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The Journal of Neurophysiology Vol. 84 No. 1 July 2000, pp. 534-548
Copyright ©2000 by the American Physiological Society
1Department of Physiology, University of Utah School of Medicine, Salt Lake City 84108; and 2Department of Neurobiology and Anatomy, University of Utah School of Medicine, Salt Lake City, Utah 84132
Piper, David R.,
Tahmina Mujtaba,
Mahendra S. Rao, and
Mary T. Lucero.
Immunocytochemical and Physiological Characterization of a
Population of Cultured Human Neural Precursors. J. Neurophysiol. 84: 534-548, 2000. Human neural precursor
cells (HNPC) have recently become commercially available. In an effort
to determine the usefulness of these cells for in vitro studies, we
have grown cultured HNPCs (cHNPCs) according to the supplier
specifications. Here we report our characterization of cHNPCs under
nondifferentiating and differentiating growth conditions and make a
comparison to primary HNPCs (pHNPCs) obtained at the same developmental
time point from a different commercial supplier. We found that under
nondifferentiating conditions, cHNPCs expressed nestin, divided
rapidly, expressed few markers of differentiated cells, and displayed
both 4-aminopyridine (4-AP)-sensitive and delayed-rectifier type
K+ currents. No inward currents were observed. On changing
to differentiating culture conditions, a majority of the cells
expressed neuronal markers, did not divide, expressed inward and
outward time- and voltage-dependent currents, and responded to the
application of the neurotransmitters acetylcholine and glutamate. The
outward current densities were indistinguishable from those in
undifferentiated cells. The inward currents included TTX-sensitive and
-resistant Na+ currents, sustained Ca2+
currents, and an inwardly rectifying K+ current. Comparison
of the properties of differentiated cells from cHNPCs with neurons
obtained from primary fetal cultures (pHNPCs) revealed two major
differences: the differentiated cHNPCs did not express embryonic neural
cell adhesion molecule (E-NCAM) immunoreactivity but did co-express
GFAP immunoreactivity. The co-expression of neuronal and glial
markers was likely due to the growth of cells in serum containing
medium as the pHNPCs that were never exposed to serum did express
E-NCAM and did not co-express glial fibrillary acidic protein (GFAP).
The relevance of these results is discussed and compared with results
from other neuronal progenitor populations and cultured human neuronal cells.
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