Centre for Genome Research, Kings Buildings, West Mains Road, Edinburgh EH9 3JQ, UK
*Author for correspondence (e-mail: v.wilson{at}ed.ac.uk)
Accepted 11 July 2002
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SUMMARY |
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Key words: Mouse, Anteroposterior axis, Tail bud, Stem cell, Chordoneural hinge
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INTRODUCTION |
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In support of this, groups of 10-20 cells from the primitive streak and tail bud of 9.5 d.p.c.-13.5 d.p.c. embryos are able to incorporate in the streak of 8.5 d.p.c. embryos (Tam and Tan, 1992). However, there is evidence from the above study to suggest that cells in the primitive streak and tail bud are not completely interchangeable, as grafted cells from older tail buds contribute to more posterior somites than cells from the streak. In the past, it has been suggested that cells in the tail bud not only have different potency, but also proliferate according to different rules from those that pertain to the streak. Holmdahl (Holmdahl, 1925
), from studies in chick, suggested that the vertebrate tail bud constitutes a blastema of undifferentiated cells with little or no regional specification of the progenitors. However, later fate mapping analysis in Xenopus showed regionalisation of distinct progenitors of neural tube, notochord and somites within a small area of the blastopore (the Xenopus equivalent of the late primitive streak) and tail bud (Gont et al., 1993
). In the tail bud, this region was termed the chordoneural hinge (CNH), and it is able to produce ectopic tails when grafted to host embryos. Gene expression within the tail bud is also strongly localised amongst the regionalised progenitors (Beck and Slack, 1998
; Gawantka et al., 1998
).
Intriguingly, however, it appears that there may be some cells in the tail bud whose fate is not specified, as marking very small groups of cells in the tail bud can result in descendants in more than one tissue type (Davis and Kirschner, 2000). Thus, while much of the tail bud in Xenopus is composed of regionalised progenitors, it is unclear whether these constitute all the axial progenitors. Alternatively, a second population of multi-fated progenitors may exist, which raises the possibility that these give rise to regionally specified progenitors.
In mouse, the descendants of single cells in the epiblast destined for the streak at early streak stage are not confined to any single tissue type (Lawson et al., 1991). Even later, mesoderm progenitors in the epiblast, although regionalised in fate, are not highly restricted in potency (Beddington, 1981
). Whether the same multipotency is conserved in the later streak and tail bud in the mouse is unknown. The ontogeny of two of the axial tissues, the myotome, a paraxial mesoderm derivative, and spinal cord, derived from neural plate, has been studied using a retrospective single cell marking technique (Nicolas et al., 1996
; Mathis and Nicolas, 2000
). In these studies, descendants of single cells that have undergone a rare somatic recombination event and are located in either myotome or spinal cord are marked. In the myotome, those descendants of single cells that populate large anteroposterior axial distances are located bilaterally, showing that their progenitors originate in the primitive streak and tail bud (Nicolas et al., 1996
). These studies indicate the existence of stem cell progenitors of both myotome and spinal cord. However, they do not give detailed information on their position and identity.
In lineage tracing experiments in cultured mouse embryos, most cells in the streak are destined for exit to differentiating axis tissues (Lawson et al., 1991; Tam and Beddington, 1987
). However, a small proportion remain in the tail bud at the end of the culture period, in some cases after the formation of some 32 somites (Wilson and Beddington, 1996
). Because we know that axial progenitors reside there, some or all of these may represent stem cells. Because stem cells are characterised by the ability to self-renew, they should be distinguishable from other cells in the axis by their capacity to contribute to both anterior and posterior differentiated tissues, and the ability to be serially passaged.
We have refined previous fate maps to show that the tail bud contains regionally separated descendants of cells in the streak using topically applied lipophilic dyes. We have exploited transgenic strains of mice that express green fluorescent protein (GFP) (Okabe et al., 1997) or lacZ (Munsie et al., 1998
) ubiquitously to explore the potency of these cells. We show that cells in the vicinity of the node and their descendants are found in an equivalent structure to the Xenopus CNH. These cells fulfil the above criteria expected of stem cells. By contrast, cells in the more ventrally located tail bud mesoderm, which were found to be descended from the CNH, are more limited in their potency.
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MATERIALS AND METHODS |
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Dissection of tissues for grafting
GFP transgenicxMF1 litters were dissected in M2 medium and those containing the transgene selected in a Nikon SMZ-U dissecting microscope with fluorescence attachment. The posterior half of the embryo containing the primitive streak was dissected using fine forceps. The primitive streak was dissected using an eyelash tool by making two longitudinal lateral cuts, isolating a thin strip of tissue containing the entire primitive streak and node and retaining both ectodermal and endodermal layers. Node and primitive streak fragments were further dissected by making transverse cuts with the eyelash tool. A schematic diagram of the sites dissected is shown in Fig. 1A.
