COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?

Manon J, Evrard R, Fievé L, et al. COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?. Orthop Procs. 2024;106-B(SUPP_2):124-124. doi:10.1302/1358-992X.2024.2.124

Manon, J., et al. “COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?.” Orthopaedic Proceedings, vol. 106-B, no. SUPP_2, 2024, pp. 124-124., https://doi.org/10.1302/1358-992X.2024.2.124

Manon, J., Evrard, R., Fievé, L., Xhema, D., Maistriaux, L., Schubert, T., Lengelé, B., Behets, C., & Cornu, O. (2024). COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?. Orthopaedic Proceedings, 106-B(SUPP_2), 124-124. https://doi.org/10.1302/1358-992X.2024.2.124

Manon, J., Evrard, R., Fievé, L., Xhema, D., Maistriaux, L., Schubert, T. et al. (2024) “COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?.” Orthopaedic Proceedings, 106-B(SUPP_2), pp. 124-124. Available at: https://doi.org/10.1302/1358-992X.2024.2.124

Manon, J., R. Evrard, L. Fievé, D. Xhema, L. Maistriaux, T. Schubert, B. Lengelé, C. Behets, and O. Cornu. “COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?.” Orthopaedic Proceedings 106-B, no. SUPP_2 (2024): 124-124. https://doi.org/10.1302/1358-992X.2024.2.124

Manon J, Evrard R, Fievé L, Xhema D, Maistriaux L, Schubert T, et al. COULD A DECELLULARIZATION PROTOCOL BE VALIDATED WITHOUT TALKING ABOUT HUMAN LEUKOCYTE ANTIGEN?. Orthop Procs. 2024 Jan 2;106-B(SUPP_2):124-124. https://doi.org/10.1302/1358-992X.2024.2.124

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Abstract

Decellularization techniques have advanced to reduce the risk of immune rejection in transplantation. Validation of these protocols typically relies on Crapo's criteria¹, which include the absence of visible nuclei and low DNA content. In our study, five decellularization protocols were compared to determine the optimal approach for human fascia lata (HFL) samples. However, our findings raised questions as to why recipients can still develop immunity despite meeting validation criteria.

HFL samples were decellularized using four protocols with SDS-Triton X100-DNase (D1 to D4-HFL) and one protocol using solvent-detergent-based baths (D5-HFL). The decellularized samples (D-HFL) were compared to native samples (N-HFL) using histology, and DNA content was measured. The human leukocyte antigen (HLA) content within the matrix was assessed using western blot analysis. Both D-HFL and N-HFL samples, along with negative control patches, were implanted in the backs of 28 Wistar rats. Anti-human IgG serum levels were evaluated after one month.

H&E and Hoechst staining revealed the absence of residual cells in all decellularization protocols. DNA content was consistently below the critical threshold (p<0.05). All implanted D-HFL samples resulted in significantly lower anti-human IgG levels compared to N-HFL (p<0.01). However, 2.5 out of 4 rats developed immunity after being implanted with D1 to D4-HFL, with varying levels of anti-human IgG. Only rats implanted with D5-HFL showed undetectable levels of IgG and were considered non-immunized. Western blot analysis indicated that only D5-HFL had a residual HLA content below 1%.

The literature on decellularization has primarily relied on Crapo's criteria, which do not consider the role of HLA mismatch in acute immune rejection. Our results suggest that a residual HLA content below 1% should also be considered to prevent immunization, even if other validation criteria are met. Further research is needed to evaluate the impact of residual HLA levels on human allotransplantation outcomes.

Email: julie.manon@uclouvain.be