly pathways. These compounds inhibit replication of HIV-1 in human T cell lines and PBMCs and are effective against a primary isolate. They reduce virus production, likely by inhibiting a post-translational step in HIV-1 Gag assembly. Notably, the compound colocalizes with HIV-1 Gag in situ; however, unexpectedly, selection experiments failed to identify compound-specific resistance mutations in gag or pol, even though known resistance mutations developed in a parallel nelfinavir selection. Thus, we hypothesized that instead of binding to Gag directly, these compounds might localize to assembly intermediates, the intracellular multiprotein complexes containing Gag and host factors that are formed during immature HIV-1 capsid assembly. Indeed, imaging of infected cells showed colocalization of the compound with two host enzymes found in assembly intermediates, ABCE1 and DDX6. While the exact target and mechanism of action of this chemotype remain to be determined, these findings suggest that these compounds represent first-in-class, host-targeting inhibitors of intracellular events in HIV-1 assembly.IMPORTANCEThe success of antiretroviral treatment for HIV-1 is at risk of being undermined by the growing problem of drug resistance. Thus, there is a need to identify antiretrovirals that act on viral life cycle stages not targeted by drugs in use, such as the events of HIV-1 Gag assembly. To address this gap, we developed a compound screen that recapitulates the intracellular events of HIV-1 assembly, including viral-host interactions that promote assembly. This effort led to identification of a new chemotype that inhibits HIV-1 replication at nanomolar concentrations by inhibiting virus production. This compound colocalized with Gag and two host enzymes that facilitate capsid assembly but resistance selection did not result in compound-specific mutations in gag, suggesting that the chemotype does not directly target Gag. We hypothesize that this chemotype may represent a first-in-class inhibitor of virus production that acts by targeting a viral-host complex important for HIV-1 Gag assembly.

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Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Identification of an antiretroviral small molecule that appears to be a host-targeting inhibitor of HIV-1 assembly

Reed

Solas²,

Kitaygorodskyy³

et al. 2020

Preprint

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“…Other changes outside of the IN coding region, including the HIV-1 env gene, can confer resistance to DTG (150). HIV-1 can infect cells through fusing directly with the cellular plasma membrane or through the virological synapse that forms between an infected cell and an uninfected cell (151) (reviewed in Ref.…”

Section: Mechanisms Of Hiv Resistance To Instismentioning

confidence: 99%

Multifaceted HIV integrase functionalities and therapeutic strategies for their inhibition

Engelman

2019

Journal of Biological Chemistry

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Figure 3. Retroviral intasome structures. A-C, representative intasomes from the spumavirus PFV (A; protein database (PDB) accession code 3OY9), ␤-retrovirus MMTV (B; PDB code 3JCA), and lentivirus MVV (C; PDB code 5M0Q) are color-coded to highlight the CIC. Green and blue, catalytically active IN protomers; cyan, supporting IN CCDs; black, DNA strands. Whereas four PFV IN molecules suffice to form the CIC, both MMTV and MVV require six IN protomers. For MMTV, critical CTDs (magenta) are donated by flanking IN dimers, leading to an overall IN octamer. In MVV, flanking IN tetramers provide the critical CTDs, resulting in an overall IN hexadecamer. Gray coloring in B and C deemphasizes IN elements that do not compose the CIC. D-F, resected CCD and CTD domains from above green IN protomers, oriented to highlight the different CCD-CTD linker regions (dark gray). Associated magenta CTDs from separate IN protomers in E and F assume similar positions as the green CTD in D. Red sticks, DDE catalytic triad residues. JBC REVIEWS: HIV integrase mechanisms and inhibition 15140 Figure 4. INSTI structures and ALLINI chemotypes. A, diagrams of the four FDA-licensed INSTIs as well as investigational second-generation compound 6p (113, 119). B, representative ALLINI chemotypes. Asterisks mark common positions of t-butoxyacid moieties. JBC REVIEWS: HIV integrase mechanisms and inhibition 15142

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“…The HIV-1 envelope (Env) has been reported in two studies to impact PI susceptibility (18,19), with a number of reports of diverse env sequence changes during PI failure (20,21). Gag is highly polymorphic across HIV-1 subtypes, and existing literature reports diverse mutations occurring both within and outside cleavage sites following treatment with older PI such as indinavir, saquinavir and nelfinavir in subtype B infections (14,(20)(21)(22)(23)(24).…”

Section: Introductionmentioning

confidence: 99%

In Vivo Emergence of a Novel Protease Inhibitor Resistance Signature in HIV-1 Matrix

Datir

Kemp

Bouzidi

et al. 2019

Preprint

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Background: Protease Inhibitors (PIs) are the second-and last-line therapy for the majority of HIV-infected patients worldwide. Only around 20% of individuals who fail PI regimens develop major resistance mutations in protease. We sought to explore the role of mutations in gag-protease genotypic and phenotypic changes within six Nigerian patients who failed PI-based regimens without known drug resistance associated protease mutations in order to identify novel determinants of PI resistance.Methods: Target enrichment and NGS by Illumina Miseq were followed by haplotype reconstruction. Full length gag-protease regions were amplified from baseline (pre-PI) and virologic failure (VF) samples, sequenced and used to construct gag/protease pseudotyped viruses. Phylogenetic analysis was performed using maximum likelihood methods.Susceptibility to lopinavir (LPV) and darunavir (DRV) were measured using a single-cycle replication assay. Western blotting was used to analyse Gag cleavage.Results: In one of six participants (subtype CRF02_AG) we found 4-fold lower LPV susceptibility in viral clones during failure of second line treatment. A combination of four mutations (S126del, H127del, T122A and G123E) in p17 matrix of baseline virus generated a similar 4x decrease in susceptibility to LPV but not darunavir. These four amino acid changes were also able to confer LPV resistance to a subtype B gag-protease backbone. Western blotting did not demonstrate significant Gag cleavage differences between sensitive and resistant isolates. Resistant viruses had around 2-fold lower infectivity compared to sensitive clones in the absence of drug. NGS combined with haplotype reconstruction revealed resistant, less fit clones emerged from a minority population at baseline and thereafter persisted alongside sensitive fitter viruses. Conclusions:We have used a multi-pronged genotypic and phenotypic approach to document emergence and temporal dynamics of a novel protease inhibitor resistance signature in p17 matrix, revealing the interplay between Gag associated resistance and fitness.

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Mutations in the HIV-1 envelope glycoprotein can broadly rescue blocks at multiple steps in the virus replication cycle

Cited by 44 publications

References 100 publications

Identification of an antiretroviral small molecule that appears to be a host-targeting inhibitor of HIV-1 assembly

Identification of an antiretroviral small molecule that appears to be a host-targeting inhibitor of HIV-1 assembly

Multifaceted HIV integrase functionalities and therapeutic strategies for their inhibition

In Vivo Emergence of a Novel Protease Inhibitor Resistance Signature in HIV-1 Matrix

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