Alterations in neural crest migration by a monoclonal antibody that affects cell adhesion.

The possible role of a 140-kD cell surface complex in neural crest adhesion and migration was examined using a monoclonal antibody JG22, first described by Greve and Gottlieb (1982, J. Cell. Biochem. 18:221-229). The addition of JG22 to neural crest cells in vitro caused a rapid change in morphology of cells plated on either fibronectin or laminin substrates. The cells became round and phase bright, often detaching from the dish or forming aggregates of rounded cells. Other tissues such as somites, notochords, and neural tubes were unaffected by the antibody in vitro even though the JG22 antigen is detectable in embryonic tissue sections on the surface of the myotome, neural tube, and notochord. The effects of the JG22 on neural crest migration in vivo were examined by a new perturbation approach in which both the antibody and the hybridoma cells were microinjected onto neural crest pathways. Hybridoma cells were labeled with a fluorescent cell marker that is nondeleterious and that is preserved after fixation and tissue sectioning. The JG22 antibody and hybridoma cells caused a marked reduction in cranial neural crest migration, a build-up of neural crest cells within the lumen of the neural tube, and some migration along aberrant pathways. Neural crest migration in the trunk was affected to a much lesser extent. In both cranial and trunk regions, a cell free zone of one or more cell diameters was generally observed between neural crest cells and the JG22 hybridoma cells. Two other monoclonal antibodies, 1-B and 1-N, were used as controls. Both 1-B and 1-N bind to bands of the 140-kD complex precipitated by JG22. Neither control antibody affected neural crest adhesion in vitro or neural crest migration in situ. This suggests that the observed alterations in neural crest migration are due to a functional block of the 140-kD complex.

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A monoclonal antibody against a laminin-heparan sulfate proteoglycan complex perturbs cranial neural crest migration in vivo.

The Journal of Cell Biology ◽

10.1083/jcb.106.4.1321 ◽

1988 ◽

Vol 106 (4) ◽

pp. 1321-1329 ◽

Cited By ~ 103

Author(s):

M Bronner-Fraser ◽

T Lallier

Keyword(s):

Monoclonal Antibody ◽

Heparan Sulfate ◽

Neural Crest ◽

Neural Tube ◽

Neural Crest Cells ◽

Heparan Sulfate Proteoglycan ◽

Sulfate Proteoglycan ◽

Cranial Neural Crest ◽

Neural Crest Migration

INO (inhibitor of neurite outgrowth) is a monoclonal antibody that blocks axon outgrowth, presumably by functionally blocking a laminin-heparan sulfate proteoglycan complex (Chiu, A. Y., W. D. Matthew, and P. H. Patterson. 1986. J. Cell Biol. 103: 1382-1398). Here the effect of this antibody on avian neural crest cells was examined by microinjecting INO onto the pathways of cranial neural crest migration. After injection lateral to the mesencephalic neural tube, the antibody had a primarily unilateral distribution. INO binding was observed in the basal laminae surrounding the neural tube, ectoderm, and endoderm, as well as within the cranial mesenchyme on the injected side of the embryo. This staining pattern was indistinguishable from those observed with antibodies against laminin or heparan sulfate proteoglycan. The injected antibody remained detectable for 18 h after injection, with the intensity of immuno-reactivity decreasing with time. Embryos ranging from the neural fold stage to the 9-somite stage were injected with INO and subsequently allowed to survive for up to 1 d after injection. These embryos demonstrated severe abnormalities in cranial neural crest migration. The predominant defects were ectopic neural crest cells external to the neural tube, neural crest cells within the lumen of the neural tube, and neural tube deformities. In contrast, embryos injected with antibodies against laminin or heparan sulfate proteoglycan were unaffected. When embryos with ten or more somites were injected with INO, no effects were noted, suggesting that embryos are sensitive for only a limited time during their development. Immunoprecipitation of the INO antigen from 2-d chicken embryos revealed a 200-kD band characteristic of laminin and two broad smears between 180 and 85 kD, which were resolved into several bands at lower molecular mass after heparinase digestion. These results indicate that INO precipitates both laminin and proteoglycans bearing heparan sulfate residues. Thus, microinjection of INO causes functional blockage of a laminin-heparan sulfate proteoglycan complex, resulting in abnormal cranial neural crest migration. This is the first evidence that a laminin-heparan sulfate proteoglycan complex is involved in aspects of neural crest migration in vivo.

