The Connection Domain Mutation N348I in HIV-1 Reverse Transcriptase Enhances Resistance to Etravirine and Rilpivirine but Restricts the Emergence of the E138K Resistance Mutation by Diminishing Viral Replication Capacity

Xu, Hongtao; Colby-Germinario, Susan P.; Oliveira, Maureen; Han, Ying-Shan; Quan, Yudong; Zanichelli, Veronica; Wainberg, Mark A.

doi:10.1128/jvi.02904-13

Cited by 16 publications

(14 citation statements)

References 95 publications

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“…When it occurs in combination with other NNRTI resistance-associated amino acid substitutions, such as K103N and Y181C, N348I has been shown to contribute to EFV, ETR, and RPV resistance (59,60). In addition, RPV resistance is enhanced by this substitution in the background of E138K (61). We have confirmed in HIV-1 subtype C that N348I alone does not affect ETR/RPV susceptibility but can significantly reduce ETR and/or RPV susceptibility when it occurs in combination with other NNRTI resistance-associated substitutions, particularly Y181C.…”

Section: Discussionsupporting

confidence: 57%

Impact of Drug Resistance-Associated Amino Acid Changes in HIV-1 Subtype C on Susceptibility to Newer Nonnucleoside Reverse Transcriptase Inhibitors

Basson

Rhee

Parry

et al. 2015

Antimicrob Agents Chemother

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The objective of this study was to assess the phenotypic susceptibility of HIV-1 subtype C isolates, with nonnucleoside reverse transcriptase inhibitor (NNRTI) resistance-associated amino acid changes, to newer NNRTIs. A panel of 52 site-directed mutants and 38 clinically derived HIV-1 subtype C clones was created, and the isolates were assessed for phenotypic susceptibility to etravirine (ETR), rilpivirine (RPV), efavirenz (EFV), and nevirapine (NVP) in an in vitro single-cycle phenotypic assay. The amino acid substitutions E138Q/R, Y181I/V, and M230L conferred high-level resistance to ETR, while K101P and Y181I/V conferred high-level resistance to RPV. Y181C, a major NNRTI resistance-associated amino acid substitution, caused decreased susceptibility to ETR and, to a lesser extent, RPV when combined with other mutations. These included N348I and T369I, amino acid changes in the connection domain that are not generally assessed during resistance testing. However, the prevalence of these genotypes among subtype C sequences was, in most cases, <1%. The more common EFV/NVP resistance-associated substitutions, such as K103N, V106M, and G190A, had no major impact on ETR or RPV susceptibility. The low-level resistance to RPV and ETR conferred by E138K was not significantly enhanced in the presence of M184V/I, unlike for EFV and NVP. Among patient samples, 97% were resistant to EFV and/or NVP, while only 24% and 16% were resistant to ETR and RPV, respectively. Overall, only a few, relatively rare NNRTI resistance-associated amino acid substitutions caused resistance to ETR and/or RPV in an HIV-1 subtype C background, suggesting that these newer NNRTIs would be effective in NVP/EFV-experienced HIV-1 subtype C-infected patients. Highly active antiretroviral therapy (HAART), which comprises the concomitant use of multiple potent antiretroviral drugs, has contributed to a significant decrease in the morbidity and mortality of people infected with HIV-1 (1). The failure of HAART through the acquisition of HIV drug resistance-associated substitutions that cause a decrease in viral susceptibility is usually due to poor adherence and insufficient drug concentrations. Although more than two-thirds of the global HIV-1 infections occur in sub-Saharan African countries, where HIV-1 infections are dominated by non-B subtypes, HAART regimens have largely been developed and tested against HIV-1 subtype B isolates (2). Subtype C accounts for almost half of all global infections and dominates the epidemic in southern Africa (3). While HAART agents are effective against all subtypes (4), greatly aiding the global response to HIV infection, specific resistance mutations and disparities in drug susceptibilities can differ by subtype (5). Examples include the K65R (6) and V106M (7) resistance-associated amino acid substitutions, which develop more frequently under drug pressure in HIV-1 subtype C than subtype B.Nonnucleoside reverse transcriptase (RT) inhibitors (NNRTIs) are a component of most first-line HAART regimens. For efavirenz (EF...

