Spatially distinct domains of cell behavior in the zebrafish organizer region

1997 ◽  
Vol 75 (5) ◽  
pp. 563-577 ◽  
Author(s):  
Leonard A D'Amico ◽  
Mark S Cooper
Keyword(s):  
Marginal Zone ◽  
Organizer Region ◽  
Time Lapse ◽  
Cell Cluster ◽  
Specific Cell ◽  
Zebrafish Embryos ◽  
Dorsal Margin ◽  
Blastula Stage ◽  
Embryonic Shield ◽  
Longitudinal Position

To determine the sequence of cell behaviors that is involved in the morphogenesis of the zebrafish organizer region, we have examined the dorsal marginal zone of vitally stained zebrafish embryos using time-lapse confocal microscopy. During the late-blastula stage, the zebrafish dorsal marginal zone segregates into several cellular domains, including a group of noninvoluting, highly endocytic marginal (NEM) cells. The NEM cell cluster, which lies in a superficial location of the dorsal marginal zone, is composed of both enveloping layer cells and one or two layers of underlying deep cells. The longitudinal position of this cellular domain accurately predicts the site of embryonic shield formation and occupies a homologous location to the organizer epithelium in Xenopus laevis. At the onset of gastrulation, deep cells underneath the superficial NEM cell domain undergo involution to form the nascent hypoblast of the embryonic shield. Deep cells within the NEM cell cluster, however, do not involute during early shield formation, but instead move in front of the blastoderm margin to form a loose mass of cells called forerunner cells. Forerunner cells coalesce into a wedge-shaped mass during late gastrulation and eventually become overlapped by the converging lateral lips of the germ ring. During early zebrafish tail elongation, most forerunner cells are incorporated into the epithelial lining of Kupffer's vesicle, a transient teleostean organ rudiment long thought to be an evolutionary vestige of the neurenteric canal. Owing to the location of NEM cells at the dorsal margin of blastula-stage embryos, as well as their early segregation from other deep cells, we hypothesized that NEM cells are specified by an early-acting dorsalizing signal. To test this possibility, we briefly treated early-blastula stage embryos with LiCl, an agent known to produce hyperdorsalized zebrafish embryos with varying degrees of expanded organizer tissue. In Li + -treated embryos, NEM cells appear either within expanded spatial domains or in ectopic locations, primarily within the marginal zone of the blastoderm. These results suggest that NEM cells represent a specific cell type that is specified by an early dorsal patterning pathway.

The anterior extent of dorsal development of the Xenopus embryonic axis depends on the quantity of organizer in the late blastula

Development ◽  
1990 ◽  
Vol 109 (2) ◽  
pp. 363-372 ◽  
Author(s):  
R.M. Stewart ◽  
J.C. Gerhart
Keyword(s):  
Xenopus Laevis ◽  
Cell Population ◽  
Marginal Zone ◽  
Organizer Region ◽  
Blastula Stage ◽  
Dorsal Midline ◽  
Anterior Dorsal ◽  
Lateral Width ◽  
Anterior Extent ◽  
Anterior Posterior

In amphibian gastrulae, the cell population of the organizer region of the marginal zone (MZ) establishes morphogenesis and patterning within itself and within surrounding regions of the MZ, presumptive neurectoderm, and archenteron roof. We have tested the effects on pattern of reducing the amount of organizer region by recombining halves of Xenopus laevis late blastulae cut at different angles from the bilateral plane. When regions within 30 degrees of the dorsal midline are excluded from recombinants, ventralized embryos develop lacking the entire anterior-posterior sequence of dorsal structures, suggesting that the organizer is only 60 degrees wide (centered on the dorsal midline) at the late blastula stage. As more and more dorsal MZ (organizer) is included in the recombinant, progressively more anterior dorsal structures are formed. In all cases, when any dorsal structures are missing they are deleted serially from the anterior end. Thus, we suggest that the amount (lateral width) of the organizer in the MZ determines the anterior extent of dorsal development.

scholarly journals The ciliary marginal zone of the zebrafish retina: clonal and time-lapse analysis of a continuously growing tissue

