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

Kwon, Young Do; Chuang, Gwo-Yu; Zhang, Baoshan; Bailer, Robert T.; Doria‐Rose, Nicole A.; Gindin, Tatyana; Lin, Bob C.; Louder, Mark K.; McKee, Krisha; O’Dell, Sijy; Pegu, Amarendra; Schmidt, Stephen D.; Asokan, Mangaiarkarasi; Chen, Xuejun; Choe, Misook; Georgiev, Ivelin S.; Jin, Vivian; Pancera, Marie; Rawi, Reda; Wang, Keyun; Chaudhuri, Rajoshi; Kueltzo, Lisa A.; Manceva, Slobodanka D.; Todd, John-Paul M.; Scorpio, Diana G.; Kim, Mi-Kyung; Reinherz, Ellis L.; Wagh, Kshitij; Korber, Bette; Connors, Mark; Shapiro, Lawrence; Mascola, John R.; Kwong, Peter D.

doi:10.1016/j.celrep.2018.01.023

Cited by 58 publications

(69 citation statements)

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“…In all tested combinations of FL Env and MPER Fab, cryo-EM analysis showed no stable, high-resolution structural features for MPER, TMD or CTD similarly to earlier cryo-EM studies ( Figure 3A) (Lee et al, 2016;Rantalainen et al, 2018;Torrents de la Pena et al, 2019). One of the tested antibodies involved a variant of 10E8, called 10E8v4_5R+100cF, which was designed to have improved membrane-interaction capacity and which showed 10-fold high neutralization potency (Kwon et al, 2018b). This antibody also failed to show stable, high-resolution structural features suggesting that stable lipid headgroup contacts are not fully recovered in this approach.…”

Section: Env-mper Fab Complexes In Detergent-lipid Micelles Show Hetesupporting

confidence: 63%

“…Nevertheless, the system is a step toward more native environment and open new possibilities for studying Env structure in lipid bilayers by single particle EM analysis. In addition to controlled lipid composition and the testing new MPER antibodies such as 10E8v4_5R+100cF with improved lipid contacts (Kwon et al, 2018b), these membrane embedded Envs may allow structural studies of the effect that CD4 receptor engagement has on the neutralization mechanism of the MPER bNAbs, which thus far has not been possible. As these complexes are likely heterogenous, excellent scalability and the classification power of single particle EM analysis becomes an important factor in addition to being able to yield high resolution structural data.…”

Section: Discussionmentioning

confidence: 99%

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HIV-1 Envelope and MPER antibody structures in lipid assemblies

Rantalainen

Berndsen

Antanasijevic

et al. 2019

Preprint

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SummaryStructural and functional studies of HIV Env as a transmembrane protein have long been complicated by challenges associated with inherent flexibility of the molecule and the membrane-embedded hydrophobic regions. Thus, most structural studies have utilized soluble forms where the regions C-terminal to the ectodomain are deleted. Here, we present approaches for incorporating full-length, wild-type HIV-1 Env, as well as C-terminally truncated and stabilized versions, into lipid assemblies, providing a modular platform for Env structural studies by single particle electron microscopy. We reconstituted a full-length Env clone into a nanodisc with MSP1D1 scaffold, complexed it with an MPER targeting antibody 10E8, and structurally defined the full quaternary epitope of 10E8 consisting of lipid, MPER and ectodomain contacts. By aligning this and other Env-MPER antibody complex reconstructions with the lipid bilayer, we observe evidence of Env tilting as part of the neutralization mechanism for MPER-targeting antibodies. We also adapted the platform toward vaccine design purposes by introducing stabilizing mutations that allow purification of unliganded Env with peptidisc scaffold.

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Section: Env-mper Fab Complexes In Detergent-lipid Micelles Show Hetesupporting

confidence: 63%

Section: Discussionmentioning

confidence: 99%

HIV-1 Envelope and MPER antibody structures in lipid assemblies

Rantalainen

Berndsen

Antanasijevic

et al. 2019

Preprint

Self Cite

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“…Variable regions of the RHA1.V2.01 antibody heavy and light chain genes were synthesized (Genscript) and subcloned into the pVRC8400 vector, in which a HRV3C cleavage site was inserted in the heavy-chain hinge region. The heavy and light chain pair was co-transfected in Expi293F cells (Thermo Fisher) using Turbo293 transfection reagent (Speed BioSystems) as described previously (113). The culture supernatant was harvested 6 days post transfection and loaded on a protein A column, the column was washed with PBS, and IgG proteins were eluted with a low pH buffer.…”

Section: Next Generation Sequencing Of Naïve B Cells and Igdiscover Amentioning

confidence: 99%

Recapitulation of HIV-1 Env-Antibody Coevolution in Macaques Leading to Neutralization Breadth

