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Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats

BACKGROUND: Blood typing for the A and B antigens is essential and crossmatching testing is generally recommended before transfusing blood to cats. OBJECTIVE: To evaluate 2 crossmatch (XM) tests. ANIMALS: Forty‐nine healthy domestic shorthair cats that had not received a blood transfusion. METHODS:...

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Autores principales: Goy‐Thollot, Isabelle, Nectoux, Alexandra, Guidetti, Maryline, Chaprier, Benjamin, Bourgeois, Sarah, Boisvineau, Catherine, Barthélemy, Anthony, Pouzot‐Nevoret, Céline, Giger, Urs
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley & Sons, Inc. 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6430866/
https://www.ncbi.nlm.nih.gov/pubmed/30557453
http://dx.doi.org/10.1111/jvim.15381
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author Goy‐Thollot, Isabelle
Nectoux, Alexandra
Guidetti, Maryline
Chaprier, Benjamin
Bourgeois, Sarah
Boisvineau, Catherine
Barthélemy, Anthony
Pouzot‐Nevoret, Céline
Giger, Urs
author_facet Goy‐Thollot, Isabelle
Nectoux, Alexandra
Guidetti, Maryline
Chaprier, Benjamin
Bourgeois, Sarah
Boisvineau, Catherine
Barthélemy, Anthony
Pouzot‐Nevoret, Céline
Giger, Urs
author_sort Goy‐Thollot, Isabelle
collection PubMed
description BACKGROUND: Blood typing for the A and B antigens is essential and crossmatching testing is generally recommended before transfusing blood to cats. OBJECTIVE: To evaluate 2 crossmatch (XM) tests. ANIMALS: Forty‐nine healthy domestic shorthair cats that had not received a blood transfusion. METHODS: Prospective study. Blood samples were typed for AB using immunochromatographic and flow cytometric techniques. A gel column (GC) and a feline antiglobulin‐enhanced gel column (AGC) XM tests were used for crossmatching. RESULTS: The population included 34 type A, 13 B, and 2 AB cats, with concordant results (r = 1, P < .005) by flow cytometry and immunochromatographic strip kit. The plasma from type A cats had either no or weak anti‐B alloantibodies. The plasma of 12 of 13 type B cats contained strong anti‐A alloantibodies. For crossmatching, plasma to RBC pairings were prepared using the GC (n = 446) and AGC (n = 630) tests. Both methods showed compatibilities in 329 and incompatibilities in 102 pairings including all A‐B mismatches. Additionally 15 pairings showed agglutination by the AGC but not GC method. Fourteen incompatibilities outside the expected A‐B mismatches were only revealed by AGC. CONCLUSIONS AND CLINICAL IMPORTANCE: AB typing using immunochromatographic strip is as accurate as laboratory flow cytometry. The 2 XM methods had good agreement with additional incompatibilities being recognized by the AGC XM beyond A‐B incompatibilities. In clinic, feline AB typing and sensitive XM test kits are available and recommended before each transfusion, although the clinical implications of incompatible XM test results and clinical benefits of such crossmatching have not been documented.
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spelling pubmed-64308662019-04-04 Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats Goy‐Thollot, Isabelle Nectoux, Alexandra Guidetti, Maryline Chaprier, Benjamin Bourgeois, Sarah Boisvineau, Catherine Barthélemy, Anthony Pouzot‐Nevoret, Céline Giger, Urs J Vet Intern Med SMALL ANIMAL BACKGROUND: Blood typing for the A and B antigens is essential and crossmatching testing is generally recommended before transfusing blood to cats. OBJECTIVE: To evaluate 2 crossmatch (XM) tests. ANIMALS: Forty‐nine healthy domestic shorthair cats that had not received a blood transfusion. METHODS: Prospective study. Blood samples were typed for AB using immunochromatographic and flow cytometric techniques. A gel column (GC) and a feline antiglobulin‐enhanced gel column (AGC) XM tests were used for crossmatching. RESULTS: The population included 34 type A, 13 B, and 2 AB cats, with concordant results (r = 1, P < .005) by flow cytometry and immunochromatographic strip kit. The plasma from type A cats had either no or weak anti‐B alloantibodies. The plasma of 12 of 13 type B cats contained strong anti‐A alloantibodies. For crossmatching, plasma to RBC pairings were prepared using the GC (n = 446) and AGC (n = 630) tests. Both methods showed compatibilities in 329 and incompatibilities in 102 pairings including all A‐B mismatches. Additionally 15 pairings showed agglutination by the AGC but not GC method. Fourteen incompatibilities outside the expected A‐B mismatches were only revealed by AGC. CONCLUSIONS AND CLINICAL IMPORTANCE: AB typing using immunochromatographic strip is as accurate as laboratory flow cytometry. The 2 XM methods had good agreement with additional incompatibilities being recognized by the AGC XM beyond A‐B incompatibilities. In clinic, feline AB typing and sensitive XM test kits are available and recommended before each transfusion, although the clinical implications of incompatible XM test results and clinical benefits of such crossmatching have not been documented. John Wiley & Sons, Inc. 2018-12-17 2019 /pmc/articles/PMC6430866/ /pubmed/30557453 http://dx.doi.org/10.1111/jvim.15381 Text en © 2018 The Authors. Journal of Veterinary Internal Medicine published by Wiley Periodicals, Inc. on behalf of the American College of Veterinary Internal Medicine. This is an open access article under the terms of the http://creativecommons.org/licenses/by-nc/4.0/ License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited and is not used for commercial purposes.
spellingShingle SMALL ANIMAL
Goy‐Thollot, Isabelle
Nectoux, Alexandra
Guidetti, Maryline
Chaprier, Benjamin
Bourgeois, Sarah
Boisvineau, Catherine
Barthélemy, Anthony
Pouzot‐Nevoret, Céline
Giger, Urs
Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
title Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
title_full Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
title_fullStr Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
title_full_unstemmed Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
title_short Detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
title_sort detection of naturally occurring alloantibody by an in‐clinic antiglobulin‐enhanced and standard crossmatch gel column test in non‐transfused domestic shorthair cats
topic SMALL ANIMAL
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6430866/
https://www.ncbi.nlm.nih.gov/pubmed/30557453
http://dx.doi.org/10.1111/jvim.15381
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