Changes in Human Immunodeficiency Virus Type 1 Gag at Positions L449 and P453 Are Linked to I50V Protease Mutants In Vivo and Cause Reduction of Sensitivity to Amprenavir and Improved Viral Fitness In Vitro

Maguire, Moira; Guinea, Rosario; Griffin, Philip; MacManus, S.; Elston, Robert C.; Wolfram, Josie; Richards, Naomi; Hanlon, Mary H.; Porter, David; Wrin, Terri; Parkin, Neil; Tisdale, Margaret; Furfine, Eric S.; Petropoulos, C; Snowden, B. Wendy; Kleim, Jörg‐Peter

doi:10.1128/jvi.76.15.7398-7406.2002

Cited by 141 publications

(164 citation statements)

References 49 publications

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“…However, efficient processing at the NC-p2 junction to produce mature NC and p2 is required for FIV infectivity. The processing efficiency of the equivalent HIV-1 NC-p1-p6 cleavage junctions has been extensively examined, and proper temporal cleavage at these sites correlates with viral fitness, replication capacity, and drug resistance (11,40,45,47,49,52). The findings of the current study reinforce the notion that the cleavage and maturation of NC-p2 in FIV and of the equivalent NC-p1-p6 in HIV-1 offer a new potential therapeutic target.…”

Section: Discussionsupporting

confidence: 75%

Generation of Infectious Feline Immunodeficiency Virus (FIV) Encoding FIV/Human Immunodeficiency Virus Chimeric Protease

Lin¹,

Torbett

Elder³

2010

J Virol

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Feline immunodeficiency virus (FIV) and human immunodeficiency virus type 1 (HIV-1) proteases (PRs)share only 23% amino acid identity and exhibit distinct specificities yet have very similar 3-dimensional structures. Chimeric PRs in which HIV residues were substituted in structurally equivalent positions in FIV PR were prepared in order to study the molecular basis of PR specificity. Previous in vitro analyses showed that such substitutions dramatically altered the inhibitor specificity of mutant PRs but changed the rate and specificity of Gag cleavage so that chimeric FIVs were not infectious. Chimeric PRs encoding combinations of the I37V, N55M, M56I, V59I, L97T, I98P, Q99V, and P100N mutations were cloned into FIV Gag-Pol, and those constructs that best approximated the temporal cleavage pattern generated by wild-type FIV PR, while maintaining HIV-like inhibitor specificity, were selected. Two mutations, M56I and L97T, were intolerant to change and caused inefficient cleavage at NC-p2. However, a mutant PR with six substitutions (I37V, N55M, V59I, I98P, Q99V, and P100N) was selected and placed in the context of full-length FIV-34TF10. This virus, termed YCL6, had low-level infectivity ex vivo, and after passage, progeny that exhibited a higher growth rate emerged. The residue at the position of one of the six mutations, I98P, further mutated on passage to either P98H or P98S. Both PRs were sensitive to the HIV-1 PR inhibitors lopinavir (LPV) and darunavir (DRV), as well as to the broad-based inhibitor TL-3, with 50% inhibitory concentrations (IC 50 ) of 30 to 40 nM, consistent with ex vivo results obtained using mutant FIVs. The chimeras offer an infectivity system with which to screen compounds for potential as broad-based PR inhibitors, define structural parameters that dictate specificity, and investigate pathways for drug resistance development.

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Section: Discussionsupporting

confidence: 75%

Generation of Infectious Feline Immunodeficiency Virus (FIV) Encoding FIV/Human Immunodeficiency Virus Chimeric Protease

Lin¹,

Torbett

Elder³

2010

J Virol

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“…Numerous studies supporting the acquisition of fitness-compensatory mutations have been published and recently reviewed by Maisner-Patin and Andersson [1,23]. Among the most clinical relevant reductions in fitness cost associated with antimicrobial resistance include isoniazid-resistant Mycobacterium tuberculosis [33], protease inhibitors-resistant HIV-1 strains [22], azole-resistant Candida albicans [7], and clarythromycin-resistant Helicobacter pylori [4].…”

Section: Discussionmentioning

confidence: 99%

Quantifying the Impact of Bacterial Fitness and Repeated Antimicrobial Exposure on the Emergence of Multidrug-Resistant Gram-Negative Bacilli

D’Agata

Horn

Webb

2007

Math. Model. Nat. Phenom.

