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First published online November 1, 2007
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2007-0567v1
26/2/330    most recent
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Submitted on July 17, 2007
Accepted on October 25, 2007

TISSUE-SPECIFIC STEM CELLS

Characterization of Transplanted GFP+ Bone Marrow Cells into Adipose Tissue

Koji Tomiyama 1, Noriko Murase 1, Donna Beer Stolz 2, Hideyoshi Toyokawa 1, Daniel R. O'Donnell 3, Darren M. Smith 3, Jason R. Dudas 3, J. Peter Rubin 4, Kacey G. Marra 5*

1 Thomas E. Starzl Transplantation Institute, Department of Surgery, University of Pittsburgh, Pittsburgh, PA
2 Department of Cell Biology and Physiology, University of Pittsburgh, Pittsburgh, PA, McGowan Institute for Regenerative Medicine, Pittsburgh, PA
3 Division of Plastic Surgery, Department of Surgery, University of Pittsburgh, Pittsburgh, PA
4 McGowan Institute for Regenerative Medicine, Pittsburgh, PA, Division of Plastic Surgery, Department of Surgery, University of Pittsburgh, Pittsburgh, PA
5 McGowan Institute for Regenerative Medicine, Pittsburgh, PA, Division of Plastic Surgery, Department of Surgery, University of Pittsburgh, Pittsburgh, PA, Department of Bioengineering, University of Pittsburgh, Pittsburgh, PA

* To whom correspondence should be addressed. E-mail: marrak{at}upmc.edu.


  Abstract

Following transplantation of green fluorescent protein (GFP)-labeled bone marrow (BM) into irradiated, wild-type Sprague-Dawley rats, propagated GFP+ cells migrate to adipose tissue compartments. In order to determine the relationship between GFP+ BM-derived cells and tissue resident GFP- cells on the stem cell population of adipose tissue, we conducted detailed immunohistochemical analysis of chimeric whole fat compartments and subsequently isolated and characterized adipose-derived stem cells (ASCs) from GFP+ BM chimeras. In immunohistochemistry, a large fraction of GFP+ cells in adipose tissue were strongly positive for CD45 and smooth muscle actin, and evenly scattered around the adipocytes and blood vessels, while all CD45+ cells within the blood vessels were GFP+. A small fraction of GFP+ cells with mesenchymal marker CD90 also existed in the perivascular area. Flow cytometric and immunocytochemical analyses showed that cultured ASCs were CD45-/CD90+/CD29+. There was a significant difference in both the cell number and phenotype of the GFP+ ASCs in two different adipose compartments, the omental (abdominal) and the inguinal fat (subcutaneous) pad; a significantly higher number of GFP-/CD90+ cells were isolated from the subcutaneous depot as compared to the abdominal depot. The in vitro adipogenic differentiation of the ASCs was achieved; however, all cells that had differentiated were GFP-. Based on phenotypical analysis, GFP+ cells in adipose tissue in this rat model appear to be of both hematopoietic and mesenchymal origin; however, infrequent isolation of GFP+ ASCs and their lack of adipogenic differentiation suggest that the contribution of BM to ASCs generation might be minor.

Key Words. adipose, chimera, stem cell, GFP






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