Isolation and Serum-Free Culture of Primary Schwann Cells from Human Fetal Peripheral Nerve

Isolation and Serum-Free Culture of Primary Schwann Cells from Human Fetal Peripheral Nerve

We have developed a method for isolating Schwann cells (SC) from human fetal peripheral nerve and maintaining these SC in vitro under serum-free conditions. This method yields essentially pure SC which have a bipolar, spindle-shaped morphology; align in fascicles; and express typical glial cell mark...

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Veröffentlicht in:Experimental neurology 1999-07, Vol.158 (1), p.1-8
Hauptverfasser: Lopez, T.J, De Vries, G.H
Format: Artikel
Sprache:eng
Schlagworte:
Antigens - immunology
Biological and medical sciences
Biomarkers
Cell Communication - physiology
Cell Culture Techniques
Coculture Techniques
Culture Media, Serum-Free - isolation & purification
dorsal root ganglia
Fibroblasts - cytology
Fibroblasts - metabolism
Fundamental and applied biological sciences. Psychology
Ganglia, Spinal - cytology
Ganglia, Spinal - embryology
Ganglia, Spinal - metabolism
Glial Fibrillary Acidic Protein - metabolism
Glycoproteins - metabolism
human Schwann cells
Humans
Immunoglobulin G - immunology
in vitro
Isolated neuron and nerve. Neuroglia
Myelin Basic Protein - immunology
Myelin Basic Protein - metabolism
Neurites - immunology
Neurites - metabolism
Protein Isoforms - metabolism
Schwann Cells - cytology
Schwann Cells - immunology
Schwann Cells - metabolism
serum-free culture
Vertebrates: nervous system and sense organs
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Zusammenfassung:We have developed a method for isolating Schwann cells (SC) from human fetal peripheral nerve and maintaining these SC in vitro under serum-free conditions. This method yields essentially pure SC which have a bipolar, spindle-shaped morphology; align in fascicles; and express typical glial cell markers. Human fetal SC can be maintained for months under serum-free conditions with the neuregulin NDFβ. These human fetal SC can mimic axonal contact in vivo by retaining the functional capacity to strongly associate with neurites of cultured human fetal dorsal root ganglia. These isolation, culture, and coculture techniques provide a method for investigating SC–neuron interactions as well as development and function of human fetal SC.
ISSN:0014-4886
1090-2430
DOI:10.1006/exnr.1999.7081