Structure and Recognition of a Novel HIV-1 gp120-gp41 Interface Antibody that Caused MPER Exposure through Viral Escape

Wibmer, Constantinos Kurt; Gorman, Jason; Ozorowski, Gabriel; Sheward, Daniel J.; Elliott, Debra; Rouelle, Julie A.; Smira, Ashley; Joyce, Michael; Ndabambi, Nonkululeko; Druz, Aliaksandr; Asokan, Mangaiarkarasi; Burton, Dennis R.; Connors, Mark; Karim, Salim Safurdeen. Abdool; Mascola, John R.; Robinson, James E.; Ward, Andrew B.; Williamson, Carolyn; Kwong, Peter D.; Morris, Lynn; Moore, Penny L.

doi:10.1371/journal.ppat.1006074

Cited by 36 publications

(38 citation statements)

References 87 publications

(98 reference statements)

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“…This bnAb has been extensively studied, using both structural (Blattner et al, 2014; Lee et al, 2016) and functional approaches (Falkowska et al, 2014; Van Gils et al, 2016; Kong et al, 2016; Wibmer et al, 2017). …”

Section: Resultsmentioning

confidence: 99%

“…These sites include residues originally mapped by mutagenesis and pseudovirus-neutralization assays: the dominantly targeted 611 glycan, the 637 glycan, and residue 647 (Figure 2B, 2C) (Falkowska et al, 2014). There was also strong differential selection at fusion-peptide sites 512 and 514, which have been mapped as part of the PGT151 epitope by structural (Lee et al, 2016) and functional (Van Gils et al, 2016; Kong et al, 2016; Wibmer et al, 2017) methods (Figure 2C). Therefore, our mutational antigenic profiling identified strong selection at epitope sites that have been identified by other approaches.…”

Section: Resultsmentioning

confidence: 99%

“…For instance, such studies mostly restrict themselves to alanine mutations at surface sites, making them biased towards certain types of escape mutations. Therefore, despite the fact that PGT151 has been a subject of multiple studies using diverse techniques (Blattner et al, 2014; Falkowska et al, 2014; Van Gils et al, 2016; Kong et al, 2016; Lee et al, 2016; Wibmer et al, 2017), our mutational antigenic profiling has yielded a far more comprehensive and unbiased map of viral escape than all this previous work.…”

Section: Discussionmentioning

confidence: 99%

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Comprehensive Mapping of HIV-1 Escape from a Broadly Neutralizing Antibody

Dingens

Haddox

Overbaugh

et al. 2017

Cell Host & Microbe

112

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Summary Precisely defining how viral mutations affect HIV’s sensitivity to antibodies is vital to develop and evaluate vaccines and antibody immunotherapeutics. Despite great effort, a full map of escape mutants has not been delineated for an anti-HIV antibody. We describe a massively parallel experimental approach to quantify how all single amino-acid mutations to HIV Envelope (Env) affect neutralizing antibody sensitivity in the context of replication-competent virus. We apply this approach to PGT151, a broadly neutralizing antibody recognizing a combination of Env residues and glycans. We confirm sites previously defined by structural and functional studies and reveal additional sites of escape, such as positively charged mutations in the antibody-Env interface. Evaluating the effect of each amino acid at each site lends insight into biochemical mechanisms of escape throughout the epitope, highlighting roles for charge-charge repulsions. Thus, comprehensively mapping HIV antibody escape gives a quantitative, mutation-level view of Env evasion of neutralization.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

See 1 more Smart Citation

Comprehensive Mapping of HIV-1 Escape from a Broadly Neutralizing Antibody

Dingens

Haddox

Overbaugh

et al. 2017

Cell Host & Microbe

112

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“…In addition to 4E10, a number of other HIV-1 broadly neutralizing antibodies have been proposed to interact with viral membrane, including antibodies 2F5 (Ofek et al, 2004), CAP248-2B (Wibmer et al, 2017), and DH511 (Williams et al, 2017) (Figure 5C). As polyreactivity, such as indicated by binding to HEp2 cells or to cardiolipin, can negatively impact the therapeutic efficacy of these antibodies, we assessed the polyreactivity of six membrane-interacting HIV-1 broadly neutralizing antibodies and of Trp-enhanced functional variants for four of the antibodies (Figure 5D; Figure S3).…”

