Complement and Non-Complement Binding Anti-HLA Antibodies Are Differentially Detected with Different Antigen Bead Assays in Renal Transplant Recipients

Author:

Ouranos Konstantinos1ORCID,Panteli Manolis23,Petasis Georgios23,Papachristou Marianthi2ORCID,Iosifidou Artemis Maria2,Iosifidou Myrto Aikaterini2,Anastasiou Aikaterini3,Samali Margarita3ORCID,Stangou Maria24ORCID,Theodorou Ioannis5ORCID,Lioulios Georgios24,Fylaktou Asimina3

Affiliation:

1. Department of Medicine, Houston Methodist Research Institute, Houston, TX 77030, USA

2. School of Medicine, Aristotle University of Thessaloniki, 45636 Thessaloniki, Greece

3. National Peripheral Histocompatibility Center, Department of Immunology, Hippokration Hospital, 54642 Thessaloniki, Greece

4. 1st Department of Nephrology, Hippokration Hospital, 54642 Thessaloniki, Greece

5. Laboratoire d’Immunologie, Hôpital Robert Debré, 75019 Paris, France

Abstract

Two semi-quantitative, Luminex-based, single-antigen bead (SAB) assays are available to detect anti-HLA antibodies and evaluate their reactivity with complement binding. Sera from 97 patients with positive panel reactive antibody tests (>5%) were analyzed with two SAB tests, Immucor (IC) and One-Lambda (OL), for anti-HLA antibody detection and the evaluation of their complement-binding capacity. IC detected 1608/8148 (mean fluorescent intensity (MFI) 4195 (1995–11,272)) and 1136/7275 (MFI 6706 (2647–13,184)) positive anti-HLA class I and II specificities, respectively. Accordingly, OL detected 1942/8148 (MFI 6185 (2855–12,099)) and 1247/7275 (MFI 9498 (3630–17,702)) positive anti-HLA class I and II specificities, respectively. For the IC assay, 428/1608 (MFI 13,900 (9540–17,999)) and 409/1136 (MFI 11,832 (7128–16,531)) positive class I and II specificities bound C3d, respectively. Similarly, OL detected 485/1942 (MFI 15,452 (9369–23,095)) and 298/1247 (MFI18,852 (14,415–24,707)) C1q-binding class I and II specificities. OL was more sensitive in detecting class I and II anti-HLA antibodies than IC was, although there was no significant difference in the number of class II specificities per case. MFI was higher for complement vs. non-complement-binding anti-HLA antibodies in both assays. Both methods were equal in detecting complement-binding anti-HLA class I antibodies, whereas the C3d assay was more sensitive in detecting complement-binding anti-HLA class II antibodies.

Publisher

MDPI AG

Subject

General Medicine

Reference25 articles.

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3. Evidence for antibody-mediated injury as a major determinant of late kidney allograft failure;Gaston;Transplantation,2010

4. Antibody-mediated rejection in kidney transplantation: A review of pathophysiology, diagnosis, and treatment options;Kim;Pharmacotherapy,2014

5. Failure to remove de novo donor-specific HLA antibodies is influenced by antibody properties and identifies kidney recipients with late antibody-mediated rejection destined to graft loss—A retrospective study;Cioni;Transpl. Int.,2019

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