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Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal

New diagnostic tests for enteric fever are urgently needed to assist with timely antimicrobial treatment of patients and to measure the efficacy of prevention measures such as vaccination. In a novel translational approach, here we use two recently developed controlled human infection models (CHIM)...

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Autores principales: Darton, Thomas C., Jones, Claire, Dongol, Sabina, Voysey, Merryn, Blohmke, Christoph J., Shrestha, Rajendra, Karkey, Abhilasha, Shakya, Mila, Arjyal, Amit, Waddington, Claire S., Gibani, Malick, Carter, Michael J., Basnyat, Buddha, Baker, Stephen, Pollard, Andrew J.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2017
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5660281/
https://www.ncbi.nlm.nih.gov/pubmed/29109704
http://dx.doi.org/10.3389/fmicb.2017.02031
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author Darton, Thomas C.
Jones, Claire
Dongol, Sabina
Voysey, Merryn
Blohmke, Christoph J.
Shrestha, Rajendra
Karkey, Abhilasha
Shakya, Mila
Arjyal, Amit
Waddington, Claire S.
Gibani, Malick
Carter, Michael J.
Basnyat, Buddha
Baker, Stephen
Pollard, Andrew J.
author_facet Darton, Thomas C.
Jones, Claire
Dongol, Sabina
Voysey, Merryn
Blohmke, Christoph J.
Shrestha, Rajendra
Karkey, Abhilasha
Shakya, Mila
Arjyal, Amit
Waddington, Claire S.
Gibani, Malick
Carter, Michael J.
Basnyat, Buddha
Baker, Stephen
Pollard, Andrew J.
author_sort Darton, Thomas C.
collection PubMed
description New diagnostic tests for enteric fever are urgently needed to assist with timely antimicrobial treatment of patients and to measure the efficacy of prevention measures such as vaccination. In a novel translational approach, here we use two recently developed controlled human infection models (CHIM) of enteric fever to evaluate an antibody-in-lymphocyte supernatant (ALS) assay, which can detect recent IgA antibody production by circulating B cells in ex vivo mononuclear cell culture. We calculated the discriminative ability of the ALS assay to distinguish diagnosed cases in the two CHIM studies in Oxford, prior to evaluating blood culture-confirmed diagnoses of patients presenting with fever to hospital in an endemic areas of Kathmandu, Nepal. Antibody responses to membrane preparations and lipopolysaccharide provided good sensitivity (>90%) for diagnosing systemic infection after oral challenge with Salmonella Typhi or S. Paratyphi A. Assay specificity was moderate (~60%) due to imperfect sensitivity of blood culture as the reference standard and likely unrecognized subclinical infection. These findings were augmented through the translation of the assay into the endemic setting in Nepal. Anti-MP IgA responses again exhibited good sensitivity (86%) but poor specificity (51%) for detecting blood culture-confirmed enteric fever cases (ROC AUC 0.79, 95%CI 0.70–0.88). Patients with anti-MP IgA ALS titers in the upper quartile exhibited a clinical syndrome synonymous with enteric fever. While better reference standards are need to assess enteric fever diagnostics, routine use of this ALS assay could be used to rule out infection and has the potential to double the laboratory detection rate of enteric fever in this setting over blood culture alone.
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spelling pubmed-56602812017-11-06 Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal Darton, Thomas C. Jones, Claire Dongol, Sabina Voysey, Merryn Blohmke, Christoph J. Shrestha, Rajendra Karkey, Abhilasha Shakya, Mila Arjyal, Amit Waddington, Claire S. Gibani, Malick Carter, Michael J. Basnyat, Buddha Baker, Stephen Pollard, Andrew J. Front Microbiol Microbiology New diagnostic tests for enteric fever are urgently needed to assist with timely antimicrobial treatment of patients and to measure the efficacy of prevention measures such as vaccination. In a novel translational approach, here we use two recently developed controlled human infection models (CHIM) of enteric fever to evaluate an antibody-in-lymphocyte supernatant (ALS) assay, which can detect recent IgA antibody production by circulating B cells in ex vivo mononuclear cell culture. We calculated the discriminative ability of the ALS assay to distinguish diagnosed cases in the two CHIM studies in Oxford, prior to evaluating blood culture-confirmed diagnoses of patients presenting with fever to hospital in an endemic areas of Kathmandu, Nepal. Antibody responses to membrane preparations and lipopolysaccharide provided good sensitivity (>90%) for diagnosing systemic infection after oral challenge with Salmonella Typhi or S. Paratyphi A. Assay specificity was moderate (~60%) due to imperfect sensitivity of blood culture as the reference standard and likely unrecognized subclinical infection. These findings were augmented through the translation of the assay into the endemic setting in Nepal. Anti-MP IgA responses again exhibited good sensitivity (86%) but poor specificity (51%) for detecting blood culture-confirmed enteric fever cases (ROC AUC 0.79, 95%CI 0.70–0.88). Patients with anti-MP IgA ALS titers in the upper quartile exhibited a clinical syndrome synonymous with enteric fever. While better reference standards are need to assess enteric fever diagnostics, routine use of this ALS assay could be used to rule out infection and has the potential to double the laboratory detection rate of enteric fever in this setting over blood culture alone. Frontiers Media S.A. 2017-10-23 /pmc/articles/PMC5660281/ /pubmed/29109704 http://dx.doi.org/10.3389/fmicb.2017.02031 Text en Copyright © 2017 Darton, Jones, Dongol, Voysey, Blohmke, Shrestha, Karkey, Shakya, Arjyal, Waddington, Gibani, Carter, Basnyat, Baker and Pollard. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
spellingShingle Microbiology
Darton, Thomas C.
Jones, Claire
Dongol, Sabina
Voysey, Merryn
Blohmke, Christoph J.
Shrestha, Rajendra
Karkey, Abhilasha
Shakya, Mila
Arjyal, Amit
Waddington, Claire S.
Gibani, Malick
Carter, Michael J.
Basnyat, Buddha
Baker, Stephen
Pollard, Andrew J.
Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal
title Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal
title_full Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal
title_fullStr Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal
title_full_unstemmed Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal
title_short Assessment and Translation of the Antibody-in-Lymphocyte Supernatant (ALS) Assay to Improve the Diagnosis of Enteric Fever in Two Controlled Human Infection Models and an Endemic Area of Nepal
title_sort assessment and translation of the antibody-in-lymphocyte supernatant (als) assay to improve the diagnosis of enteric fever in two controlled human infection models and an endemic area of nepal
topic Microbiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5660281/
https://www.ncbi.nlm.nih.gov/pubmed/29109704
http://dx.doi.org/10.3389/fmicb.2017.02031
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