Development ◽  
2016 ◽  
Vol 143 (7) ◽  
pp. 1099-1107 ◽  
Author(s):  
Yinan Wan ◽  
Alexandra D. Almeida ◽  
Steffen Rulands ◽  
Naima Chalour ◽  
Leila Muresan ◽  
...  
Keyword(s):  
Marginal Zone ◽  
Time Lapse ◽  
Ciliary Marginal Zone

Axis-inducing activities and cell fates of the zebrafish organizer

Development ◽  
2000 ◽  
Vol 127 (16) ◽  
pp. 3407-3417 ◽  
Author(s):  
L. Saude ◽  
K. Woolley ◽  
P. Martin ◽  
W. Driever ◽  
D.L. Stemple
Keyword(s):  
Organizer Region ◽  
Complete Removal ◽  
Floor Plate ◽  
Significant Loss ◽  
Cell Fates ◽  
Deep Tissue ◽  
Head Formation ◽  
Prechordal Plate ◽  
Embryonic Shield ◽  
Organizer Activity

We have investigated axis-inducing activities and cellular fates of the zebrafish organizer using a new method of transplantation that allows the transfer of both deep and superficial organizer tissues. Previous studies have demonstrated that the zebrafish embryonic shield possesses classically defined dorsal organizer activity. When we remove the morphologically defined embryonic shield, embryos recover and are completely normal by 24 hours post-fertilization. We find that removal of the morphological shield does not remove all goosecoid- and floating head-expressing cells, suggesting that the morphological shield does not comprise the entire organizer region. Complete removal of the embryonic shield and adjacent marginal tissue, however, leads to a loss of both prechordal plate and notochord. In addition, these embryos are cyclopean, show a significant loss of floor plate and primary motorneurons and display disrupted somite patterning. Motivated by apparent discrepancies in the literature we sought to test the axis-inducing activity of the embryonic shield. A previous study suggested that the shield is capable of only partial axis induction, specifically being unable to induce the most anterior neural tissues. Contrary to this study, we find shields can induce complete secondary axes when transplanted into host ventral germ-ring. In induced secondary axes donor tissue contributes to notochord, prechordal plate and floor plate. When explanted shields are divided into deep and superficial fragments and separately transplanted we find that deep tissue is able to induce the formation of ectopic axes with heads but lacking posterior tissues. We conclude that the deep tissue included in our transplants is important for proper head formation.

Conditioning of a culture substratum by the ectodermal layer promotes attachment and oriented locomotion by amphibian gastrula mesodermal cells

1983 ◽  
Vol 59 (1) ◽  
pp. 43-60 ◽  
Author(s):  
N. Nakatsuji ◽  
K.E. Johnson
Keyword(s):  
Cell Migration ◽  
Time Lapse ◽  
Ambystoma Maculatum ◽  
Specific Cell ◽  
Animal Pole ◽  
Micron Diameter ◽  
The Relationship ◽  
Extracellular Fibrils ◽  
Scanning Electron

We have found that ectodermal fragments of Ambystoma maculatum gastrulae deposit immense numbers of 0.1 micron diameter extracellular fibrils on plastic coverslips. When migrating mesodermal cells from A. maculatum gastrulae are seeded on such conditioned plastic substrata, they attach and begin migrating after 15–30 min in vitro. We did a detailed analysis of the relationship between fibril orientation and cell migration using time-lapse cinemicrography, scanning electron microscopy, and a microcomputer with a graphics tablet and morphometric program. We found that cells move in directions closely related to the orientation of fibrils. Usually fibrils are oriented in dense arrays with a predominance of fibrils running parallel to the blastopore-animal pole axis of the explant, and cells move preferentially along lines parallel to the blastopore-animal pole axis. When fibrils are unaligned, cells move at random. We have also shown that cells move with a slightly stronger tendency towards the animal pole direction. These results are discussed concerning the mechanism of specific cell migration during amphibian gastrulation.

