Dendritic cells focus CTL responses toward highly conserved and topologically important HIV-1 epitopes

I4C and RV254 Study Groups

doi:10.1016/j.ebiom.2020.103175

Dendritic cells focus CTL responses toward highly conserved and topologically important HIV-1 epitopes

I4C and RV254 Study Groups

Global Health

University of Pittsburgh
Armed Forces Research Institute of Medical Sciences, Thailand
Henry M. Jackson Foundation
Walter Reed Army Institute of Research
Thai Red Cross Society
Amsterdam UMC - University of Amsterdam
Los Alamos National Laboratory
Massachusetts Institute of Technology
Harvard University
Broad Institute
Howard Hughes Medical Institute

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

Background: During early HIV-1 infection, immunodominant T cell responses to highly variable epitopes lead to the establishment of immune escape virus variants. Here we assessed a type 1-polarized monocyte-derived dendritic cell (MDC1)-based approach to selectively elicit cytotoxic T lymphocyte (CTL) responses against highly conserved and topologically important HIV-1 epitopes in HIV-1-infected individuals from the Thailand RV254/SEARCH 010 cohort who initiated antiretroviral therapy (ART) during early infection (Fiebig stages I-IV). Methods: Autologous MDC1 were used as antigen presenting cells to induce in vitro CTL responses against HIV-1 Gag, Pol, Env, and Nef as determined by flow cytometry and ELISpot assay. Ultra-conserved or topologically important antigens were respectively identified using the Epigraph tool and a structure-based network analysis approach and compared to overlapping peptides spanning the Gag proteome. Findings: MDC1 presenting either the overlapping Gag, Epigraph, or Network 14–21mer peptide pools consistently activated and expanded HIV-1-specific T cells to epitopes identified at the 9–13mer peptide level. Interestingly, some CTL responses occurred outside known or expected HLA associations, providing evidence of new HLA-associated CTL epitopes. Comparative analyses demonstrated more sequence conservation among Epigraph antigens but a higher magnitude of CTL responses to Network and Gag peptide groups. Importantly, CTL responses against topologically constrained Gag epitopes contained in both the Network and Gag peptide pools were selectively enhanced in the Network pool-initiated cultures. Interpretation: Our study supports the use of MDC1 as a therapeutic strategy to induce and focus CTL responses toward putative fitness-constrained regions of HIV-1 to prevent immune escape and control HIV-1 infection. Funding: A full list of the funding sources is detailed in the Acknowledgment section of the manuscript.

Original language	English
Article number	103175
Journal	EBioMedicine
Volume	63
DOIs	https://doi.org/10.1016/j.ebiom.2020.103175
Publication status	Published - 1 Jan 2021

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

SDG 3 Good Health and Well-being

Keywords

Cytotoxic T cell
Dendritic cell
Epitopes
HIV-1 cure
Immunotherapy

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10.1016/j.ebiom.2020.103175

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@article{21efd8b08ce84f379b7e86fb5ea98343,

title = "Dendritic cells focus CTL responses toward highly conserved and topologically important HIV-1 epitopes",

abstract = "Background: During early HIV-1 infection, immunodominant T cell responses to highly variable epitopes lead to the establishment of immune escape virus variants. Here we assessed a type 1-polarized monocyte-derived dendritic cell (MDC1)-based approach to selectively elicit cytotoxic T lymphocyte (CTL) responses against highly conserved and topologically important HIV-1 epitopes in HIV-1-infected individuals from the Thailand RV254/SEARCH 010 cohort who initiated antiretroviral therapy (ART) during early infection (Fiebig stages I-IV). Methods: Autologous MDC1 were used as antigen presenting cells to induce in vitro CTL responses against HIV-1 Gag, Pol, Env, and Nef as determined by flow cytometry and ELISpot assay. Ultra-conserved or topologically important antigens were respectively identified using the Epigraph tool and a structure-based network analysis approach and compared to overlapping peptides spanning the Gag proteome. Findings: MDC1 presenting either the overlapping Gag, Epigraph, or Network 14–21mer peptide pools consistently activated and expanded HIV-1-specific T cells to epitopes identified at the 9–13mer peptide level. Interestingly, some CTL responses occurred outside known or expected HLA associations, providing evidence of new HLA-associated CTL epitopes. Comparative analyses demonstrated more sequence conservation among Epigraph antigens but a higher magnitude of CTL responses to Network and Gag peptide groups. Importantly, CTL responses against topologically constrained Gag epitopes contained in both the Network and Gag peptide pools were selectively enhanced in the Network pool-initiated cultures. Interpretation: Our study supports the use of MDC1 as a therapeutic strategy to induce and focus CTL responses toward putative fitness-constrained regions of HIV-1 to prevent immune escape and control HIV-1 infection. Funding: A full list of the funding sources is detailed in the Acknowledgment section of the manuscript.",

