What to do and what not to do in serological diagnosis of pertussis: Recommendations from EU reference laboratories

Nicole Guiso; Guy Berbers; Norman Fry; Qiushui He; Marion Riffelmann; C. H. Wirsing Von König; Jussi Mertsola; Sophie Guillot; Hans Hallander; Abdolreza Advani; Frits R. Mooi; Anna Lutynska; Karen Krogfelt; Tine Dalby; Dorothy Xing; Camille Locht; David Hot; Clara Ausiello; Per Sandven; Jann Storsaeter

doi:10.1007/s10096-010-1104-y

What to do and what not to do in serological diagnosis of pertussis: Recommendations from EU reference laboratories

Nicole Guiso
, Guy Berbers
, Norman Fry
, Qiushui He
, Marion Riffelmann
, C. H. Wirsing Von König
, Jussi Mertsola
, Sophie Guillot
, Hans Hallander
, Abdolreza Advani
, Frits R. Mooi
, Anna Lutynska
, Karen Krogfelt
, Tine Dalby
, Dorothy Xing
, Camille Locht
, David Hot
, Clara Ausiello
, Per Sandven
, Jann Storsaeter

Immunisation & Vaccine Preventable Diseases

Research output: Contribution to journal › Review article › peer-review

233 Citations (Scopus)

Abstract

Bordetella pertussis-specific antibodies can be detected by enzyme-linked immunosorbent assays (ELISAs) or multiplex immunoassays. Assays use purified or mixed antigens, and only pertussis toxin (PT) is specific for B. pertussis. The interpretation of results can be based on dual-sample or single-sample serology using one or two cut-offs. The EU Pertstrain group recommends that: (i) ELISAs and multiplex immunoassays should use purified non-detoxified PT as an antigen, that they should have a broad linear range and that they should express results quantitatively in International Units per millilitre (IU/ml); (ii) a single or dual diagnostic cut-off for single-serum serology using IgG-anti-PT between 50 and 120 IU/ml should be used, and diagnostic serology cannot be validly interpreted for one year after vaccination with acellular pertussis (aP) vaccines; (iii) IgA-anti-PT should only be used with indeterminate IgG-anti-PT levels or when a second sample cannot be obtained. This group discourages using: (i) other antigens in routine diagnostics, as they are not specific; (ii) micro-agglutination, due to its lack of sensitivity; (iii) immunoblots for pertussis serodiagnosis, as results cannot be quantified; (iv) other methods, such as complement fixation or indirect immunofluorescence, due to their low sensitivity and/or specificity.

Original language	English
Pages (from-to)	307-312
Number of pages	6
Journal	European Journal of Clinical Microbiology and Infectious Diseases
Volume	30
Issue number	3
DOIs	https://doi.org/10.1007/s10096-010-1104-y
Publication status	Published - Mar 2011

UN SDGs

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

SDG 3 Good Health and Well-being

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10.1007/s10096-010-1104-y

Cite this

Guiso, N., Berbers, G., Fry, N., He, Q., Riffelmann, M., Wirsing Von König, C. H., Mertsola, J., Guillot, S., Hallander, H., Advani, A., Mooi, F. R., Lutynska, A., Krogfelt, K., Dalby, T., Xing, D., Locht, C., Hot, D., Ausiello, C., Sandven, P., & Storsaeter, J. (2011). What to do and what not to do in serological diagnosis of pertussis: Recommendations from EU reference laboratories. European Journal of Clinical Microbiology and Infectious Diseases, 30(3), 307-312. https://doi.org/10.1007/s10096-010-1104-y

@article{c35a3fc27f2743cb8620693a84188318,

title = "What to do and what not to do in serological diagnosis of pertussis: Recommendations from EU reference laboratories",

abstract = "Bordetella pertussis-specific antibodies can be detected by enzyme-linked immunosorbent assays (ELISAs) or multiplex immunoassays. Assays use purified or mixed antigens, and only pertussis toxin (PT) is specific for B. pertussis. The interpretation of results can be based on dual-sample or single-sample serology using one or two cut-offs. The EU Pertstrain group recommends that: (i) ELISAs and multiplex immunoassays should use purified non-detoxified PT as an antigen, that they should have a broad linear range and that they should express results quantitatively in International Units per millilitre (IU/ml); (ii) a single or dual diagnostic cut-off for single-serum serology using IgG-anti-PT between 50 and 120 IU/ml should be used, and diagnostic serology cannot be validly interpreted for one year after vaccination with acellular pertussis (aP) vaccines; (iii) IgA-anti-PT should only be used with indeterminate IgG-anti-PT levels or when a second sample cannot be obtained. This group discourages using: (i) other antigens in routine diagnostics, as they are not specific; (ii) micro-agglutination, due to its lack of sensitivity; (iii) immunoblots for pertussis serodiagnosis, as results cannot be quantified; (iv) other methods, such as complement fixation or indirect immunofluorescence, due to their low sensitivity and/or specificity.",

