Diabetic Kidney Disease Alters the Transcriptome and Function of Human Adipose-Derived Mesenchymal Stromal Cells but Maintains Immunomodulatory and Paracrine Activities Important for Renal Repair

Author:

Hickson LaTonya J.12ORCID,Eirin Alfonso1,Conley Sabena M.1,Taner Timucin34,Bian Xiaohui15,Saad Ahmed1,Herrmann Sandra M.1,Mehta Ramila A.6,McKenzie Travis J.3,Kellogg Todd A.3,Kirkland James L.278,Tchkonia Tamar278,Saadiq Ishran M.1,Tang Hui1,Jordan Kyra L.1,Zhu Xiangyang1,Griffin Mathew D.9,Rule Andrew D.1,van Wijnen Andre J.10,Textor Stephen C.1,Lerman Lilach O.1

Affiliation:

1. Division of Nephrology and Hypertension, Department of Medicine, Mayo Clinic, Rochester, MN

2. Division of Geriatric Medicine and Gerontology, Department of Medicine, Mayo Clinic, Rochester, MN

3. Department of Surgery, Mayo Clinic, Rochester, MN

4. Department of Immunology, Mayo Clinic, Rochester, MN

5. Department of Nephrology, Shengjing Hospital of China Medical University, Shenyang, China

6. Division of Clinical Trials and Biostatistics, Department of Quantitative Health Sciences, Mayo Clinic, Rochester, MN

7. Robert and Arlene Kogod Center on Aging, Mayo Clinic, Rochester, MN

8. Department of Physiology and Engineering, Mayo Clinic, Rochester, MN

9. Regenerative Medicine Institute (REMEDI) at CÚRAM SFI Centre for Research in Medical Devices, School of Medicine, National University of Ireland Galway, Galway, Ireland

10. Orthopedic Surgery, Mayo Clinic, Rochester, MN

Abstract

Mesenchymal stem/stromal cells (MSCs) facilitate repair in experimental diabetic kidney disease (DKD). However, the hyperglycemic and uremic milieu may diminish regenerative capacity of patient-derived therapy. We hypothesized that DKD reduces human MSC paracrine function. Adipose-derived MSC from 38 participants with DKD and 16 control subjects were assessed for cell surface markers, trilineage differentiation, RNA sequencing (RNA-seq), in vitro function (coculture or conditioned medium experiments with T cells and human kidney cells [HK-2]), secretome profile, and cellular senescence abundance. The direction of association between MSC function and patient characteristics were also tested. RNA-seq analysis identified 353 differentially expressed genes and downregulation of several immunomodulatory genes/pathways in DKD-MSC versus Control-MSC. DKD-MSC phenotype, differentiation, and tube formation capacity were preserved, but migration was reduced. DKD-MSC with and without interferon-γ priming inhibited T-cell proliferation greater than Control-MSC. DKD-MSC medium contained higher levels of anti-inflammatory cytokines (indoleamine 2,3-deoxygenase 1 and prostaglandin-E2) and prorepair factors (hepatocyte growth factor and stromal cell–derived factor 1) but lower IL-6 versus control-MSC medium. DKD-MSC medium protected high glucose plus transforming growth factor-β–exposed HK-2 cells by reducing apoptotic, fibrotic, and inflammatory marker expression. Few DKD-MSC functions were affected by patient characteristics, including age, sex, BMI, hemoglobin A1c, kidney function, and urine albumin excretion. However, senescence-associated β-galactosidase activity was lower in DKD-MSC from participants on metformin therapy. Therefore, while DKD altered the transcriptome and migratory function of culture-expanded MSCs, DKD-MSC functionality, trophic factor secretion, and immunomodulatory activities contributing to repair remained intact. These observations support testing of patient-derived MSC therapy and may inform preconditioning regimens in DKD clinical trials.

Publisher

American Diabetes Association

Subject

Endocrinology, Diabetes and Metabolism,Internal Medicine

Reference67 articles.

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