Detection of Intragraft Anti-Blood Group A and B Antibodies Following Renal Transplantation

Tsukasa Nakamura; Takayuki Shirouzu; Shintaro Kawai; Yui Imanishi; Takehisa Matsuyama; Shumpei Harada; Shuji Nobori; Norio Yoshimura; Hidetaka Ushigome

doi:10.1016/j.transproceed.2019.01.128

Detection of Intragraft Anti-Blood Group A and B Antibodies Following Renal Transplantation

Transplant Proc. 2019 Jun;51(5):1371-1377. doi: 10.1016/j.transproceed.2019.01.128.

Authors

Tsukasa Nakamura¹, Takayuki Shirouzu², Shintaro Kawai², Yui Imanishi³, Takehisa Matsuyama⁴, Shumpei Harada⁴, Shuji Nobori⁴, Norio Yoshimura⁴, Hidetaka Ushigome⁴

Affiliations

¹ Department of Organ Transplantation and General Surgery, Kyoto Prefectural University of Medicine, Kajii-cho 465, Kamigyo-ku, Kyoto-prefecture, Japan. Electronic address: tsukasa@koto.kpu-m.ac.jp.
² Wakunaga Pharmaceutical Co, Ltd, Molecular Diagnostics Division, Osaka, Japan.
³ Department of Blood Transfusion and Cell Therapy, Kyoto Prefectural University of Medicine, Kyoto, Japan.
⁴ Department of Organ Transplantation and General Surgery, Kyoto Prefectural University of Medicine, Kajii-cho 465, Kamigyo-ku, Kyoto-prefecture, Japan.

PMID: 31155175
DOI: 10.1016/j.transproceed.2019.01.128

Abstract

Background: Graft immunocomplex capture fluorescence analysis is an attractive method to detect intragraft donor-specific anti-HLA antibodies. In ABO-incompatible transplantation, anti-A and B antibodies are also considered to be important donor specific antibodies (ABO-DSA). Therefore, it is useful to monitor intragraft ABO-DSAs to assess antibody-mediated rejection.

Methods: To capture A and B antigens, anti-Band III, von Willebrand factor (VW), and plasmalemma vesicle-associated protein (PLVAP) beads were produced. The allograft specimen was homogenized in a lysis buffer. Subsequently, A and B antigens were captured by anti-Band III, VW, or PLVAP beads. The immune complexes were then detected by phycoerythrin-conjugated anti-human IgG antibodies and analyzed using a Luminex system.

Results: Although Band III and VW beads yielded false positives and false negatives, PLVAP beads captured A and B antigens with high sensitivity (91.7%) and specificity (100%) when an index > 1.5 was considered positive. The proximity in A and B antigens and PLVAP expression was confirmed using immunohistochemical evaluation. Furthermore, sodium dodecyl sulfate polyacrylamide gel electrophoresis supported that PLVAP is an A and B antigen carrier protein.

Case report: Biopsies were conducted following an ABO-incompatible renal transplant (type A to O) and evaluated for ABO-DSA. Graft immunocomplex capture fluorescence analysis was demonstrated as follows: 3.19 (1 h, serum creatinine [s-Cr] 3.95 mg/dL, titer IgG 1:512, glomerulitis [g] 0, peritubular capillaritis [ptc] 0, complement 4d [C4d] 1); 1.8 (4 d, s-Cr 2.29 mg/dL, titer 1:256, g 0, ptc 0, C4d 3); 1.2 (22 d, s-Cr 1.58 mg/dL, titer 1:128, g 0, ptc 2, C4d 3). This result indicated that the remnant ABO-DSA were adsorbed and subsequently removed from the allograft successfully.

Conclusions: This novel application could be used to detect intragraft ABO-DSAs, which could lead to a correct diagnosis and shed light on the ABO-DSA kinetics following ABO-incompatible transplantation.

MeSH terms

Adult
Biopsy
Blood Group Antigens / analysis*
Female
Fluorescent Antibody Technique / methods*
Graft Rejection / immunology*
HLA Antigens / immunology
Humans
Isoantibodies / analysis*
Kidney Transplantation*
Male
Tissue Donors
Transplantation, Homologous

Substances

Blood Group Antigens
HLA Antigens
Isoantibodies