TY - JOUR
T1 - Human Monoclonal Antibodies against NS1 Protein Protect against Lethal West Nile Virus Infection
AU - Wessel, Alex W.
AU - Doyle, Michael P.
AU - Engdahl, Taylor B.
AU - Rodriguez, Jessica
AU - Crowe, James E.
AU - Diamond, Michael S.
N1 - Funding Information:
This study was supported by NIH grant no. R01 AI073755 and 75N93019C00062 and contract no. HHSN272201400058C and HHSN272201700060C. A.W.W. was supported by an NIH predoctoral training grant award (T32 5T32AI007172-38) and the Medical Scientist Training Program. T.C.P. was supported by the Intramural Program of NIAID.
Funding Information:
This study was supported by NIH grant no. R01 AI073755 and 75N93019C00062 and contract no. HHSN272201400058C and HHSN272201700060C. A.W.W. was supported by an NIH predoctoral training grant award (T32 5T32AI007172-38) and the Medical Scientist Training Program. T.C.P. was supported by the Intramural Program of NIAID. We thank Rachel Nargi, Rachel Sutton, Erica Armstrong, and Robert Carnahan of Vanderbilt for help with preparation of recombinant human antibodies and Robin Bombardi, Joe Reidy, and Andrew Trivette of Vanderbilt for sequence analysis support. We also thank Wendy Chung, Dallas County Health and Human Services, for assistance with distributing information about the study in Dallas County, TX. A.W.W. performed epitope mapping, ELISA, flow cytometry, and animal studies. M.P.D. performed NS1 hybridoma screening and BLI competition studies. M.P.D. and T.B.E. generated the human anti-NS1 MAbs. M.P.D. and J.R. performed recombinant antibody generation. A.W.W. performed data analysis. J.E.C. oversaw the human subject work. J.E.C. and M.S.D. acquired resources and directed the project. A.W.W. and M.S.D. wrote the initial manuscript draft. All other authors provided editorial comments. M.S.D. is a consultant for Inbios, Vir Biotechnology, and Carnival Corporation and is on the Scientific Advisory Board of Moderna and Immunome. The Diamond laboratory has received unrelated funding support in sponsored research agreements from Moderna, Vir Biotechnology, and Emergent BioSolutions. J.E.C. has served as a consultant for Luna Biologics, is a member of the Scientific Advisory Board of Meissa Vaccines, and is Founder of IDBiologics. The Crowe laboratory has received unrelated funding support in sponsored research agreements from IDBiologics, Astra Zeneca, and Takeda. All other authors declare no competing interests.
Publisher Copyright:
Copyright © 2021 Wessel et al.
PY - 2021/10/1
Y1 - 2021/10/1
N2 - Envelope protein-targeted vaccines for flaviviruses are limited by concerns of antibody-dependent enhancement (ADE) of infections. Nonstructural protein 1 (NS1) provides an alternative vaccine target that avoids this risk since this protein is absent from the virion. Beyond its intracellular role in virus replication, extracellular forms of NS1 function in immune modulation and are recognized by host-derived antibodies. The rational design of NS1-based vaccines requires an extensive understanding of the antigenic sites on NS1, especially those targeted by protective antibodies. Here, we isolated human monoclonal antibodies (MAbs) from individuals previously naturally infected with WNV, mapped their epitopes using structure-guided mutagenesis, and evaluated their efficacy in vivo against lethal WNV challenge. The most protective epitopes clustered at three antigenic sites that are exposed on cell surface forms of NS1: (i) the wing flexible loop, (ii) the outer, electrostatic surface of the wing, and (iii) the spaghetti loop face of the b-ladder. One additional MAb mapped to the distal tip of the b-ladder and conferred a lower level of protection against WNV despite not binding to NS1 on the surface of infected cells. Our study defines the epitopes and modes of binding of protective anti-NS1 MAb antibodies following WNV infection, which may inform the development of NS1-based countermeasures against flaviviruses. IMPORTANCE Therapeutic antibodies against flaviviruses often promote neutralization by targeting the envelope protein of the virion. However, this approach is hindered by a possible concern for antibody-dependent enhancement of infection and paradoxical worsening of disease. As an alternative strategy, antibodies targeting flavivirus nonstructural protein 1 (NS1), which is absent from the virion, can protect against disease and do not cause enhanced infection. Here, we evaluate the structure-function relationships and protective activity of West Nile virus (WNV) NS1-specific monoclonal antibodies (MAbs) isolated from the memory B cells of a naturally infected human donor. We identify several anti-NS1 MAbs that protect mice against lethal WNV challenge and map their epitopes using charge reversal mutagenesis. Antibodies targeting specific regions in the NS1 structure could serve as the basis for countermeasures that control WNV infection in humans.
AB - Envelope protein-targeted vaccines for flaviviruses are limited by concerns of antibody-dependent enhancement (ADE) of infections. Nonstructural protein 1 (NS1) provides an alternative vaccine target that avoids this risk since this protein is absent from the virion. Beyond its intracellular role in virus replication, extracellular forms of NS1 function in immune modulation and are recognized by host-derived antibodies. The rational design of NS1-based vaccines requires an extensive understanding of the antigenic sites on NS1, especially those targeted by protective antibodies. Here, we isolated human monoclonal antibodies (MAbs) from individuals previously naturally infected with WNV, mapped their epitopes using structure-guided mutagenesis, and evaluated their efficacy in vivo against lethal WNV challenge. The most protective epitopes clustered at three antigenic sites that are exposed on cell surface forms of NS1: (i) the wing flexible loop, (ii) the outer, electrostatic surface of the wing, and (iii) the spaghetti loop face of the b-ladder. One additional MAb mapped to the distal tip of the b-ladder and conferred a lower level of protection against WNV despite not binding to NS1 on the surface of infected cells. Our study defines the epitopes and modes of binding of protective anti-NS1 MAb antibodies following WNV infection, which may inform the development of NS1-based countermeasures against flaviviruses. IMPORTANCE Therapeutic antibodies against flaviviruses often promote neutralization by targeting the envelope protein of the virion. However, this approach is hindered by a possible concern for antibody-dependent enhancement of infection and paradoxical worsening of disease. As an alternative strategy, antibodies targeting flavivirus nonstructural protein 1 (NS1), which is absent from the virion, can protect against disease and do not cause enhanced infection. Here, we evaluate the structure-function relationships and protective activity of West Nile virus (WNV) NS1-specific monoclonal antibodies (MAbs) isolated from the memory B cells of a naturally infected human donor. We identify several anti-NS1 MAbs that protect mice against lethal WNV challenge and map their epitopes using charge reversal mutagenesis. Antibodies targeting specific regions in the NS1 structure could serve as the basis for countermeasures that control WNV infection in humans.
KW - Antibody function
KW - Epitope
KW - Flavivirus
KW - Viral pathogenesis
UR - http://www.scopus.com/inward/record.url?scp=85121015231&partnerID=8YFLogxK
U2 - 10.1128/mBio.02440-21
DO - 10.1128/mBio.02440-21
M3 - Article
C2 - 34634945
AN - SCOPUS:85121015231
SN - 2161-2129
VL - 12
JO - mBio
JF - mBio
IS - 5
M1 - e02440-21
ER -