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DiI labelling
Embryos were labelled with CellTracker CM-DiI and CMFDA (Molecular Probes) as described previously (Wilson and Beddington, 1996). Dissected CNH and TBM were labelled by expelling DiI from a pipette held directly above the tissue to be labelled for a few seconds. The graft was then washed in fresh M2. Dissected 10.5 d.p.c. tail pieces were labelled in the neural tube by inserting a fine pipette into the lumen and expelling a small amount of dye, which covered most or all of the luminal surface. Labelling of the most posterior end was checked either by observing a faint pink colour under brightfield illumination, or by viewing in a dissecting microscope with fluorescence attachment. Label sites are shown in Fig. 1A.
Grafting labelled tissue
Grafts were performed using a hand-drawn micropipette. The embryo was held loosely in place with forceps while suction was gently applied with the micropipette to the anterior primitive streak immediately abutting the node to create an opening for the graft. The tissue to be grafted was then drawn into the pipette, and the pipette inserted in the opening. The graft was gently expelled as the pipette was drawn out of the embryo, leaving the tissue lodged in the opening (Fig. 1C). The embryos were then placed in a universal container in 50% rat serum, 50% GMEM or DMEM in an incubator gassed at 5% CO2 in air for 30 minutes to allow the grafts to heal before sealing the Universals and placing them in a roller culture apparatus at 37°C overnight. Embryos which had developed normally were cultured for a further 24 hours in 75% rat serum in 40% oxygen, 5% CO2, 55% nitrogen. At the end of the culture period fluorescence was assessed either in a Nikon SMZ-U dissecting microscope or, for more detailed analysis, in a Zeiss Axiovert inverted microscope. Images were captured using Improvision Openlab software and processed using Adobe Photoshop.
X-gal staining with in situ hybridisation
Embryos carrying the ubiquitously expressed Zin40 gene trap integration were used as donors for experiments testing the gene expression of grafted cells. Grafted embryos were first stained with X-gal and then subjected to in situ hybridisation (Tajbakhsh and Houzelstein, 1995) with probes specific for T (Wilkinson et al., 1990
), sonic hedgehog (Echelard et al., 1993
), Delta like 1 (Dll1) (Dunwoodie et al., 1997
) and Pax3 (Goulding et al., 1991
). Embryos were then dehydrated via a methanol series and processed for paraffin wax histology.
Histology
DiI-labelled embryos and embryos that received grafts of GFP transgenic cells were sectioned transversely in a Series 1000 Vibratome at 50 µm as and images obtained as described above. Embryos subjected to X-gal staining with in situ hybridisation were sectioned transversely at 7 µm and photographed in an Olympus Vanox compound microscope.
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RESULTS |
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Regionalisation of primitive streak descendants in the tail bud
Previous studies have shown that some descendants of cells in the node and primitive streak at 8.5 d.p.c. are present in the tail bud at 10.5 d.p.c. (Wilson and Beddington, 1996). To determine whether there is any relationship between origin of the cells in the streak and their subsequent location in the tail bud, two distinct sites were labelled: the ventral layer of the node and anterior primitive streak. In accordance with previous fate-mapping studies, the descendants of cells in the node were located in the notochord (Fig. 2A,E), whereas those of the anterior streak were predominantly somitic (Fig. 2B,G). Descendants of anterior streak were also located in the ventral neurectoderm, but not notochord (Fig. 2F). The anterior limit of labelling was around somite 12. In the tail bud after node labelling, the labelled notochord widened and ended abruptly beneath the neural tube, anterior to the end of the tail such that the mesoderm in the tail bud (Fig. 2A,K) was unlabelled. Descendants of the anterior streak were located in the tail bud in two domains: the posterior ectoderm continuous with the ventral posterior neural tube (termed posterior neural plate) and the TBM. (Fig. 2B,M).
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Before posterior neuropore closure, the posterior neural plate is a source of mesoderm for somites (Wilson and Beddington, 1996). As labelled anterior streak contributed descendants to both posterior neurectoderm and mesoderm, it was of interest to determine whether the posterior neural plate continues to produce mesoderm after posterior neuropore closure. To test this, the entire neurectoderm of dissected 10.5 d.p.c. tail pieces that had undergone posterior neuropore closure was labelled using DiI. After 48 hours, labelled mesoderm was detected in the posterior region of six out of six cultured tail pieces (Fig. 3). Here, too, there is some evidence that the most posterior notochord is populated by ectoderm descendants (compare notochord in Fig. 3B with that in 3C) Therefore, a region continuous with the neurectoderm most probably the posterior ventral neurectoderm, which is descended from the streak (Fig. 2M) contributes to the mesoderm of the tail. The region composed of the posterior neural plate and the posterior end of the notochord is thus topologically equivalent to the CNH defined in Xenopus.
