Natural Killer Cells Differentiate Human Adipose-Derived Stem Cells and Modulate Their Adipogenic Potential

Kameron S Rezzadeh; Akishige Hokugo; Anahid Jewett; Anna Kozlowska; Luis Andres Segovia; Patricia Zuk; Reza Jarrahy

doi:10.1097/PRS.0000000000001536

Natural Killer Cells Differentiate Human Adipose-Derived Stem Cells and Modulate Their Adipogenic Potential

Plast Reconstr Surg. 2015 Sep;136(3):503-510. doi: 10.1097/PRS.0000000000001536.

Authors

Kameron S Rezzadeh¹, Akishige Hokugo, Anahid Jewett, Anna Kozlowska, Luis Andres Segovia, Patricia Zuk, Reza Jarrahy

Affiliation

¹ Los Angeles, Calif. From the Regenerative Bioengineering and Repair Laboratory, Division of Plastic and Reconstructive Surgery, Department of Surgery, David Geffen School of Medicine at the University of California, Los Angeles; and the Division of Oral Biology and Oral Medicine, The Jane and Jerry Weintraub Center for Reconstructive Biotechnology, University of California, Los Angeles, School of Dentistry.

PMID: 26313823
DOI: 10.1097/PRS.0000000000001536

Abstract

Background: Natural killer cells are thought to represent more than 30 percent of all lymphocytes within the stromal vascular fraction of lipoaspirates. However, their physiologic interaction with adipocytes and their precursors has never been specifically examined. The authors hypothesized that natural killer cells, by means of cytokine secretion, are capable of promoting the differentiation of adipose-derived stem cells.

Methods: Human natural killer cells purified from healthy donors' peripheral blood mononuclear cells were activated with a combination of interleukin-2 and anti-CD16 monoclonal antibody; natural killer cell supernatant was collected. Adipose-derived stem cells isolated from raw human lipoaspirates from healthy patients were treated with growth media, growth media with natural killer cell supernatant, adipogenic media, and adipogenic media with natural killer cells supernatant. Flow cytometric analysis was performed on cells using antibodies against B7H1, CD36, CD44, CD34, CD29, and MHC-1. Adipogenic-related gene expression (PPAR-γ, LPL, GPD-1, and aP2) was assessed. Oil Red O staining was performed as a functional assay of adipocyte differentiation and adipogenesis.

Results: Adipose-derived stem cells maintained in growth media with natural killer cell supernatant lost markers of "stemness," including CD44, CD34, and CD29; and expressed markers of differentiation, including B7H1 and MHC-1. Adipose-derived stem cells treated with natural killer cell supernatant accumulated small amounts of lipid after 10 days of natural killer cell supernatant treatment. Adipose-derived stem cells treated with natural killer cell supernatant showed altered expression of adipogenesis-associated genes compared with cells maintained in growth media. Adipose-derived stem cells maintained in adipogenic media with natural killer cell supernatant accumulated less lipid than those cells in adipogenic media alone.

Conclusions: The authors demonstrate that, through secreted factors, natural killer cells are capable of differentiating adipose-derived stem cells. In cells maintained in adipogenic media, treatment with natural killer cell supernatant modulated adipogenic potential.

Publication types

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

MeSH terms

Adipocytes / physiology*
Adipogenesis / physiology*
Adult
Biomarkers / metabolism
Female
Flow Cytometry
Humans
Killer Cells, Natural / physiology*
Lipectomy
Middle Aged
Real-Time Polymerase Chain Reaction
Stem Cells / physiology*
Subcutaneous Fat / cytology

Substances

Biomarkers