Interpreting ELISA analyses from wild animal samples: Some recurrent issues and solutions
International audience Many studies in disease and ecological immunology rely on the use of assays thatquantify the amount of specific antibodies (immunoglobulin) in samples. Enzymelinkedimmunosorbent assays (ELISAs) are increasingly used in ecology due to theiravailability for a broad array of anti...
Published in: | Functional Ecology |
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Main Authors: | , , , , , , , |
Other Authors: | , , , , , , , , , , , , |
Format: | Article in Journal/Newspaper |
Language: | English |
Published: |
HAL CCSD
2017
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Subjects: | |
Online Access: | https://hal.science/hal-01882627 https://hal.science/hal-01882627/document https://hal.science/hal-01882627/file/672476.pdf https://doi.org/10.1111/1365-2435.12942 |
Summary: | International audience Many studies in disease and ecological immunology rely on the use of assays thatquantify the amount of specific antibodies (immunoglobulin) in samples. Enzymelinkedimmunosorbent assays (ELISAs) are increasingly used in ecology due to theiravailability for a broad array of antigens and the limited amount of sampling materialthey require. Two recurrent methodological issues are nevertheless faced byresearchers: (1) the limited availability of immunological assays and reagents developedfor non-model species, and (2) the statistical determination of the cut-offthreshold used to distinguish individual samples that are likely to have or not tohave antibodies against a specific antigen.Here, we outline two solutions to deal with these issues. First, we show that implementingtwo assays with differing detection methods can help validate the use ofreagents, such as antibodies, in species different from their intended target. We illustrate this by comparing the quantification of specific vaccinal antibodies against Newcastle disease virus (NDV) using two ELISA approaches in four seabird species (Cory’s shearwater, European shag, European storm petrel and Southern rockhopper penguin).Second, we provide a simple way to determine from the distribution of ELISA valueswhether the assayed samples are likely to be made of a single group of individuals(likely negative) or of two groups of individuals (negative and positive). We illustrate the use of this approach with two independent data sets: NDV antibody levels following vaccination and anti-Borrelia antibody levels following natural exposure.The practical implementation of these methodological approaches could provide away to efficiently apply ELISAs and other immune-based assays to address questions in the growing fields of ecological immunology and disease ecology |
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