Characterizing the antibody response to amustaline/glutathione pathogen-reduced red blood cells

Christopher Karim; Anil Panigrahi; Ronald G Pearl; Neel R Sodha; Thomas M Beaver; J Peter R Pelletier; Gregory A Nuttall; T Brett Reece; Anna Erickson; Teresa Hedrick; Kathy Liu; Stanley Bentow; Laurence Corash; Nina Mufti; Jeanne Varrone; Richard J Benjamin

doi:10.1111/trf.18117

Characterizing the antibody response to amustaline/glutathione pathogen-reduced red blood cells

Transfusion. 2024 Dec 25. doi: 10.1111/trf.18117. Online ahead of print.

Authors

Christopher Karim¹, Anil Panigrahi², Ronald G Pearl², Neel R Sodha³, Thomas M Beaver⁴, J Peter R Pelletier⁴, Gregory A Nuttall⁵, T Brett Reece⁶, Anna Erickson¹, Teresa Hedrick¹, Kathy Liu¹, Stanley Bentow¹, Laurence Corash¹, Nina Mufti¹, Jeanne Varrone¹, Richard J Benjamin¹

Affiliations

¹ Cerus Corporation, Concord, California, USA.
² Stanford University, Stanford, California, USA.
³ Rhode Island Hospital, Providence, Rhode Island, USA.
⁴ University of Florida, Gainesville, Florida, USA.
⁵ Mayo Clinic, Rochester, Minnesota, USA.
⁶ University of Colorado Hospital, Denver, Colorado, USA.

PMID: 39719927
DOI: 10.1111/trf.18117

Abstract

Background: The clinical significance of natural and treatment-emergent antibodies specific for amustaline/glutathione pathogen-reduced red blood cells (PRRBCs) is not known.

Study design and methods: A Phase 3, randomized clinical trial of PRRBCs (ReCePI) compared PRRBCs with conventional RBCs in cardiac or thoracic-aorta surgery. Subjects transfused during and for 7 days after surgery were screened for PRRBC-specific antibodies at baseline, 28 and 75 days post-surgery. Subjects with treatment-emergent antibodies were assessed for evidence of hemolysis. Cryopreserved subject RBC samples were assayed by flow cytometry for circulating PRRBCs using an acridine-specific (2S197-2M1) monoclonal antibody, and for human IgG-coated RBCs. RBC-surface acridine density was quantitated using a commercial calibrated phycoerythrin (PE)-bead panel.

Results: Five of 159 (3.1%) PRRBC and zero of 162 conventional RBC recipients developed treatment-emergent PRRBC-specific IgG, low titer antibodies detected 26-80 days post-surgery after exposure to 1-3 PRRBC units, without clinical evidence of hemolysis. DAT and eluate were weak (w+) positive and PRRBC-specific in one subject. A monocyte monolayer assay (MMA) was non-reactive in the three subjects with an interpretable result. Flow cytometry demonstrated circulating PRRBCs in all five subjects expressing surface acridine concentrations at the limit of detection (approximately 150-301 PE molecules/RBC) compared with freshly transfused PRRBCs (approximately 7500 PE molecules/RBC). In some samples, loss of surface acridine expression could not be distinguished from clearance of the PRRBCs.

Discussion: Treatment-emergent PRRBC-specific antibodies with the characteristics of nonclinically significant antibodies were detected in five subjects transfused with PRRBCs. Flow cytometry demonstrated persistent circulating PRRBCs with minimal surface acridine expression. (www.

Clinicaltrials: gov Identifier NCT03459287).

Keywords: RBCs; antibodies; pathogen reduction.

Associated data

ClinicalTrials.gov/NCT03459287

Grants and funding

HHS010020160009c/Biomedical Advanced Research and Development Authority