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Exploring Natural Immune Responses to Shigella Exposure Using Multiplex Bead Assays on Dried Blood Spots in High-Burden Countries: Protocol From a Multisite Diarrhea Surveillance Study

Abstract Background Molecular diagnostics on human fecal samples have identified a larger burden of shigellosis than previously appreciated by culture. Evidence of fold changes in immunoglobulin G (IgG) to conserved and type-specific Shigella antigens could be used to validate the molecular assignme...

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Published in:Open forum infectious diseases 2024-03, Vol.11 (Supplement_1), p.S58-S64
Main Authors: Benedicto-Matambo, Prisca, Avolio, Lindsay N, Badji, Henry, Batool, Rabab, Khanam, Farhana, Munga, Stephen, Tapia, Milagritos D, Peñataro Yori, Pablo, Awuor, Alex O, Ceesay, Bubacarr E, Cornick, Jennifer, Cunliffe, Nigel A, Garcia Bardales, Paul F, Heaney, Christopher D, Hotwani, Aneeta, Ireen, Mahzabeen, Taufiqul Islam, Md, Jallow, Ousman, Kaminski, Robert W, Shapiama Lopez, Wagner V, Maiden, Victor, Ikumapayi, Usman Nurudeen, Nyirenda, Ruth, Ochieng, John Benjamin, Omore, Richard, Paredes Olortegui, Maribel, Pavlinac, Patricia B, Pisanic, Nora, Qadri, Firdausi, Qureshi, Sonia, Rahman, Nazia, Rogawski McQuade, Elizabeth T, Schiaffino, Francesca, Secka, Ousman, Sonye, Catherine, Sultana, Shazia, Timite, Drissa, Traore, Awa, Yousafzai, Mohammad Tahir, Taufiqur Rahman Bhuiyan, Md, Jahangir Hossain, M, Jere, Khuzwayo C, Kosek, Margaret N, Kotloff, Karen L, Qamar, Farah Naz, Sow, Samba O, Platts-Mills, James A
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Language:English
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Summary:Abstract Background Molecular diagnostics on human fecal samples have identified a larger burden of shigellosis than previously appreciated by culture. Evidence of fold changes in immunoglobulin G (IgG) to conserved and type-specific Shigella antigens could be used to validate the molecular assignment of type-specific Shigella as the etiology of acute diarrhea and support polymerase chain reaction (PCR)–based microbiologic end points for vaccine trials. Methods We will test dried blood spots collected at enrollment and 4 weeks later using bead-based immunoassays for IgG to invasion plasmid antigen B and type-specific lipopolysaccharide O-antigen for Shigella flexneri 1b, 2a, 3a, and 6 and Shigella sonnei in Shigella-positive cases and age-, site-, and season-matched test-negative controls from all sites in the Enterics for Global Health (EFGH) Shigella surveillance study. Fold antibody responses will be compared between culture-positive, culture-negative but PCR-attributable, and PCR-positive but not attributable cases and test-negative controls. Age- and site-specific seroprevalence distributions will be identified, and the association between baseline antibodies and Shigella attribution will be estimated. Conclusions The integration of these assays into the EFGH study will help support PCR-based attribution of acute diarrhea to type-specific Shigella, describe the baseline seroprevalence of conserved and type-specific Shigella antibodies, and support correlates of protection for immunity to Shigella diarrhea. These insights can help support the development and evaluation of Shigella vaccine candidates. Multiplex bead-based immunoassays for IgG to conserved and type-specific Shigella antigens will be performed on acute and convalescent dried blood spots to characterize conserved and type-specific immune responses and validate molecular identification of type-specific Shigella diarrhea.
ISSN:2328-8957
2328-8957
DOI:10.1093/ofid/ofad650