Short-term assays for mesenchymal stromal cell immunosuppression of T-lymphocytes

Maryanne C Herzig; Barbara A Christy; Robbie K Montgomery; Carolina Cantu-Garza; Gema D Barrera; Ji H Lee; Nicholas Mucha; Jennifer R Talackine; Isaac A Abaasah; James A Bynum; Andrew P Cap

doi:10.3389/fimmu.2023.1225047

Short-term assays for mesenchymal stromal cell immunosuppression of T-lymphocytes

Front Immunol. 2023 Sep 26:14:1225047. doi: 10.3389/fimmu.2023.1225047. eCollection 2023.

Affiliations

¹ Blood and Shock Research, US Army Institute of Surgical Research, Fort Sam Houston, TX, United States.
² Department of Surgery, University of Texas, Health Science Center, San Antonio, TX, United States.

Abstract

Introduction: Trauma patients are susceptible to coagulopathy and dysfunctional immune responses. Mesenchymal stromal cells (MSCs) are at the forefront of the cellular therapy revolution with profound immunomodulatory, regenerative, and therapeutic potential. Routine assays to assess immunomodulation activity examine MSC effects on proliferation of peripheral blood mononuclear cells (PBMCs) and take 3-7 days. Assays that could be done in a shorter period of time would be beneficial to allow more rapid comparison of different MSC donors. The studies presented here focused on assays for MSC suppression of mitogen-stimulated PBMC activation in time frames of 24 h or less.

Methods: Three potential assays were examined-assays of apoptosis focusing on caspase activation, assays of phosphatidyl serine externalization (PS+) on PBMCs, and measurement of tumor necrosis factor alpha (TNFα) levels using rapid ELISA methods. All assays used the same initial experimental conditions: cryopreserved PBMCs from 8 to 10 pooled donors, co-culture with and without MSCs in 96-well plates, and PBMC stimulation with mitogen for 2-72 h.

Results: Suppression of caspase activity in activated PBMCs by incubation with MSCs was not robust and was only significant at times after 24 h. Monitoring PS+ of live CD3+ or live CD4+/CD3+ mitogen-activated PBMCs was dose dependent, reproducible, robust, and evident at the earliest time point taken, 2 h, although no increase in the percentage of PS+ cells was seen with time. The ability of MSC in co-culture to suppress PBMC PS+ externalization compared favorably to two concomitant assays for MSC co-culture suppression of PBMC proliferation, at 72 h by ATP assay, or at 96 h by fluorescently labeled protein signal dilution. TNFα release by mitogen-activated PBMCs was dose dependent, reproducible, robust, and evident at the earliest time point taken, with accumulating signal over time. However, suppression levels with MSC co-culture was reliably seen only after 24 h.

Discussion: Takeaways from these studies are as follows: (1) while early measures of PBMC activation is evident at 2-6 h, immunosuppression was only reliably detected at 24 h; (2) PS externalization at 24 h is a surrogate assay for MSC immunomodulation; and (3) rapid ELISA assay detection of TNFα release by PBMCs is a robust and sensitive assay for MSC immunomodulation at 24 h.

Keywords: IL-6; caspase; cytokine; mesenchymal stromal cell; peripheral blood mononuclear cells; phosphatidyl serine; tNF-alpha.

Publication types

Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

Caspases
Humans
Immunosuppression Therapy / methods
Intercellular Signaling Peptides and Proteins / pharmacology
Leukocytes, Mononuclear
Mesenchymal Stem Cells*
Mitogens / pharmacology
T-Lymphocytes*
Tumor Necrosis Factor-alpha / pharmacology

Substances

Tumor Necrosis Factor-alpha
Mitogens
Intercellular Signaling Peptides and Proteins
Caspases

Grants and funding

This research was funded by the United States Army Medical Research and Development Command and by the Medical Technology Enterprise Consortium, grants MTEC-16-01-Regen-02 and MTEC-19-07-Biomfg-004.