Collagen Type VI in Neural Crest Development: Distribution In Situ and Interaction With Cells In Vitro
Abstract
We have examined the spatiotemporal distribution of collagen type VI (Col VI) during neural crest development in vivo and its ability to promote neural crest cell attachment and migration in vitro. An affinity purified antiserum and chain-specific monoclonal antibodies against chicken Col VI were employed to immunolocalize the collagen in tissue sections and by immunoblotting. At stages of initial neural crest cell migration, the α1(VI) and α2(VI) chains were immunolocalized in apposition with basement membrances of the neural tube, somites, notochord and ectoderm, whereas no immunoreactivity was seen for the α3(VI) chain. Immunoblotting analysis confirmed the expression of α1(VI) and α2(VI) chains and the lack of detectable immunoreactivity for the α3(VI) chain at these early phases of neural crest development. Conversely, at advanced phases of migration and following gangliogenesis, expression of α3(VI) chain coincided with that of α1(VI) and α2(VI) chains in apposition with basement membrances, around the dorsal root ganglia, and in fibrillar arrangements within the developing dermis and ventral sclerotome. The ability of Col VI to promote neural crest cell attachment and migration was tested in vitro using quantitative assays for these processes. Both native microfilaments and isolated tetramers of Col VI strongly promoted neural crest cell attachment and migration. Optimal stimulation of neural crest cell adhesion and migration was dependent upon structural integrity of Col VI since unfolded and disassembled α chains only weakly promoted cell attachment and were virtually inactive in supporting cell movement. The importance of a native macromolecular organization of Col VI further was analyzed in experiments in which dissociated tetramers were reassociated by Ca^(2+)- and temperature-dependent self-aggregation. In contrast to native microfilaments, these oligomeric complexes were less effective in promoting neural crest cell movement, but still retained the ability to stimulate maximal cell attachment. The results indicate that Col VI is a primary component of the extracellular matrix deposited along neural crest migratory pathways, where it may participate in the regulation of cell movement by functioning as a migratory substrate. The ability of Col VI to promote neural crest cell adhesion and motility is highly dependent upon maintainance of a native macromolecular arrangement.
Additional Information
© 1993 Wiley-Liss, Inc. Received June 28, 1993; accepted August 26, 1993. Article first published online: 3 Feb 2005. The authors wish to thank Dr. Alfonso Colombatti for providing purified chicken Col VI, antibodies to chicken Col VI and for critical reading of the manuscript. We are indebted to Douglas Keene for performing the electron microscopy at The Shriners Hospital's Facilities which are supported in part by grants from the R. Blaine Bramble Medical Research Foundation and the Fred Mayer Charitable Trust. Scott Leibold, Tammy Dillon and Susan De Maggio are thanked for their assistance with cell adhesion assays and video time-lapse microscopy. Kristin Artinger, Bruce Donaldson, Laura Magris, and Paolo Pontonutti are gratefully acknowledged for their excellent technical assistance. The work was supported in part by grants USPHS HD-15527 to M.B.-F. and from the Shriners Hospital for Crippled Children to R.W.G.Additional details
- Eprint ID
- 65931
- DOI
- 10.1002/aja.1001980207
- Resolver ID
- CaltechAUTHORS:20160405-113538594
- R. Blaine Bramble Medical Research Foundation
- Fred Mayer Charitable Trust
- HD-15527
- U.S. Public Health Service (USPHS)
- Shriners Hospital for Crippled Children
- Created
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2016-04-06Created from EPrint's datestamp field
- Updated
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2021-11-10Created from EPrint's last_modified field