Abstract
There are several methods available for the production of Schwann cell cultures from fetal and neonatal peripheral nervous tissue. We have investigated methods for producing Schwann cell-rich cultures from adult tissue. Dorsal root ganglia from normal adult cats were used to initiate explant cultures or subjected to primary dissociation. The resulting cultures were compared in terms of growth, the proportions of fibroblastic and Schwann-like cells in primary cultures and the effects of subculture on the relative frequency of these cell types. We found that excision and transfer of explanted ganglion pieces after 14 days in culture produced a secondary outgrowth rich in small, bipolar, spindle-shaped Schwann-like cells. Subculture of this outgrowth produced secondary cultures of predominantly Schwann-like cells with typical spindle-shaped morphology. The use of antimitotic agents in the media to inhibit fibroblast growth was not observed to be necessary or beneficial with this adult tissue. Primary dissociation of ganglia with enzymes (trypsin or collagenase) and mechanical agitation was even more effective in producing secondary cultures and cell lines that were, by morphological criteria, predominantly or exclusively Schwann-like cells. One of these Schwann-like cell lines, designated GSA, has been carried over 24 subcultures while retaining characteristic Schwann cell morphology. Cells of this line have been examined by scanning and transmission electron microscopy. Karyotype analysis indicates a chromosome complement consistent with the species of origin, a normal cat.
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