Outer membrane protein size and LPS O-antigen define protective antibody targeting to the Salmonella surface

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作者
C. Coral Domínguez-Medina
Marisol Pérez-Toledo
Anna E. Schager
Jennifer L. Marshall
Charlotte N. Cook
Saeeda Bobat
Hyea Hwang
Byeong Jae Chun
Erin Logan
Jack A. Bryant
Will M. Channell
Faye C. Morris
Sian E. Jossi
Areej Alshayea
Amanda E. Rossiter
Paul A. Barrow
William G. Horsnell
Calman A. MacLennan
Ian R. Henderson
Jeremy H. Lakey
James C. Gumbart
Constantino López-Macías
Vassiliy N. Bavro
Adam F. Cunningham
机构
[1] University of Birmingham,Institute of Immunology and Immunotherapy
[2] University of Birmingham,Institute of Microbiology and Infection
[3] Specialties Hospital,Medical Research Unit on Immunochemistry
[4] National Medical Centre “Siglo XXI” Mexican Institute for Social Security,School of Materials Science and Engineering
[5] Georgia Institute of Technology,Institute of Infectious Disease and Molecular Medicine
[6] University of Cape Town,School of Veterinary Medicine and Science
[7] University of Nottingham,Jenner Institute, Nuffield Department of Medicine, Old Road Campus Research Building, Roosevelt Drive
[8] University of Oxford,Institute for Cell and Molecular Biosciences
[9] University of Newcastle,School of Physics
[10] Georgia Institute of Technology,School of Life Sciences
[11] University of Essex,undefined
[12] Wivenhoe Park,undefined
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摘要
Lipopolysaccharide (LPS) O-antigen (O-Ag) is known to limit antibody binding to surface antigens, although the relationship between antibody, O-Ag and other outer-membrane antigens is poorly understood. Here we report, immunization with the trimeric porin OmpD from Salmonella Typhimurium (STmOmpD) protects against infection. Atomistic molecular dynamics simulations indicate this is because OmpD trimers generate footprints within the O-Ag layer sufficiently sized for a single IgG Fab to access. While STmOmpD differs from its orthologue in S. Enteritidis (SEn) by a single amino-acid residue, immunization with STmOmpD confers minimal protection to SEn. This is due to the OmpD-O-Ag interplay restricting IgG binding, with the pairing of OmpD with its native O-Ag being essential for optimal protection after immunization. Thus, both the chemical and physical structure of O-Ag are key for the presentation of specific epitopes within proteinaceous surface-antigens. This enhances combinatorial antigenic diversity in Gram-negative bacteria, while reducing associated fitness costs.
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