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Potency depends on location in the tail bud
We compared the capacity of dissected 10.5-12.5 d.p.c. CNH or TBM to differentiate relative to control isochronic grafts, when grafted to the 8.5 d.p.c. primitive streak/node border (Table 1). The donor tissues were derived either from GFP transgenic embryos, Zin40 embryos or wild-type tissue labelled with DiI. Although a high proportion of control isochronic grafts had incorporated well in the axis (Table 1), we observed a reduction in the proportion of grafts from the TBM that incorporated correctly, with cells remaining predominantly as morphologically undifferentiated clumps (Fig. 4A,B). Differentiation of only one out of 11 heterochronic grafts of TBM, derived from a 10.5 d.p.c. embryo, was observed. In this embryo, labelled cells were restricted to a short unilateral stretch of somitic mesoderm and did not populate the tail bud (data not shown).
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To verify that these apparently well-integrated donor tissues indeed differentiated appropriately, a subset of the embryos were grafted with cells expressing the transgenic marker Zin40, a developmentally neutral gene trap integration containing a ubiquitously expressed lacZ gene (Munsie et al., 1998). This histologically stable marker allowed processing of grafted embryos for in situ hybridisation to markers of differentiation in axial tissues (Tajbakhsh and Houzelstein, 1995
). Co-expression of lacZ and the differentiation marker was scored in serial transverse sections.
Within the axis, brachyury (T) and sonic hedgehog (Shh) are expressed in the notochord, and Shh is additionally expressed in the floorplate (Echelard et al., 1993; Wilkinson et al., 1990
). In embryos that received an 8.5 d.p.c. node graft, both T and Shh were expressed appropriately in donor cells in the notochord, and graft-derived cells in the floorplate expressed Shh but not T (Fig. 5A-D; Table 2). Cells immediately dorsal to the floorplate express the neural marker Pax6, and graft-derived cells populating this region also appropriately expressed Pax6 (Table 2). Medially located donor cells in the paraxial mesoderm showed no ectopic T expression (data not shown). The tail buds of the embryos shown in Fig. 5A-D had been removed prior to processing and were not assayed for marker gene expression. This apparently normal differentiation therefore correlates well with the morphological assessment of incorporation in tissue derived from isochronic grafts. To determine whether this was true of grafted 10.5 d.p.c. tissue, the expression of T, Shh and two additional markers of paraxial mesoderm differentiation, Dll1 (Dunwoodie et al., 1997
) and Pax3 were assayed. Within the axis, where donor cells appeared morphologically incorporated in a tissue, they correctly co-expressed all differentiation markers assayed (Fig. 5E-H; Table 2). Furthermore, the incorporated cells did not ectopically express differentiation markers (Fig. 5H, arrow). In the tail bud mesoderm and CNH, many donor cells also expressed T, showing that these cells also express markers appropriate for tail bud (data not shown).
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The CNH, but not TBM, is serially transplantable
The population of host CNH by grafted CNH cells separated by up to 4 days in developmental stage from the host (Table 1; Fig. 4), together with their ability to participate in differentiated axial tissue formation, suggested that axial stem cells reside there, and not in the TBM. Such stem cells should also contribute cells to the axis and repopulate CNH on multiple passages through host embryos. We therefore tested this by regrafting GFP-labelled CNH and TBM to 8.5 d.p.c. embryos.
In second generation grafts, groups of cells containing labelled TBM derived from initial anterior streak grafts were also disadvantaged relative to CNH from incorporating in the axis (Table 3). Similar to the results above, when they did incorporate in the axis, they did so only over short axial distances (Fig. 6), and only one embryo showed label in the tail bud. In this embryo, no contribution to more anterior positions in the axis were observed, and it is therefore impossible to determine whether these grafted cells truly retained potential to contribute to the axis. Thus, even though these cells were now retained in the tail bud 48 hours after transplant to the anterior primitive streak, this did not select for greater ability to generate descendants both in axis and tail bud.
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DISCUSSION |
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The dramatic involution movements during Xenopus gastrulation cease by the neural plate stage (Gont et al., 1993), as does the transit of a large part of the epiblast through the streak and node/organiser to generate mesoderm in mouse by the equivalent headfold stage (Kinder et al., 2001
; Snow, 1981
). In chick, passage of lateral epiblast cells early during gastrulation through Hensens node ceases prior to node regression (Joubin and Stern, 1999
). Thus, at the start of somitogenesis in vertebrates, the neural, mesodermal and notochordal precursors are no longer in mass transit from the ectoderm but are contained in the region of ingression. We have extended previous studies in the mouse to show that this ingression of cells to the mesoderm layer continues even after posterior neuropore closure around the 35-somite stage. In chick, ingression movements after posterior neuropore closure have also been observed (Knezevic et al., 1998
). These can apparently occur from the dorsal surface, perhaps indicating subtle differences in the organisation and/or movements of vertebrate tail bud tissues. In Xenopus and chick therefore, as in mouse, the posterior neural plate may merely represent a localised remnant of the outer layer of the marginal zone/primitive streak, which continues a form of ingression after gastrulation.
