A portable surface plasmon resonance (SPR) sensor for the detection of immunoglobulin A in plasma

Author:

Dubois Caroline1ORCID,Ducas Éric2,Laforce‐Lavoie Audrey2ORCID,Robidoux Jonathan2ORCID,Delorme Alexandre1ORCID,Live Ludovic S.3,Brouard Danny2,Masson Jean‐François1ORCID

Affiliation:

1. Département de Chimie, Quebec Center for Advanced Materials, Regroupement Québécois sur les Matériaux de Pointe, and Centre Interdisciplinaire de Recherche sur le Cerveau et l'Apprentissage, Institut Courtois Université de Montréal Montréal Canada

2. Héma‐Québec, Affaires Médicales et Innovation Québec City Québec Canada

3. Affinité Instruments Montréal Québec Canada

Abstract

AbstractBackgroundA life‐threatening anaphylactic shock can occur if a patient with undiagnosed immunoglobulin A (IgA) deficiency (i.e., IgA levels <500 ng/mL) receives IgA‐containing blood, hence the need for a rapid, point‐of‐care (POC) method for IgA deficiency screening. Enzyme‐linked immunosorbent assay (ELISA) is routinely used to detect IgA, but this method requires trained specialists and ≥24 h to obtain a result. We developed a surface plasmon resonance (SPR)‐based protocol to identify IgA‐deficient patients or donors within 1 h.Materials and MethodsThe SPR sensor relies on the detection of IgAs captured by primary antibodies adsorbed on the SPR chip and quantified with secondary antibodies. The sensor was calibrated from 0 to 2000 ng/mL in buffer, IgA‐depleted human serum, and plasma samples from IgA‐deficient individuals. A critical concentration of 500 ng/mL was set for IgA deficiency. The optimized sensor was then tested on eight plasma samples with known IgA status (determined by ELISA), including five with IgA deficiency and three with normal IgA levels.ResultsThe limit of detection was estimated at 30 ng/mL in buffer and 400 ng/mL in diluted plasma. The results obtained fully agreed with ELISA among the eight plasma samples tested. The protocol distinguished IgA‐deficient from normal samples, even for samples with an IgA concentration closer to critical concentration.DiscussionIn conclusion, we developed a reliable POC assay for the quantification of IgA in plasma. This test may permit POC testing at blood drives and centralized centers to maintain reserves of IgA‐deficient blood and in‐hospital testing of blood recipients.

Funder

Mitacs

Université de Montréal

Publisher

Wiley

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