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Section: Discussionsupporting

confidence: 57%

Impact of Drug Resistance-Associated Amino Acid Changes in HIV-1 Subtype C on Susceptibility to Newer Nonnucleoside Reverse Transcriptase Inhibitors

Basson

Rhee

Parry

et al. 2015

Antimicrob Agents Chemother

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“…In contrast, M184I does not result in a defect in the efficiency of polymerization at high dNTP concentrations (29,42), but the simultaneous presence of M184I and E138K can restore the efficiency of processive DNA synthesis and viral replication capacity (29). Another example is the N348I substitution in the connection subdomain of HIV-1 RT, which significantly decreases catalytic efficiency (43) and diminishes polymerization efficiency without impairing enzyme processivity, as demonstrated in gel-based assays (30). To determine whether W153L might affect the efficiency of DNA polymerization, we ran gel-based RNA-dependent DNA polymerase assays at high dNTP concentrations (200 M) in time course experiments using the WT, W153L, W153L/K65R, W153L/M184I, W153L/K101E, W153L/K103N, W153L/E138K, and W153L/Y181C recombinant RT enzymes.…”

Section: Resultsmentioning

confidence: 99%

“…RNase H activity was assayed using a 41-mer 5=-end 32 P-labeled heteropolymeric RNA template termed kim40R that was annealed to a complementary 32-nucleotide DNA oligomer termed kim32D at a 1:4 molar ratio as described previously (29,30). The reactions were conducted at 37°C in mixtures containing an RNA-DNA duplex substrate (20 nM) with equal amounts of RT enzymes in assay buffer (50 mM Tris-HCl, pH 7.8, 60 mM KCl, and 5 mM MgCl 2 ).…”

Section: Methodsmentioning

confidence: 99%

Effects of the W153L Substitution in HIV Reverse Transcriptase on Viral Replication and Drug Resistance to Multiple Categories of Reverse Transcriptase Inhibitors

Colby-Germinario

Oliveira

et al. 2014

Antimicrob Agents Chemother

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A W153L substitution in HIV-1 reverse transcriptase (RT) was recently identified by selection with a novel nucleotide-competing RT inhibitor (NcRTI) termed compound A that is a member of the benzo[4,5]furo[3,2,d]pyrimidin-2-one NcRTI family of drugs.To investigate the impact of W153L, alone or in combination with the clinically relevant RT resistance substitutions K65R (change of Lys to Arg at position 65), M184I, K101E, K103N, E138K, and Y181C, on HIV-1 phenotypic susceptibility, viral replication, and RT enzymatic function, we generated recombinant RT enzymes and viruses containing each of these substitutions or various combinations of them. We found that W153L-containing viruses were impaired in viral replicative capacity and were hypersusceptible to tenofovir (TFV) while retaining susceptibility to most nonnucleoside RT inhibitors. The nucleoside 3TC retained potency against W153L-containing viruses but not when the M184I substitution was also present. W153L was also able to reverse the effects of the K65R substitution on resistance to TFV, and K65R conferred hypersusceptibility to compound A. Biochemical assays demonstrated that W153L alone or in combination with K65R, M184I, K101E, K103N, E138K, and Y181C impaired enzyme processivity and polymerization efficiency but did not diminish RNase H activity, providing mechanistic insights into the low replicative fitness associated with these substitutions. We show that the mechanism of the TFV hypersusceptibility conferred by W153L is mainly due to increased efficiency of TFV-diphosphate incorporation. These results demonstrate that compound A and/or derivatives thereof have the potential to be important antiretroviral agents that may be combined with tenofovir to achieve synergistic results. C urrent standard anti-HIV-1 therapy, termed highly active antiretroviral therapy (HAART), consists of three or more antiretroviral compounds from six distinct classes, including nucleoside reverse transcriptase (RT) inhibitors (NRTIs), nonnucleoside RT inhibitors (NNRTIs), protease inhibitors (PIs), fusion inhibitors, entry inhibitors, and integrase inhibitors (INIs) (for recent reviews, see references 1 and 2). HAART commonly includes two NRTIs in combination with either an NNRTI, a PI, or more recently, an INI (66). HAART has been effective at suppressing HIV-1 replication, partially reversing immunodeficiency, reducing HIV-1-associated complications, and prolonging life (3, 4). However, all antiretrovirals can be compromised by the development of drug resistance (5, 6) that arises from the rapid replication rate of HIV-1 and the error-prone nature of its RT (7, 8). In the absence of an effective vaccine against HIV-1 infection, it is important to develop novel effective antiretrovirals with superior resistance profiles.There are currently 8 approved NRTIs that all compete with natural deoxynucleoside triphosphate (dNTP) substrates to act as DNA chain terminators. In contrast, NNRTIs act allosterically and noncompetitively by inducing conformational changes in RT. The me...