author = "Nicole Guiso and Guy Berbers and Norman Fry and Qiushui He and Marion Riffelmann and \{Wirsing Von K{\"o}nig\}, \{C. H.\} and Jussi Mertsola and Sophie Guillot and Hans Hallander and Abdolreza Advani and Mooi, \{Frits R.\} and Anna Lutynska and Karen Krogfelt and Tine Dalby and Dorothy Xing and Camille Locht and David Hot and Clara Ausiello and Per Sandven and Jann Storsaeter",

year = "2011",

month = mar,

doi = "10.1007/s10096-010-1104-y",

language = "English",

volume = "30",

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Guiso, N, Berbers, G, Fry, N, He, Q, Riffelmann, M, Wirsing Von König, CH, Mertsola, J, Guillot, S, Hallander, H, Advani, A, Mooi, FR, Lutynska, A, Krogfelt, K, Dalby, T, Xing, D, Locht, C, Hot, D, Ausiello, C, Sandven, P & Storsaeter, J 2011, 'What to do and what not to do in serological diagnosis of pertussis: Recommendations from EU reference laboratories', European Journal of Clinical Microbiology and Infectious Diseases, vol. 30, no. 3, pp. 307-312. https://doi.org/10.1007/s10096-010-1104-y

TY - JOUR

T1 - What to do and what not to do in serological diagnosis of pertussis

T2 - Recommendations from EU reference laboratories

AU - Guiso, Nicole

AU - Berbers, Guy

AU - Fry, Norman

AU - He, Qiushui

AU - Riffelmann, Marion

AU - Wirsing Von König, C. H.

AU - Mertsola, Jussi

AU - Guillot, Sophie

AU - Hallander, Hans

AU - Advani, Abdolreza

AU - Mooi, Frits R.

AU - Lutynska, Anna

AU - Krogfelt, Karen

AU - Dalby, Tine

AU - Xing, Dorothy

AU - Locht, Camille

AU - Hot, David

AU - Ausiello, Clara

AU - Sandven, Per

AU - Storsaeter, Jann

PY - 2011/3

Y1 - 2011/3

N2 - Bordetella pertussis-specific antibodies can be detected by enzyme-linked immunosorbent assays (ELISAs) or multiplex immunoassays. Assays use purified or mixed antigens, and only pertussis toxin (PT) is specific for B. pertussis. The interpretation of results can be based on dual-sample or single-sample serology using one or two cut-offs. The EU Pertstrain group recommends that: (i) ELISAs and multiplex immunoassays should use purified non-detoxified PT as an antigen, that they should have a broad linear range and that they should express results quantitatively in International Units per millilitre (IU/ml); (ii) a single or dual diagnostic cut-off for single-serum serology using IgG-anti-PT between 50 and 120 IU/ml should be used, and diagnostic serology cannot be validly interpreted for one year after vaccination with acellular pertussis (aP) vaccines; (iii) IgA-anti-PT should only be used with indeterminate IgG-anti-PT levels or when a second sample cannot be obtained. This group discourages using: (i) other antigens in routine diagnostics, as they are not specific; (ii) micro-agglutination, due to its lack of sensitivity; (iii) immunoblots for pertussis serodiagnosis, as results cannot be quantified; (iv) other methods, such as complement fixation or indirect immunofluorescence, due to their low sensitivity and/or specificity.

AB - Bordetella pertussis-specific antibodies can be detected by enzyme-linked immunosorbent assays (ELISAs) or multiplex immunoassays. Assays use purified or mixed antigens, and only pertussis toxin (PT) is specific for B. pertussis. The interpretation of results can be based on dual-sample or single-sample serology using one or two cut-offs. The EU Pertstrain group recommends that: (i) ELISAs and multiplex immunoassays should use purified non-detoxified PT as an antigen, that they should have a broad linear range and that they should express results quantitatively in International Units per millilitre (IU/ml); (ii) a single or dual diagnostic cut-off for single-serum serology using IgG-anti-PT between 50 and 120 IU/ml should be used, and diagnostic serology cannot be validly interpreted for one year after vaccination with acellular pertussis (aP) vaccines; (iii) IgA-anti-PT should only be used with indeterminate IgG-anti-PT levels or when a second sample cannot be obtained. This group discourages using: (i) other antigens in routine diagnostics, as they are not specific; (ii) micro-agglutination, due to its lack of sensitivity; (iii) immunoblots for pertussis serodiagnosis, as results cannot be quantified; (iv) other methods, such as complement fixation or indirect immunofluorescence, due to their low sensitivity and/or specificity.

UR - https://www.scopus.com/pages/publications/79951726961

U2 - 10.1007/s10096-010-1104-y

DO - 10.1007/s10096-010-1104-y

M3 - Review article

C2 - 21069406

AN - SCOPUS:79951726961

SN - 0934-9723

VL - 30

SP - 307

EP - 312

JO - European Journal of Clinical Microbiology and Infectious Diseases

JF - European Journal of Clinical Microbiology and Infectious Diseases

IS - 3

ER -

What to do and what not to do in serological diagnosis of pertussis: Recommendations from EU reference laboratories

Abstract

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