keywords = "Cytotoxic T cell, Dendritic cell, Epitopes, HIV-1 cure, Immunotherapy",

author = "Garcia-Bates, \{Tatiana M.\} and Palma, \{Mariana L.\} and Anderko, \{Renee R.\} and Hsu, \{Denise C.\} and Jintanat Ananworanich and Korber, \{Bette T.\} and Gaiha, \{Gaurav D.\} and Nittaya Phanuphak and Rasmi Thomas and Sodsai Tovanabutra and Walker, \{Bruce D.\} and Mellors, \{John W.\} and Piazza, \{Paolo A.\} and Eugene Kroon and Riddler, \{Sharon A.\} and Michael, \{Nelson L.\} and \{I4C and RV254 Study Groups\} and Rinaldo, \{Charles R.\} and Mailliard, \{Robbie B.\}",

note = "Funding Information: JWM reports grants from the NIH and Gilead Sciences, personal fees (consultant) from Gilead Sciences, Merck, Accelevir Diagnostics, and others from Co-Crystal Pharmaceuticals, Inc., Infectious Diseases Connect, and Abound Bio, Inc., outside the submitted work; JA reports grants from The Henry M. Jackson Foundation for the Advancement of Military Medicine, Inc., the U.S. Department of Defense, and others from ViiV Healthcare, Gilead, Merck, Roche, and AbbVie, outside the submitted work; SAR reports grants from the NIH; RBM and CRR report a patent PCT/US2020/039843, Pitt Ref: 04973 (pending) for use of antigen presenting cells in HIV therapy: GDG reports a patent PCT/US2020/022403 (pending), Network Immunogen Composition; and BTK reports several provisional patents not directly related to the present work but to HIV vaccines in general. The most recent of these patents is US 2020/0055901, Signature-based human immunodeficiency virus envelope trimer vaccines and methods of using the same. Funding Information: This study was in part supported by the U.S. NIH , National Institute of Allergy and Infectious Diseases Grants R21-AI131763 , R21-AI138716 , UM1-AI126603 , and U01-AI35041 . The RV254/SEARCH 010 is supported by cooperative agreements (WW81XWH-18-2-0040) between the Henry M. Jackson Foundation for the Advancement of Military Medicine, Inc. , and the U.S. Department of Defense and by an intramural grant from the Thai Red Cross AIDS Research Centre. Antiretroviral therapy for RV254/SEARCH 010 participants was supported by the Thai Government Pharmaceutical Organization, Gilead, Merck , and ViiV Healthcare . The funding sources did not play a role in the study design, data generation and analysis, interpretation of the findings, manuscript preparation, or decision for publishing. Publisher Copyright: {\textcopyright} 2020 The Authors",

year = "2021",

month = jan,

day = "1",

doi = "10.1016/j.ebiom.2020.103175",

language = "English",

volume = "63",

journal = "EBioMedicine",

issn = "2352-3964",

publisher = "Elsevier B.V.",

}

TY - JOUR

T1 - Dendritic cells focus CTL responses toward highly conserved and topologically important HIV-1 epitopes

AU - Garcia-Bates, Tatiana M.

AU - Palma, Mariana L.

AU - Anderko, Renee R.

AU - Hsu, Denise C.

AU - Ananworanich, Jintanat

AU - Korber, Bette T.

AU - Gaiha, Gaurav D.

AU - Phanuphak, Nittaya

AU - Thomas, Rasmi

AU - Tovanabutra, Sodsai

AU - Walker, Bruce D.

AU - Mellors, John W.

AU - Piazza, Paolo A.

AU - Kroon, Eugene

AU - Riddler, Sharon A.

AU - Michael, Nelson L.

AU - I4C and RV254 Study Groups

AU - Rinaldo, Charles R.

AU - Mailliard, Robbie B.

N1 - Funding Information: JWM reports grants from the NIH and Gilead Sciences, personal fees (consultant) from Gilead Sciences, Merck, Accelevir Diagnostics, and others from Co-Crystal Pharmaceuticals, Inc., Infectious Diseases Connect, and Abound Bio, Inc., outside the submitted work; JA reports grants from The Henry M. Jackson Foundation for the Advancement of Military Medicine, Inc., the U.S. Department of Defense, and others from ViiV Healthcare, Gilead, Merck, Roche, and AbbVie, outside the submitted work; SAR reports grants from the NIH; RBM and CRR report a patent PCT/US2020/039843, Pitt Ref: 04973 (pending) for use of antigen presenting cells in HIV therapy: GDG reports a patent PCT/US2020/022403 (pending), Network Immunogen Composition; and BTK reports several provisional patents not directly related to the present work but to HIV vaccines in general. The most recent of these patents is US 2020/0055901, Signature-based human immunodeficiency virus envelope trimer vaccines and methods of using the same. Funding Information: This study was in part supported by the U.S. NIH , National Institute of Allergy and Infectious Diseases Grants R21-AI131763 , R21-AI138716 , UM1-AI126603 , and U01-AI35041 . The RV254/SEARCH 010 is supported by cooperative agreements (WW81XWH-18-2-0040) between the Henry M. Jackson Foundation for the Advancement of Military Medicine, Inc. , and the U.S. Department of Defense and by an intramural grant from the Thai Red Cross AIDS Research Centre. Antiretroviral therapy for RV254/SEARCH 010 participants was supported by the Thai Government Pharmaceutical Organization, Gilead, Merck , and ViiV Healthcare . The funding sources did not play a role in the study design, data generation and analysis, interpretation of the findings, manuscript preparation, or decision for publishing. Publisher Copyright: © 2020 The Authors