Roark

Williams

et al. 2020

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Neutralizing antibodies elicited by HIV-1 coevolve with viral Envs in distinctive patterns, in some cases acquiring substantial breadth. Here we show that primary HIV-1 Envs, when expressed by simian-human immunodeficiency viruses in rhesus macaques, elicited patterns of Env-antibody coevolution strikingly similar to those in humans. This included conserved immunogenetic, structural and chemical solutions to epitope recognition and precise Env-amino acid substitutions, insertions and deletions leading to virus persistence. The structure of one rhesus antibody, capable of neutralizing 49% of a 208-strain panel, revealed a V2-apex mode of recognition like that of human bNAbs PGT145/PCT64-35M. Another rhesus antibody bound the CD4-binding site by CD4 mimicry mirroring human bNAbs 8ANC131/CH235/VRC01. Virus-antibody coevolution in macaques can thus recapitulate developmental features of human bNAbs, thereby guiding HIV-1 immunogen design.One sentence summaryVirus-antibody coevolution in rhesus macaques recapitulates developmental features of human antibodies.

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“…Infected cell binding of MPER-specific antibodies varied. 10E8v4-V5R-100cF (a version of 10E8 optimized for increased solubility and potency [47]) at 5 g/ml bound to 30 of 35 isolates, with high-level binding (MFI ratios of Ͼ4) observed for 13 of these. However, 10E8 and 10E8v4-V5R-100cF also showed substantial binding to uninfected bystanders (Gag Ϫ population) (see Fig.…”

Section: Virus Neutralization Profiles Of Bnabs and Bnab Combinationsmentioning

confidence: 99%

Susceptibility to Neutralization by Broadly Neutralizing Antibodies Generally Correlates with Infected Cell Binding for a Panel of Clade B HIV Reactivated from Latent Reservoirs

Ren

Korom

Truong

et al. 2018

J Virol

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Efforts to cure human immunodeficiency virus (HIV) infection are obstructed by reservoirs of latently infected CD4 T cells that can reestablish viremia. HIV-specific broadly neutralizing antibodies (bNAbs), defined by unusually wide neutralization breadths against globally diverse viruses, may contribute to the elimination of these reservoirs by binding to reactivated cells, thus targeting them for immune clearance. However, the relationship between neutralization of reservoir isolates and binding to corresponding infected primary CD4 T cells has not been determined. Thus, the extent to which neutralization breadths and potencies can be used to infer the corresponding parameters of infected cell binding is currently unknown. We assessed the breadths and potencies of bNAbs against 36 viruses reactivated from peripheral blood CD4 T cells from antiretroviral (ARV)-treated HIV-infected individuals by using paired neutralization and infected cell binding assays. Single-antibody breadths ranged from 0 to 64% for neutralization (80% inhibitory concentration [IC] of ≤10 μg/ml) and from 0 to 89% for binding, with two-antibody combinations (results for antibody combinations are theoretical/predicted) reaching levels of 0 to 83% and 50 to 100%, respectively. Infected cell binding correlated with virus neutralization for 10 of 14 antibodies (e.g., for 3BNC117, = 0.82 and < 0.0001). Heterogeneity was observed, however, with a lack of significant correlation for 2G12, CAP256.VRC26.25, 2F5, and 4E10. Our results provide guidance on the selection of bNAbs for interventional cure studies, both by providing a direct assessment of intra- and interindividual variabilities in neutralization and infected cell binding in a novel cohort and by defining the relationships between these parameters for a panel of bNAbs. Although antiretroviral therapies have improved the lives of people who are living with HIV, they do not cure infection. Efforts are being directed towards harnessing the immune system to eliminate the virus that persists, potentially resulting in virus-free remission without medication. HIV-specific antibodies hold promise for such therapies owing to their ability to both prevent the infection of new cells (neutralization) and direct the killing of infected cells. We isolated 36 HIV strains from individuals whose virus was suppressed by medication and tested 14 different antibodies for neutralization of these viruses and for binding to cells infected with the same viruses (critical for engaging natural killer cells). For both neutralization and infected cell binding, we observed variation both between individuals and amongst different viruses within an individual. For most antibodies, neutralization activity correlated with infected cell binding. These data provide guidance on the selection of antibodies for clinical trials.

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

Cited by 58 publications

References 50 publications

HIV-1 Envelope and MPER antibody structures in lipid assemblies

HIV-1 Envelope and MPER antibody structures in lipid assemblies

Recapitulation of HIV-1 Env-Antibody Coevolution in Macaques Leading to Neutralization Breadth

Susceptibility to Neutralization by Broadly Neutralizing Antibodies Generally Correlates with Infected Cell Binding for a Panel of Clade B HIV Reactivated from Latent Reservoirs

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