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Regulation of the onset of neural crest migration by coordinated activity of BMP4 and Noggin in the dorsal neural tube

Development ◽

10.1242/dev.126.21.4749 ◽

1999 ◽

Vol 126 (21) ◽

pp. 4749-4762 ◽

Cited By ~ 22

Author(s):

D. Sela-Donenfeld ◽

C. Kalcheim

Keyword(s):

Neural Crest ◽

Neural Tube ◽

Specific Inhibitor ◽

Neural Crest Cells ◽

Concomitant Treatment ◽

Neural Tubes ◽

Dorsal Neural Tube ◽

Dependent Inhibition ◽

Neural Crest Migration

For neural crest cells to engage in migration, it is necessary that epithelial premigratory crest cells convert into mesenchyme. The mechanisms that trigger cell delamination from the dorsal neural tube remain poorly understood. We find that, in 15- to 40-somite-stage avian embryos, BMP4 mRNA is homogeneously distributed along the longitudinal extent of the dorsal neural tube, whereas its specific inhibitor noggin exists in a gradient of expression that decreases caudorostrally. This rostralward reduction in signal intensity coincides with the onset of emigration of neural crest cells. Hence, we hypothesized that an interplay between Noggin and BMP4 in the dorsal tube generates graded concentrations of the latter that in turn triggers the delamination of neural crest progenitors. Consistent with this suggestion, disruption of the gradient by grafting Noggin-producing cells dorsal to the neural tube at levels opposite the segmental plate or newly formed somites, inhibited emigration of HNK-1-positive crest cells, which instead accumulated within the dorsal tube. Similar results were obtained with explanted neural tubes from the same somitic levels exposed to Noggin. Exposure to Follistatin, however, had no effect. The Noggin-dependent inhibition was overcome by concomitant treatment with BMP4, which when added alone, also accelerated cell emigration compared to untreated controls. Furthermore, the observed inhibition of neural crest emigration in vivo was preceded by a partial or total reduction in the expression of cadherin-6B and rhoB but not in the expression of slug mRNA or protein. Altogether, these results suggest that a coordinated activity of Noggin and BMP4 in the dorsal neural tube triggers delamination of specified, slug-expressing neural crest cells. Thus, BMPs play multiple and discernible roles at sequential stages of neural crest ontogeny, from specification through delamination and later differentiation of specific neural crest derivatives.

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MAPRE2 mutations result in altered human cranial neural crest migration, underlying craniofacial malformations in CSC-KT syndrome

Scientific Reports ◽

10.1038/s41598-021-83771-3 ◽

2021 ◽

Vol 11 (1) ◽

Author(s):

Cedric Thues ◽

Jorge S. Valadas ◽

Liesbeth Deaulmerie ◽

Ann Geens ◽

Amit K. Chouhan ◽

...

Keyword(s):