PY - 2021/1/1

Y1 - 2021/1/1

N2 - Background: During early HIV-1 infection, immunodominant T cell responses to highly variable epitopes lead to the establishment of immune escape virus variants. Here we assessed a type 1-polarized monocyte-derived dendritic cell (MDC1)-based approach to selectively elicit cytotoxic T lymphocyte (CTL) responses against highly conserved and topologically important HIV-1 epitopes in HIV-1-infected individuals from the Thailand RV254/SEARCH 010 cohort who initiated antiretroviral therapy (ART) during early infection (Fiebig stages I-IV). Methods: Autologous MDC1 were used as antigen presenting cells to induce in vitro CTL responses against HIV-1 Gag, Pol, Env, and Nef as determined by flow cytometry and ELISpot assay. Ultra-conserved or topologically important antigens were respectively identified using the Epigraph tool and a structure-based network analysis approach and compared to overlapping peptides spanning the Gag proteome. Findings: MDC1 presenting either the overlapping Gag, Epigraph, or Network 14–21mer peptide pools consistently activated and expanded HIV-1-specific T cells to epitopes identified at the 9–13mer peptide level. Interestingly, some CTL responses occurred outside known or expected HLA associations, providing evidence of new HLA-associated CTL epitopes. Comparative analyses demonstrated more sequence conservation among Epigraph antigens but a higher magnitude of CTL responses to Network and Gag peptide groups. Importantly, CTL responses against topologically constrained Gag epitopes contained in both the Network and Gag peptide pools were selectively enhanced in the Network pool-initiated cultures. Interpretation: Our study supports the use of MDC1 as a therapeutic strategy to induce and focus CTL responses toward putative fitness-constrained regions of HIV-1 to prevent immune escape and control HIV-1 infection. Funding: A full list of the funding sources is detailed in the Acknowledgment section of the manuscript.

AB - Background: During early HIV-1 infection, immunodominant T cell responses to highly variable epitopes lead to the establishment of immune escape virus variants. Here we assessed a type 1-polarized monocyte-derived dendritic cell (MDC1)-based approach to selectively elicit cytotoxic T lymphocyte (CTL) responses against highly conserved and topologically important HIV-1 epitopes in HIV-1-infected individuals from the Thailand RV254/SEARCH 010 cohort who initiated antiretroviral therapy (ART) during early infection (Fiebig stages I-IV). Methods: Autologous MDC1 were used as antigen presenting cells to induce in vitro CTL responses against HIV-1 Gag, Pol, Env, and Nef as determined by flow cytometry and ELISpot assay. Ultra-conserved or topologically important antigens were respectively identified using the Epigraph tool and a structure-based network analysis approach and compared to overlapping peptides spanning the Gag proteome. Findings: MDC1 presenting either the overlapping Gag, Epigraph, or Network 14–21mer peptide pools consistently activated and expanded HIV-1-specific T cells to epitopes identified at the 9–13mer peptide level. Interestingly, some CTL responses occurred outside known or expected HLA associations, providing evidence of new HLA-associated CTL epitopes. Comparative analyses demonstrated more sequence conservation among Epigraph antigens but a higher magnitude of CTL responses to Network and Gag peptide groups. Importantly, CTL responses against topologically constrained Gag epitopes contained in both the Network and Gag peptide pools were selectively enhanced in the Network pool-initiated cultures. Interpretation: Our study supports the use of MDC1 as a therapeutic strategy to induce and focus CTL responses toward putative fitness-constrained regions of HIV-1 to prevent immune escape and control HIV-1 infection. Funding: A full list of the funding sources is detailed in the Acknowledgment section of the manuscript.

KW - Cytotoxic T cell

KW - Dendritic cell

KW - Epitopes

KW - HIV-1 cure

KW - Immunotherapy

UR - https://www.scopus.com/pages/publications/85099206723

U2 - 10.1016/j.ebiom.2020.103175

DO - 10.1016/j.ebiom.2020.103175

M3 - Article

C2 - 33450518

SN - 2352-3964

VL - 63

JO - EBioMedicine

JF - EBioMedicine

M1 - 103175

ER -

Dendritic cells focus CTL responses toward highly conserved and topologically important HIV-1 epitopes

Abstract

UN SDGs

Keywords

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