The marginal zone and its contribution to the hypoblast and primitive streak of the chick embryo

Development ◽  
1990 ◽  
Vol 109 (3) ◽  
pp. 667-682 ◽  
Author(s):  
C.D. Stern
Keyword(s):  
Chick Embryo ◽  
Marginal Zone ◽  
Primitive Streak ◽  
Time Lapse ◽  
Study Time ◽  
Fate Mapping ◽  
Deep Part ◽  
Germ Layers ◽  
Gut Endoderm ◽  
Transplantation Experiments

The marginal zone of the chick embryo has been shown to play an important role in the formation of the hypoblast and of the primitive streak. In this study, time-lapse filming, fate mapping, ablation and transplantation experiments were combined to study its contribution to these structures. It was found that the deep (endodermal) portion of the posterior marginal zone contributes to the hypoblast and to the junctional endoblast, while the epiblast portion of the same region contributes to the epiblast of the primitive streak and to the definitive (gut) endoderm derived from it. Within the deep part of the posterior marginal zone, a subpopulation of HNK-1-positive cells contributes to the hypoblast. Removal of the deep part of the marginal zone prevents regeneration of the hypoblast but not the formation of a primitive streak. Removal of both layers of the marginal zone leads to a primitive streak of abnormal morphology but mesendodermal cells nevertheless differentiate. These results show that the two main properties of the posterior marginal zone (contributing to the hypoblast and controlling the site of primitive streak formation) are separable, and reside in different germ layers. This conclusion does not support the idea that the influence of the posterior marginal zone on the development of axial structures is due to it being the source of secondary hypoblast cells.

Properties of the primary organization field in the embryo of Xenopus laevis

Development ◽  
1972 ◽  
Vol 28 (1) ◽  
pp. 13-26
Author(s):  
J. Cooke
Keyword(s):  
Marginal Zone ◽  
Organizer Region ◽  
Angular Distance ◽  
Cell Polarization ◽  
Subsequent Paper ◽  
Basic Operation ◽  
Primary Organization ◽  
Organizer Activity ◽  
Set Up ◽  
Cell Immigration

The work presented, in this and the subsequent papers of a series, was begun in order to re-examine the properties of the amphibian primary embryonic field, in the light of current theories concerning the nature of individuation fields in developing animal systems. A detailed description is given of the basic operation whose results are described in this and the subsequent paper. This involves the transplantation, into a late blastula or stage-10 gastrula host, of a supernumerary stage-10 organizer region. The consequences of such operations during the following 4–6 h, up to the late gastrula stage, are also described. Evidence is presented that, from a time some 2·5 h before the organizer site first becomes externally visible, its presumptive region is immune from interference by the proximity of another, implanted organizer, even one which is itself 2·5 h older. That is to say, the final site of development of host organizer activity is not altered by the presence of such an implant. Pairs of early organizers at comparable stages of activity appear to set up competing fields of cellular orientation and immigration, which show a fairly sharp boundary at their interface. This is most obvious for pairs of organizers fairly close together, since the cell polarization and stretching is most pronounced in the region near to the apex of the field, i.e. the initial site of cell immigration. Independent initial fields of immigration due to two organizers can reliably be distinguished in cases where they are as little as 30° of angular distance apart in the marginal zone of the host. These results are to be considered in relation to those of Paper II, for the same series of operations, where the final patterns of cell differentiation are studied, and to those of Paper III, where evidence is given for the development of autonomous polarity in the region of the organizer.

Three-Dimensional Time-Lapse Digital Movie Analysis of the Developing Fruit Fly Eye in Organ Culture

1997 ◽  
Vol 3 (S2) ◽  
pp. 1129-1130
Author(s):  
John Archie Pollock ◽  
Bejon T. Maneckshana ◽  
Teresa E. Leonardo
Keyword(s):  
Organ Culture ◽  
Compound Eye ◽  
Eye Development ◽  
Larval Instar ◽  
Three Dimensional ◽  
Fruit Fly ◽  
Time Lapse ◽  
Cell Types ◽  
Specific Cell ◽  
The Brain

The compound eye of the fruit fly, Drosophila melanogaster, is composed of a highly ordered array of facets (FIG. 1), each containing a precise set of neurons and supporting cells. The eye arises during the third larval instar from an undifferentiated epithelium, the eye imaginai disc, which is connected to the brain via the optic stalk (FIG. 2). During eye development, movement of the morphogenetic furrow, progressive recruitment of specific cell types and the growth of photoreceptor axons into the brain are each dynamic processes that are routinely studied indirectly in fixed tissues. While stereotyped development and the ‘crystalline’ like structure of the eye facilitates this analysis, certain experiments are hindered by the inability to observe developmental processes as they occur. To overcome this limitation, we have combined organ culture with advanced microscopy tools to enable the observation of eye development in living tissue.

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