Neural Crest ◽

Induced Pluripotent Stem Cell ◽

Neural Crest Cells ◽

Branchial Arch ◽

Cellular Migration ◽

Cranial Neural Crest ◽

Craniofacial Malformations ◽

Neural Crest Migration

AbstractCircumferential skin creases (CSC-KT) is a rare polymalformative syndrome characterised by intellectual disability associated with skin creases on the limbs, and very characteristic craniofacial malformations. Previously, heterozygous and homozygous mutations in MAPRE2 were found to be causal for this disease. MAPRE2 encodes for a member of evolutionary conserved microtubule plus end tracking proteins, the end binding (EB) family. Unlike MAPRE1 and MAPRE3, MAPRE2 is not required for the persistent growth and stabilization of microtubules, but plays a role in other cellular processes such as mitotic progression and regulation of cell adhesion. The mutations identified in MAPRE2 all reside within the calponin homology domain, responsible to track and interact with the plus-end tip of growing microtubules, and previous data showed that altered dosage of MAPRE2 resulted in abnormal branchial arch patterning in zebrafish. In this study, we developed patient derived induced pluripotent stem cell lines for MAPRE2, together with isogenic controls, using CRISPR/Cas9 technology, and differentiated them towards neural crest cells with cranial identity. We show that changes in MAPRE2 lead to alterations in neural crest migration in vitro but also in vivo, following xenotransplantation of neural crest progenitors into developing chicken embryos. In addition, we provide evidence that changes in focal adhesion might underlie the altered cell motility of the MAPRE2 mutant cranial neural crest cells. Our data provide evidence that MAPRE2 is involved in cellular migration of cranial neural crest and offers critical insights into the mechanism underlying the craniofacial dysmorphisms and cleft palate present in CSC-KT patients. This adds the CSC-KT disorder to the growing list of neurocristopathies.

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How inhibitory cues can both constrain and promote cell migration

The Journal of Cell Biology ◽

10.1083/jcb.201605074 ◽

2016 ◽

Vol 213 (5) ◽

pp. 505-507 ◽

Cited By ~ 1

Author(s):

Marianne E. Bronner

Keyword(s):

Mathematical Modeling ◽

Cell Migration ◽

Neural Crest ◽

Neural Crest Cells ◽

Collective Cell Migration ◽

Promote Cell Migration ◽

Neural Crest Migration ◽

Physical Boundary

Collective cell migration is a common feature in both embryogenesis and metastasis. By coupling studies of neural crest migration in vivo and in vitro with mathematical modeling, Szabó et al. (2016, J. Cell Biol., http://dx.doi.org/10.1083/jcb.201602083) demonstrate that the proteoglycan versican forms a physical boundary that constrains neural crest cells to discrete streams, in turn facilitating their migration.

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Differentiation in vitro of sympathetic cells from chick embryo sensory ganglia

Development ◽

10.1242/dev.33.1.43 ◽

1975 ◽

Vol 33 (1) ◽

pp. 43-56

Author(s):

D. F. Newgreen ◽

R. O. Jones

Keyword(s):

Chick Embryo ◽

Neural Crest ◽

Neural Tube ◽

Neural Crest Cells ◽

Sensory Ganglia ◽

Sensory Ganglion ◽

Neural Crest Origin ◽

Fluorescent Cells

This study was carried out in order to determine what factors control the differentiation of certain neural crest cells in the chick embryo. Emphasis was placed on the morphologically and biochemically divergent sensory and sympathetic pathways of differentiation. Embryos were precisely staged according to Hamburger & Hamilton (1951) and it was observed that sensory ganglia with somites, explanted at stages 21–24, gave rise to cells showing formaldehyde-induced fluorescence in more than 25% of explants. These cells were identical in properties to the fluorescent cells of the sympathetic system of embryos of similar age, and appeared by 12 days in vitro. These fluorescent cells did not appear when somites and sensory ganglia explants were maintained separately. The incidence of fluorescent cells in combined explants was considerably reduced or absent when cultures were maintained for 7 days or less, or when the explants were obtainedfrom stage 25–26 embryos. Furthermore, when neural tube was also included in the cultures, the appearance of fluorescent cells was markedly inhibited. The requirement for somitic tissue to induce fluorescent cells in combined explants can be replaced by forelimb-bud tissue. The origin of these cells and the factors that control their differentiation in vitro are discussed with reference to the neural crest origin of the sensory ganglion, and the possible conditions pertaining in vivo in this region.

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Induction of melanocyte precursors from neural crest cells surrounding the neural tube-like structures developed in vitro using mouse ES cell culture

Inflammation and Regeneration ◽

10.2492/inflammregen.27.45 ◽

2007 ◽

Vol 27 (1) ◽

pp. 45-52

Author(s):

Koh-ichi Atoh ◽

Manae S. Kurokawa ◽

Hideshi Yoshikawa ◽

Chieko Masuda ◽

Erika Takada ◽

...

