Rapid Immunochromatographic Detection of Serum Anti-[alpha]-Galactosidase A Antibodies in Fabry Patients after Enzyme Replacement Therapy

We developed an immunochromatography-based assay for detecting antibodies against recombinant [alpha]-galactosidase A proteins in serum. The evaluation of 29 serum samples from Fabry patients, who had received enzyme replacement therapy with agalsidase alpha and/or agalsidase beta, was performed by...

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Veröffentlicht in:	PloS one 2015-06, Vol.10 (6)
Hauptverfasser:	Nakano, Sachie, Tsukimura, Takahiro, Togawa, Tadayasu, Ohashi, Toya, Kobayashi, Masahisa, Takayama, Katsuyoshi, Kobayashi, Yukuharu, Abiko, Hiroshi, Satou, Masatsugu, Nakahata, Tohru, Warnock, David G, Sakuraba, Hitoshi, Shibasaki, Futoshi
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Sprache:	eng
Schlagworte:	Antibodies Biopharmaceuticals Enzyme therapy Enzyme-linked immunosorbent assay Enzymes Gene therapy
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creator	Nakano, Sachie Tsukimura, Takahiro Togawa, Tadayasu Ohashi, Toya Kobayashi, Masahisa Takayama, Katsuyoshi Kobayashi, Yukuharu Abiko, Hiroshi Satou, Masatsugu Nakahata, Tohru Warnock, David G Sakuraba, Hitoshi Shibasaki, Futoshi
description	We developed an immunochromatography-based assay for detecting antibodies against recombinant [alpha]-galactosidase A proteins in serum. The evaluation of 29 serum samples from Fabry patients, who had received enzyme replacement therapy with agalsidase alpha and/or agalsidase beta, was performed by means of this assay method, and the results clearly revealed that the patients exhibited the same level of antibodies against both agalsidase alpha and agalsidase beta, regardless of the species of recombinant [alpha]-galactosidase A used for enzyme replacement therapy. A conventional enzyme-linked immunosorbent assay supported the results. Considering these, enzyme replacement therapy with agalsidase alpha or agalsidase beta would generate antibodies against the common epitopes in both agalsidase alpha and agalsidase beta. Most of the patients who showed immunopositive reaction exhibited classic Fabry phenotype and harbored gene mutations affecting biosynthesis of [alpha]-galactosidase A. As immunochromatography is a handy and simple assay system which can be available at bedside, this assay method would be extremely useful for quick evaluation or first screening of serum antibodies against agalsidase alpha or agalsidase beta in Fabry disease with enzyme replacement therapy.
doi_str_mv	10.1371/journal.pone.0128351
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The evaluation of 29 serum samples from Fabry patients, who had received enzyme replacement therapy with agalsidase alpha and/or agalsidase beta, was performed by means of this assay method, and the results clearly revealed that the patients exhibited the same level of antibodies against both agalsidase alpha and agalsidase beta, regardless of the species of recombinant [alpha]-galactosidase A used for enzyme replacement therapy. A conventional enzyme-linked immunosorbent assay supported the results. Considering these, enzyme replacement therapy with agalsidase alpha or agalsidase beta would generate antibodies against the common epitopes in both agalsidase alpha and agalsidase beta. Most of the patients who showed immunopositive reaction exhibited classic Fabry phenotype and harbored gene mutations affecting biosynthesis of [alpha]-galactosidase A. As immunochromatography is a handy and simple assay system which can be available at bedside, this assay method would be extremely useful for quick evaluation or first screening of serum antibodies against agalsidase alpha or agalsidase beta in Fabry disease with enzyme replacement therapy.</abstract><pub>Public Library of Science</pub><doi>10.1371/journal.pone.0128351</doi></addata></record>
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subjects	Antibodies Biopharmaceuticals Enzyme therapy Enzyme-linked immunosorbent assay Enzymes Gene therapy
title	Rapid Immunochromatographic Detection of Serum Anti-[alpha]-Galactosidase A Antibodies in Fabry Patients after Enzyme Replacement Therapy
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