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Abstract. The emergence of multidrug resistance among gram-negative bacilli is complex. Numerous factors need to be considered, including the biological fitness cost of resistance, fitnesscompensatory mutations and frequency and type of antibiotic exposure. A mathematical model evaluating these complex relationships was developed in an individual colonized with strains of pan-susceptible, single-, two-and multidrug-resistant (MDR) gram-negative bacilli (GN). The effect of bacterial fitness, compensatory mutations and the frequency of three-antimicrobial regimen exposure to predominance of multidrug-resistant strains were quantified. The model predicts that initially, in the absence of antibiotic exposure, the biologically fitter pan-susceptible strain predominates over the resistant strains. Over time, the fitness of the MDR strains increases faster with repeated antimicrobial exposure, through compensatory-fitness mutations. Increasing the frequency of exposure to the three-antimicrobial regimen or, increasing the initial fitness of the resistant strains, substantially decreases the time to MDR-GN predominance. The model implies that when MDR-GN strains evolve into strains that are fitter than susceptible strains, a reduction in antimicrobial exposure may not result in a decrease of MDR-GN, since the absence of selective antimicrobial pressure would no longer favor susceptible strains. The model also implies that antimicrobial cycling may promote the emergence of MDR-GN.

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“…In an analysis of a clinical sequence database, the L449F and P453L mutations at the p1/p6 cleavage site in Gag were frequently observed in combination with the major protease inhibitor resistance mutation I50V, although the two cleavage site mutations were not observed together in individual clones derived from patient samples (107). These mutations each partially improved the replication fitness of HIV-1 strains containing the I50V mutation and increased the degree of protease inhibitor resistance; no effect on protease inhibitor resistance was seen when these mutations were introduced into a drug-sensitive laboratory strain (107).…”

Section: Extragenic Interactionsmentioning

confidence: 99%

“…These mutations each partially improved the replication fitness of HIV-1 strains containing the I50V mutation and increased the degree of protease inhibitor resistance; no effect on protease inhibitor resistance was seen when these mutations were introduced into a drug-sensitive laboratory strain (107). In the absence of these mutations, the I50V mutant accumulated uncleaved p1/p6 protein; this abnormality was partially corrected by the addition of one of the cleavage site mutations (107). Those studies also confirmed that purified protease containing the I50V mutation cleaved a mutant p1/p6 cleavage site more efficiently than a wild-type cleavage site (107).…”

Section: Extragenic Interactionsmentioning

confidence: 99%

“…In the absence of these mutations, the I50V mutant accumulated uncleaved p1/p6 protein; this abnormality was partially corrected by the addition of one of the cleavage site mutations (107). Those studies also confirmed that purified protease containing the I50V mutation cleaved a mutant p1/p6 cleavage site more efficiently than a wild-type cleavage site (107). Positive and negative associations between specific cleavage site and major protease-inhibitor resistance mutations were also observed in another study of treatment-experienced patients (170).…”

Section: Extragenic Interactionsmentioning

confidence: 99%

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Clinical Significance of Human Immunodeficiency Virus Type 1 Replication Fitness

Dykes

Demeter

2007

Clin Microbiol Rev

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SUMMARY The relative fitness of a variant, according to population genetics theory, is that variant's relative contribution to successive generations. Most drug-resistant human immunodeficiency virus type 1 (HIV-1) variants have reduced replication fitness, but at least some of these deficits can be compensated for by the accumulation of second-site mutations. HIV-1 replication fitness also appears to influence the likelihood of a drug-resistant mutant emerging during treatment failure and is postulated to influence clinical outcomes. A variety of assays are available to measure HIV-1 replication fitness in cell culture; however, there is no agreement regarding which assays best correlate with clinical outcomes. A major limitation is that there is no high-throughput assay that incorporates an internal reference strain as a control and utilizes intact virus isolates. Some retrospective studies have demonstrated statistically significant correlations between HIV-1 replication fitness and clinical outcomes in some patient populations. However, different studies disagree as to which clinical outcomes are most closely associated with fitness. This may be in part due to assay design, sample size limitations, and differences in patient populations. In addition, the strength of the correlations between fitness and clinical outcomes is modest, suggesting that, at present, it would be difficult to utilize these assays for clinical management.

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Changes in Human Immunodeficiency Virus Type 1 Gag at Positions L449 and P453 Are Linked to I50V Protease Mutants In Vivo and Cause Reduction of Sensitivity to Amprenavir and Improved Viral Fitness In Vitro

Cited by 141 publications

References 49 publications

Generation of Infectious Feline Immunodeficiency Virus (FIV) Encoding FIV/Human Immunodeficiency Virus Chimeric Protease

Generation of Infectious Feline Immunodeficiency Virus (FIV) Encoding FIV/Human Immunodeficiency Virus Chimeric Protease

Quantifying the Impact of Bacterial Fitness and Repeated Antimicrobial Exposure on the Emergence of Multidrug-Resistant Gram-Negative Bacilli

Clinical Significance of Human Immunodeficiency Virus Type 1 Replication Fitness

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