Keyword(s):

Cell Culture ◽

Neural Crest ◽

Neural Tube ◽

Neural Crest Cells ◽

Es Cell ◽

Mouse Es Cell

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An experimental study on neural crest migration in Barbus conchonius (Cyprinidae, Teleostei), with special reference to the origin of the enteroendocrine cells

Development ◽

10.1242/dev.62.1.309 ◽

1981 ◽

Vol 62 (1) ◽

pp. 309-323

Author(s):

C. H. J. Lamers ◽

J. W. H. M. Rombout ◽

L. P. M. Timmermans

Keyword(s):

Neural Crest ◽

Neural Tube ◽

Ganglion Cells ◽

Neural Crest Cells ◽

Enteroendocrine Cells ◽

Pigment Cells ◽

Transplantation Technique ◽

Spinal Ganglion Cells ◽

Neural Crest Origin ◽

Neural Crest Migration

A neural crest transplantation technique is described for fish. As in other classes ofvertebrates, two pathways of neural crest migration can be distinguished: a lateroventral pathway between somites and ectoderm, and a medioventral pathway between somites and neural tube/notochord. In this paper evidence is presented for a neural crest origin of spinal ganglion cells and pigment cells, and indication for such an origin is obtained for sympathetic and enteric ganglion cells and for cells that are probably homologues to adrenomedullary and paraganglion cells in the future kidney area. The destiny of neural crest cells near the developing lateral-line sense organs is discussed. When grafted into the yolk, neural crest cells or neural tube cells appear to differentiate into ‘periblast cells’; this suggests a highly activating influence of the yolk. Many neural crest cells are found around the urinary ducts and, when grafted below the notochord, even within the urinary duct epithelium. These neural crest cells do not invade the gut epithelium, even when grafted adjacent to the developing gut. Consequently enteroendocrine cells in fish are not likely to have a trunkor rhombencephalic neural crest origin. Another possible origin of these cells will be proposed.

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Lineage-specific requirements of β-catenin in neural crest development

The Journal of Cell Biology ◽

10.1083/jcb.200209039 ◽

2002 ◽

Vol 159 (5) ◽

pp. 867-880 ◽

Cited By ~ 207

Author(s):

Lisette Hari ◽

Véronique Brault ◽

Maurice Kléber ◽

Hye-Youn Lee ◽

Fabian Ille ◽

...

Keyword(s):

Transcription Factor ◽

Neural Crest ◽

Neural Crest Cells ◽

Neural Crest Stem Cells ◽

Downstream Signaling ◽

Neural Crest Development ◽

Sensory Neurogenesis

β-Catenin plays a pivotal role in cadherin-mediated cell adhesion. Moreover, it is a downstream signaling component of Wnt that controls multiple developmental processes such as cell proliferation, apoptosis, and fate decisions. To study the role of β-catenin in neural crest development, we used the Cre/loxP system to ablate β-catenin specifically in neural crest stem cells. Although several neural crest–derived structures develop normally, mutant animals lack melanocytes and dorsal root ganglia (DRG). In vivo and in vitro analyses revealed that mutant neural crest cells emigrate but fail to generate an early wave of sensory neurogenesis that is normally marked by the transcription factor neurogenin (ngn) 2. This indicates a role of β-catenin in premigratory or early migratory neural crest and points to heterogeneity of neural crest cells at the earliest stages of crest development. In addition, migratory neural crest cells lateral to the neural tube do not aggregate to form DRG and are unable to produce a later wave of sensory neurogenesis usually marked by the transcription factor ngn1. We propose that the requirement of β-catenin for the specification of melanocytes and sensory neuronal lineages reflects roles of β-catenin both in Wnt signaling and in mediating cell–cell interactions.

