A novel cryopreservation and biobanking strategy to study lymphoid tissue stromal cells in human disease

Author:

Brandstadter Joshua D.1,De Martin Angelina2,Lϋtge Mechthild2,Ferreira Antonio3,Gaudette Brian T.4,Stanossek Yves5,Wang Shumei3,Gonzalez Michael V.6,Camiolo Edward7,Wertheim Gerald7,Austin Bridget6,Allman David4ORCID,Bagg Adam4,Lim Megan S.8,Fajgenbaum David C.6,Aster Jon C.3,Ludewig Burkhard2,Maillard Ivan1

Affiliation:

1. Division of Hematology/Oncology Perelman School of Medicine University of Pennsylvania Philadelphia PA USA

2. Institute of Immunobiology Kantonsspital St. Gallen St. Gallen Switzerland

3. Department of Pathology Brigham and Women's Hospital, Harvard Medical School Boston MA USA

4. Department of Pathology and Laboratory Medicine, Perelman School of Medicine University of Pennsylvania Philadelphia PA USA

5. Department of Otorhinolaryngology, Head and Neck Surgery Kantonsspital St. Gallen St. Gallen Switzerland

6. Center for Cytokine Storm Treatment and Laboratory, Division of Translational Medicine and Human Genetics, Perelman School of Medicine University of Pennsylvania Philadelphia PA USA

7. Department of Pathology and Laboratory Medicine Children's Hospital of Philadelphia Philadelphia PA USA

8. Department of Pathology and Laboratory Medicine Memorial Sloan Kettering Cancer Center New York NY USA

Abstract

AbstractNonhematopoietic lymph node stromal cells (LNSCs) regulate lymphocyte trafficking, survival, and function for key roles in host defense, autoimmunity, alloimmunity, and lymphoproliferative disorders. However, the study of LNSCs in human diseases is complicated by a dependence on viable lymphoid tissues, which are most often excised prior to establishment of a specific diagnosis. Here, we demonstrate that cryopreservation can be used to bank lymphoid tissue for the study of LNSCs in human disease. Using human tonsils and lymph nodes (LN), lymphoid tissue fragments were cryopreserved for subsequent enzymatic digestion and recovery of viable nonhematopoietic cells. Flow cytometry and single‐cell transcriptomics identified comparable proportions of LN stromal cell types in fresh and cryopreserved tissue. Moreover, cryopreservation had little effect on transcriptional profiles, which showed significant overlap between tonsils and LN. The presence and spatial distribution of transcriptionally defined cell types were confirmed by in situ analyses. Our broadly applicable approach promises to greatly enable research into the roles of LNSCs in human disease.

Funder

National Cancer Institute

Doris Duke Charitable Foundation

National Institute of Allergy and Infectious Diseases

National Heart, Lung, and Blood Institute

Publisher

Wiley

Subject

Immunology,Immunology and Allergy

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