Section: Resultsmentioning

confidence: 99%

Surface-Matrix Screening Identifies Semi-specific Interactions that Improve Potency of a Near Pan-reactive HIV-1-Neutralizing Antibody

et al. 2018

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SUMMARY Highly effective HIV-1-neutralizing antibodies could have utility in the prevention or treatment of HIV-1 infection. To improve the potency of 10E8, an antibody capable of near pan-HIV-1 neutralization, we engineered 10E8-surface mutants and screened for improved neutralization. Variants with the largest functional enhancements involved the addition of hydrophobic or positively charged residues, which were positioned to interact with viral membrane lipids or viral glycan-sialic acids, respectively. In both cases, the site of improvement was spatially separated from the region of antibody mediating molecular contact with the protein component of the antigen, thereby improving peripheral semi-specific interactions while maintaining unmodified dominant contacts responsible for broad recognition. The optimized 10E8 antibody, with mutations to phenylalanine and arginine, retained the extraordinary breadth of 10E8 but with ~10-fold increased potency. We propose surface-matrix screening as a general method to improve antibodies, with improved semi-specific interactions between antibody and antigen enabling increased potency without compromising breadth.

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“…Glycan arrays have been developed to study the glycan-binding profiles of antibodies and have proven to be particularly useful in determining the types of glycan structures that are bound by HIV-1 bNAbs [10, 11, 18–25] . In addition, the anti-glycan antibody responses in sera of non-human primates after Ad5hr-SIV vaccination and SIV infection [26] and HIV vaccine responses in rabbits have been assayed on arrays [20, 27, 28] .…”

Section: Introductionmentioning

confidence: 99%

Serum glycan-binding IgG antibodies in HIV-1 infection and during the development of broadly neutralizing responses

Scheepers

Chowdhury

Wright

et al. 2017

Aids

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Background The HIV-1 envelope is covered with glycans that provide structural integrity and protect conserved regions from host antibody responses. However, these glycans are often the target of broadly neutralizing antibodies (bNAbs) that emerge in some HIV infected individuals. We aimed to determine whether anti-glycan IgG antibodies are a general response to HIV-1 infection or specific to individuals who develop bNAbs. Methods IgG binding to glycans was assessed using arrays that contained 245 unique components including N-linked carbohydrates, glycolipids and Tn-peptides. Sera from 20 HIV negative and 27 HIV positive women (including 12 individuals who developed bNAbs) were profiled longitudinally. HIV-1 gp120 proteins were used to compete for binding to the array. Results Anti-glycan IgG antibodies fluctuated over a three-year period irrespective of HIV infection. However, HIV positive individuals had elevated binding to 40 components on the array that included Man8, Man9, Tn-peptides, heat shock protein and glycolipids. Competition experiments confirmed that a proportion of these glycan-binding IgG antibodies were HIV-1 specific, some of which were higher in individuals who developed bNAbs. Conclusions HIV-1 infection is associated with elevated levels of IgG antibodies to specific glycans. Furthermore, some anti-glycan IgG antibodies were more abundant in individuals with bNAbs, suggesting a unique phenotype that may be informative for HIV vaccine design.

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Structure and Recognition of a Novel HIV-1 gp120-gp41 Interface Antibody that Caused MPER Exposure through Viral Escape

Cited by 36 publications

References 87 publications

Comprehensive Mapping of HIV-1 Escape from a Broadly Neutralizing Antibody

Comprehensive Mapping of HIV-1 Escape from a Broadly Neutralizing Antibody

Surface-Matrix Screening Identifies Semi-specific Interactions that Improve Potency of a Near Pan-reactive HIV-1-Neutralizing Antibody

Serum glycan-binding IgG antibodies in HIV-1 infection and during the development of broadly neutralizing responses

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