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Evidence for collapsin-1 functioning in the control of neural crest migration in both trunk and hindbrain regions

Development ◽

10.1242/dev.126.10.2181 ◽

1999 ◽

Vol 126 (10) ◽

pp. 2181-2189 ◽

Cited By ~ 7

Author(s):

B.J. Eickholt ◽

S.L. Mackenzie ◽

A. Graham ◽

F.S. Walsh ◽

P. Doherty

Keyword(s):

Cell Migration ◽

Neural Crest ◽

Neural Crest Cell ◽

Axon Growth ◽

Neural Crest Cells ◽

Neural Crest Cell Migration ◽

Neural Crest Migration ◽

Migration Pathways ◽

Crest Cell

Collapsin-1 belongs to the Semaphorin family of molecules, several members of which have been implicated in the co-ordination of axon growth and guidance. Collapsin-1 can function as a selective chemorepellent for sensory neurons, however, its early expression within the somites and the cranial neural tube (Shepherd, I., Luo, Y., Raper, J. A. and Chang, S. (1996) Dev. Biol. 173, 185–199) suggest that it might contribute to the control of additional developmental processes in the chick. We now report a detailed study on the expression of collapsin-1 as well as on the distribution of collapsin-1-binding sites in regions where neural crest cell migration occurs. collapsin-1 expression is detected in regions bordering neural crest migration pathways in both the trunk and hindbrain regions and a receptor for collapsin-1, neuropilin-1, is expressed by migrating crest cells derived from both regions. When added to crest cells in vitro, a collapsin-1-Fc chimeric protein induces morphological changes similar to those seen in neuronal growth cones. In order to test the function of collapsin-1 on the migration of neural crest cells, an in vitro assay was used in which collapsin-1-Fc was immobilised in alternating stripes consisting of collapsin-Fc/fibronectin versus fibronectin alone. Explanted neural crest cells derived from both trunk and hindbrain regions avoided the collapsin-Fc-containing substratum. These results suggest that collapsin-1 signalling can contribute to the patterning of neural crest cell migration in the developing chick.

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Pax3 is required for cardiac neural crest migration in the mouse: evidence from the splotch (Sp2H) mutant

Development ◽

10.1242/dev.124.2.505 ◽

1997 ◽

Vol 124 (2) ◽

pp. 505-514 ◽

Cited By ~ 14

Author(s):

S.J. Conway ◽

D.J. Henderson ◽

A.J. Copp

Keyword(s):

Neural Crest ◽

Neural Tube ◽

Neural Crest Cells ◽

Outflow Tract ◽

Avian Embryo ◽

Cardiac Neural Crest ◽

Branchial Arches ◽

Aortic Arches ◽

Cardiac Outflow

Neural crest cells originating in the occipital region of the avian embryo are known to play a vital role in formation of the septum of the cardiac outflow tract and to contribute cells to the aortic arches, thymus, thyroid and parathyroids. This ‘cardiac’ neural crest sub-population is assumed to exist in mammals, but without direct evidence. In this paper we demonstrate, using RT-PCR and in situ hybridisation, that Pax3 expression can serve as a marker of cardiac neural crest cells in the mouse embryo. Cells of this lineage were traced from the occipital neural tube, via branchial arches 3, 4 and 6, into the aortic sac and aorto-pulmonary outflow tract. Confirmation that these Pax3-positive cells are indeed cardiac neural crest is provided by experiments in which hearts were deprived of a source of colonising neural crest, by organ culture in vitro, with consequent lack of up-regulation of Pax3. Occipital neural crest cell outgrowths in vitro were also shown to express Pax3. Mutation of Pax3, as occurs in the splotch (Sp2H) mouse, results in development of conotruncal heart defects including persistent truncus arteriosus. Homozygotes also exhibit defects of the aortic arches, thymus, thyroid and parathyroids. Pax3-positive neural crest cells were found to emigrate from the occipital neural tube of Sp2H/Sp2H embryos in a relatively normal fashion, but there was a marked deficiency or absence of neural crest cells traversing branchial arches 3, 4 and 6, and entering the cardiac outflow tract. This decreased expression of Pax3 in Sp2H/Sp2H embryos was not due to down-regulation of Pax3 in neural crest cells, as use of independent neural crest markers, Hoxa-3, CrabpI, Prx1, Prx2 and c-met also revealed a deficiency of migrating cardiac neural crest cells in homozygous embryos. This work demonstrates the essential role of the cardiac neural crest in formation of the heart and great vessels in the mouse and, furthermore, shows that Pax3 function is required for the cardiac neural crest to complete its migration to the developing heart.

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