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a Departments of Neurology,
b Biochemistry and Molecular Pharmacology,
c Cell Biology, University of Massachusetts Medical School, Worcester, Massachusetts, USA;
d Department of Neurology and Clinical Neurosciences, Stanford University, Palo Alto, California, USA
Key Words. Neural stem cells • Blastocyst injections • Differentiation • Pluripotency
Correspondence: Lawrence D. Recht, M.D., Department of Neurology, Stanford University Medical Center, 1201 Welch Road, Room P-208, Stanford, California 94305, USA. Telephone: 650-498-6320; Fax: 650-498-6262; e-mail: LRecht{at}stanford.edu
Earlier studies reported that neural stem (NS) cells injected into blastocysts appeared to be pluripotent, differentiating into cells of all three germ layers. In this study, we followed in vitro green fluorescent protein (GFP)labeled NS and embryonic stem (ES) cells injected into blastocysts. Forty-eight hours after injection, significantly fewer blastocysts contained GFP-NS cells than GFP-ES cells. By 96 hours, very few GFP-NS cells remained in blastocysts compared with ES cells. Moreover, 48 hours after injection, GFP-NS cells in blastocysts extended long cellular processes, ceased expressing the NS cell marker nestin, and instead expressed the astrocytic marker glial fibrillary acidic protein. GFP-ES cells in blastocysts remained morphologically undifferentiated, continuing to express the pluripotent marker stage-specific embryonic antigen-1. Selecting cells from the NS cell population that preferentially formed neurospheres for injection into blastocysts resulted in identical results. Consistent with this in vitro behavior, none of almost 80 mice resulting from NS cellinjected blastocysts replaced into recipient mothers were chimeric. These results strongly support the idea that NS cells cannot participate in chimera formation because of their rapid differentiation into glia-like cells. Thus, these results raise doubts concerning the pluripotency properties of NS cells.
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