Epigenetic reprogramming induces the expansion of cord blood stem cells
Pratima Chaurasia, … , Sunita D’Souza, Ronald Hoffman
Pratima Chaurasia, … , Sunita D’Souza, Ronald Hoffman
Published April 24, 2014
Citation Information: J Clin Invest. 2014;124(6):2378-2395. https://doi.org/10.1172/JCI70313.
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Epigenetic reprogramming induces the expansion of cord blood stem cells

Abstract

Cord blood (CB) cells that express CD34 have extensive hematopoietic capacity and rapidly divide ex vivo in the presence of cytokine combinations; however, many of these CB CD34+ cells lose their marrow-repopulating potential. To overcome this decline in function, we treated dividing CB CD34+ cells ex vivo with several histone deacetylase inhibitors (HDACIs). Treatment of CB CD34+ cells with the most active HDACI, valproic acid (VPA), following an initial 16-hour cytokine priming, increased the number of multipotent cells (CD34+CD90+) generated; however, the degree of expansion was substantially greater in the presence of both VPA and cytokines for a full 7 days. Treated CD34+ cells were characterized based on the upregulation of pluripotency genes, increased aldehyde dehydrogenase activity, and enhanced expression of CD90, c-Kit (CD117), integrin α6 (CD49f), and CXCR4 (CD184). Furthermore, siRNA-mediated inhibition of pluripotency gene expression reduced the generation of CD34+CD90+ cells by 89%. Compared with CB CD34+ cells, VPA-treated CD34+ cells produced a greater number of SCID-repopulating cells and established multilineage hematopoiesis in primary and secondary immune–deficient recipient mice. These data indicate that dividing CB CD34+ cells can be epigenetically reprogrammed by treatment with VPA so as to generate greater numbers of functional CB stem cells for use as transplantation grafts.

Authors

Pratima Chaurasia, David C. Gajzer, Christoph Schaniel, Sunita D’Souza, Ronald Hoffman

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Figure 4

Effect of VPA on the different cell cycle phases of CD34+CD90+ cells.

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Effect of VPA on the different cell cycle phases of CD34+CD90+ cells. (A...
(A) Flow cytometric cell cycle analysis of CD34+CD90+ cells following SF culture under control (upper panel: 26.4%) conditions or cultures containing VPA (lower panel: 82.9%) for 7 days, with corresponding dot plots showing cells in different phases of the cell cycle by BrdU pulse labeling (2.5 hours) and staining with 7AAD (G0/G1, S, and G2/M). One of three representative experiments is shown. (B) Percentage of CD34+CD90+ cells that were in different phases of the cell cycle. A significant increase in the number of CD34+CD90+ cells was observed in G0/G1 (*P < 0.05), S (*P < 0.05), and G2/M (****P < 0.0001) phases in the VPA-containing cultures (mean ± SD; ANOVA, P < 0.002; n = 3).