Ultrastructural and tissue-culture studies on the role of fibronectin, collagen and glycosaminoglycans in the migration of neural crest cells in the fowl embryo

Ultrastructural and tissue-culture studies on the role of fibronectin, collagen and glycosaminoglycans in the migration of neural crest cells in the fowl embryo

The initial migration of neural crest (NC) cells into cell-free space was studied by transmission electron microscopy at trunk levels of fowl embryos, some of which were fixed in the presence of ruthenium red. Migrating NC cells occurred in zones which contained fewer ruthenium-red stained 15-40nm d...

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Veröffentlicht in:Cell and tissue research 1982, Vol.221 (3), p.521-549
Hauptverfasser: Newgreen, D F, Gibbins, I L, Sauter, J, Wallenfels, B, Wütz, R
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Cell Movement - drug effects
Collagen - pharmacology
Extracellular Space - physiology
Fibronectins - pharmacology
Glycosaminoglycans - pharmacology
Microscopy, Electron
Neural Crest - drug effects
Neural Crest - physiology
Neural Crest - ultrastructure
Poultry - physiology
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container_end_page 549
container_issue 3
container_start_page 521
container_title Cell and tissue research
container_volume 221
creator Newgreen, D F
Gibbins, I L
Sauter, J
Wallenfels, B
Wütz, R
description The initial migration of neural crest (NC) cells into cell-free space was studied by transmission electron microscopy at trunk levels of fowl embryos, some of which were fixed in the presence of ruthenium red. Migrating NC cells occurred in zones which contained fewer ruthenium-red stained 15-40nm diameter granules than other regions. The ruthenium-red stained granules were linked by similarly stained thin (greater than 3nm diameter) microfibrils. The granules resemble proteoglycan and the microfibrils may be hyaluronate. NC cells contacted thicker (greater than 10 nm diameter) fibrils and interstitial bodies, which did not require ruthenium red for visualization. Cytoplasmic microfilaments were sometimes aligned at the point of contact with the extracellular fibrils, which may be fibronectin and collagen. Phase-contrast time-lapse videotaping and scanning electron microscopy showed that NC cells of the fowl embryo in vitro migrated earlier and more extensively on glass coated with fibronectin-rich fibrous material and adsorbed fibronectin molecules than on glass coated with collagen type I (fibres and adsorbed molecules). NC cells became completely enmeshed in fibronectin-rich fibres, but generally remained on the surface of collagen-fibre gels. When given a choice, NC cells strongly preferred fibronectin coatings to plain glass, and plain glass to dried collagen gels. NC cells showed a slight preference for plain glass over glass to which collagen was adsorbed. Addition to the culture medium of hyaluronate (initial conc. 20 mg/ml), chondroitin (5 mg/ml) and fully sulphated chondroitin sulphate and dermatan sulphate (up to 10 mg/ml) did not drastically alter NC cell migration on fibronectin-rich fibrous substrates.
doi_str_mv 10.1007/bf00215700
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source MEDLINE; SpringerNature Journals
subjects Animals
Cell Movement - drug effects
Collagen - pharmacology
Extracellular Space - physiology
Fibronectins - pharmacology
Glycosaminoglycans - pharmacology
Microscopy, Electron
Neural Crest - drug effects
Neural Crest - physiology
Neural Crest - ultrastructure
Poultry - physiology
title Ultrastructural and tissue-culture studies on the role of fibronectin, collagen and glycosaminoglycans in the migration of neural crest cells in the fowl embryo
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