Welcome to the new version of CaltechAUTHORS. Login is currently restricted to library staff. If you notice any issues, please email coda@library.caltech.edu
CaltechAUTHORS
Published May 5, 2020 | Published + Supplemental Material
Journal Article Open

Structural basis for Zika envelope domain III recognition by a germline version of a recurrent neutralizing antibody

Esswein, Shannon R. ORCID icon
Gristick, Harry B. ORCID icon
Jurado, Andrea ORCID icon
Peace, Avery ORCID icon
Keeffe, Jennifer R. ORCID icon
Lee, Yu E.
Voll, Alisa V.
Saeed, Mohsan ORCID icon
Nussenzweig, Michel C. ORCID icon
Rice, Charles M. ORCID icon
Robbiani, Davide F. ORCID icon
MacDonald, Margaret R. ORCID icon
Bjorkman, Pamela J. ORCID icon

Abstract

Recent epidemics demonstrate the global threat of Zika virus (ZIKV), a flavivirus transmitted by mosquitoes. Although infection is usually asymptomatic or mild, newborns of infected mothers can display severe symptoms, including neurodevelopmental abnormalities and microcephaly. Given the large-scale spread, symptom severity, and lack of treatment or prophylaxis, a safe and effective ZIKV vaccine is urgently needed. However, vaccine design is complicated by concern that elicited antibodies (Abs) may cross-react with other flaviviruses that share a similar envelope protein, such as dengue virus, West Nile virus, and yellow fever virus. This cross-reactivity may worsen symptoms of a subsequent infection through Ab-dependent enhancement. To better understand the neutralizing Ab response and risk of Ab-dependent enhancement, further information on germline Ab binding to ZIKV and the maturation process that gives rise to potently neutralizing Abs is needed. Here we use binding and structural studies to compare mature and inferred-germline Ab binding to envelope protein domain III of ZIKV and other flaviviruses. We show that affinity maturation of the light-chain variable domain is important for strong binding of the recurrent VH3-23/VK1-5 neutralizing Abs to ZIKV envelope protein domain III, and identify interacting residues that contribute to weak, cross-reactive binding to West Nile virus. These findings provide insight into the affinity maturation process and potential cross-reactivity of VH3-23/VK1-5 neutralizing Abs, informing precautions for protein-based vaccines designed to elicit germline versions of neutralizing Abs.

Additional Information

© 2020 National Academy of Sciences. Published under the PNAS license. Edited by Stephen C. Harrison, Boston Children's Hospital, Boston, MA, and approved March 23, 2020 (received for review November 3, 2019). PNAS first published April 22, 2020. We thank Dr. Jost Vielmetter at the Caltech Protein Expression Center funded by the Beckman Institute at the California Institute of Technology for protein expression and surface plasmon resonance instrument usage; Dr. Jens Kaiser at the California Institute of Technology Molecular Observatory for assistance with X-ray data collection; Dr. Anthony West for discussions regarding germline gene assignments; Alex Cohen for suggestions on EDIII production; Dr. Christopher Barnes for coordinating Advanced Photon Source (APS) beamline collection and beamline scientists at Stanford Synchrotron Radiation Lightsource and APS GM/CA 23-ID-D; and Dr. Ted Pierson for providing pDENV1/WP/CprME and pDENV2/16681/CprME plasmids. The California Institute of Technology Molecular Observatory is supported by the Gordon and Betty Moore Foundation, the Beckman Institute, and the Sanofi-Aventis Bioengineering Research Program. Operations at Stanford Synchrotron Radiation Lightsource are supported by the US Department of Energy and NIH. Operations at APS are supported by US Department of Energy. This work was supported by NIH Grant P01AI138938 (to D.F.R., C.M.R., M.C.N., P.J.B.); NIH Training Grant 5-T32-GM007616-40 (to S.R.E.); NIH National Research Service Award Fellowship F30AI147579 (to S.R.E.); and NIH National Institute of General Medical Sciences Training Grant T32-GM008042 (to S.R.E.) through the University of California, Los Angeles–California Institute of Technology Medical Scientist Training Program. Data Availability: Crystallographic coordinates for structures Z004_(iGL) Fab–ZIKV EDIII and Z032_(mature) Fab–WNV EDIII are available from the Protein Data Bank under ID codes 6UTA and 6UTE. Author contributions: S.R.E., J.R.K., M.R.M., and P.J.B. designed research; S.R.E., H.B.G., A.J., A.P., Y.E.L., and A.V.V. performed research; S.R.E., Y.E.L., M.S., M.C.N., C.M.R., and D.F.R. contributed new reagents/analytic tools; S.R.E., J.R.K., D.F.R., M.R.M., and P.J.B. analyzed data; and S.R.E. and P.J.B. wrote the paper. Competing interest statement: D.F.R., M.C.N., and The Rockefeller University have filed a patent application for antibody Z004. This article is a PNAS Direct Submission. Data deposition: The atomic coordinates and structure factors have been deposited in the Protein Data Bank, www.pdb.org (PDB ID codes 6UTA and 6UTE). This article contains supporting information online at https://www.pnas.org/lookup/suppl/doi:10.1073/pnas.1919269117/-/DCSupplemental.

Attached Files

Published - 9865.full.pdf

Supplemental Material - pnas.1919269117.sapp.pdf

Files

pnas.1919269117.sapp.pdf
Files (53.1 MB)
Name Size Download all
md5:1dcd1557331d18952fa0c5e668c59c9c
50.3 MB Preview Download
md5:68e9e9d2634fcc049113f569f4806fbe
2.8 MB Preview Download

Additional details

Identifiers Funding Dates Caltech Custom Metadata
Created:
August 22, 2023
Modified:
December 22, 2023