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“…34 The N348I mutation occurred in 11% of viruses in Southern Brazil and it is associated with major resistance to nevirapine, etravirine, and rilpivirine, and as an accessory mutation for thymidine analogs. 40,41,51,52 Of note, A376S has been associated with failure to NNRTI, particularly nevirapine-containing regimens, 53,54 suggesting a functional link between this mutation and K103N.…”

Section: Novel Hiv-1 Rt C-terminal Mutationsmentioning

confidence: 99%

Identification of Novel Resistance-Related Polymorphisms in HIV-1 Subtype C RT Connection and RNase H Domains from Patients Under Virological Failure in Brazil

Barral

Sousa

Santos

et al. 2017

AIDS Research and Human Retroviruses

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Mutations in the connection and RNase H C-terminal reverse transcriptase (RT) domains of HIV-1 have been shown to impact drug resistance to RT inhibitors. However, their impact in the context of non-B subtypes has been poorly assessed. This study aimed to characterize resistance-related mutations in the C-terminal portions of RT in treatment-failing patients from southern Brazil, a region with endemic HIV-1 subtype C (HIV-1C). Viral RNA was isolated and reverse transcribed from 280 infected subjects, and genomic regions were analyzed by polymerase chain reaction, DNA sequencing, and phylogenetic analysis. Two novel mutations, M357R and E529D, were evidenced in Brazilian HIV-1C strains from treatment-failing patients. In global viral isolates of subjects on treatment, M357R was selected in HIV-1C and CRF01_AE and E529D was selected in HIV-1 subtype B (HIV-1B). While most C-terminal RT mutations described for HIV-1B also occur in HIV-1C, this work pinpointed novel mutations that display subtype-specific predominance or occurrence.

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The Connection Domain Mutation N348I in HIV-1 Reverse Transcriptase Enhances Resistance to Etravirine and Rilpivirine but Restricts the Emergence of the E138K Resistance Mutation by Diminishing Viral Replication Capacity

Cited by 16 publications

References 95 publications

Impact of Drug Resistance-Associated Amino Acid Changes in HIV-1 Subtype C on Susceptibility to Newer Nonnucleoside Reverse Transcriptase Inhibitors

Impact of Drug Resistance-Associated Amino Acid Changes in HIV-1 Subtype C on Susceptibility to Newer Nonnucleoside Reverse Transcriptase Inhibitors

Effects of the W153L Substitution in HIV Reverse Transcriptase on Viral Replication and Drug Resistance to Multiple Categories of Reverse Transcriptase Inhibitors

Identification of Novel Resistance-Related Polymorphisms in HIV-1 Subtype C RT Connection and RNase H Domains from Patients Under Virological Failure in Brazil

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