The mouse ventral node has been identified previously as a putative self-renewing progenitor region for the notochord (Beddington, 1994; Wilson and Beddington, 1996
), as its posterior extremity contains labelled cells after culture. In the present study, the apparent population of the posterior end of the notochord by anterior streak derivatives and the posterior neural plate (Fig. 2N,P; Fig. 3C) suggests that the ventral node itself may not contain all notochord progenitors. Instead, the notochord may be supplied from cells in the ectoderm layer that represent more primitive notochord precursors. In chick, too, there is evidence that some notochord progenitors reside in the ectodermal layer, rather than in the ventral node region (Catala et al., 1996
; Catala et al., 1995
; Psychoyos and Stern, 1996
). Furthermore, while passage through Hensens node is a prerequisite for incorporation in the notochord, some notochord progenitors originate outside Hensens node in the anterior primitive streak and are only incorporated there later, presumably during node regression (Psychoyos and Stern, 1996
). The hypothesis that the mouse ventral node does not contain all notochord progenitors is supported by the relative quiescence of cells in the node and notochord (as few as 10% appear to cycle), while cells around the node are dividing rapidly (Bellomo et al., 1996
). Furthermore, the ability of grafted 8.5 d.p.c. node to give rise to notochord in the present study, even when grafted to the anterior streak, suggests that the ventral node contains committed notochord precursors. Therefore the ventral node may contain cells destined only for exit to the notochord, and although dramatic elongation of this structure occurs, mediolateral intercalation (Wilson and Keller, 1991
) may account for much of this elongation. This therefore suggests that notochord, somite and neural progenitors are located close together in the ectoderm layer near the node at 8.5 d.p.c., and we show that these progenitors remain closely apposed in the later CNH.
In the Xenopus tail bud, there is also evidence from labelling very small groups of around one to three cells in the CNH itself during tail elongation that the progenitors of notochord, muscle and neural tube are located close together, or represent single multilineage cells (Davis and Kirschner, 2000). Earlier, during blastopore closure at the neural plate stage, there appear to be more regionally separated cells (Gont et al., 1993
). However, if multilineage cells were located in only a small proportion of the blastopore, lineage labelling larger groups of cells using DiI may not have highlighted such a population.
A stem cell population in the CNH ectoderm?
It has been hypothesised in chick and mouse that cells remaining in the streak or tail bud at the termination of prospective lineage labelling studies represent a minority population composed of self-renewing stem cells in the streak (Beddington, 1994; Psychoyos and Stern, 1996
; Tam and Beddington, 1987
; Wilson and Beddington, 1996
). Evidence for stem cell precursors of myotome (Nicolas et al., 1996
) and spinal cord (Mathis and Nicolas, 2000
) located in or near the posterior midline of the embryo strengthens this hypothesis. However, so far, evidence showing that the prospective lineage labelled cells in the streak are indeed stem cells, and not dead or quiescent cells, has been lacking. We tested whether the two major areas colonised by primitive streak descendants in the tail bud, the TBM and CNH, fulfilled criteria expected of axial stem cells by grafting GFP transgenic cells to 8.5 d.p.c. embryos.
Potency of tail bud in contributing to anterior axial positions
In this study we have shown that the tissues in the tail bud are not developmentally equipotent. Unlike TBM, CNH cells can efficiently incorporate in the axis, differentiating into somites, ventral neural tube and notochord, and giving rise to descendants in the tail bud itself. Within the tail bud, CNH descendants are found in both CNH and TBM, consistent with the observation that the posterior neural plate continues to generate mesoderm long into axial elongation. There was no apparent difference between 10.5 and 12.5 d.p.c. CNH in the anterior extent of labelling or the tissue types colonised. It is therefore likely that this region contains self-renewing progenitors.
The strong bias towards contribution to somites by CNH cells compared with their node-derived antecedents is intriguing. This may result from the composition of the graft. Somites form most of the bulk of the tail, while the neural tube and notochord are a relatively minor population. Alternatively, cells or growth factors at the graft site, at the anterior of the primitive streak, may influence the CNH population to differentiate towards somites. A further characteristic of the graft-derived somites was the occurrence of medially located ectopic somites, sometimes in embryos that also had bona fide intermingling of grafted cells with wild type cells in somites. It is possible that the cluster of grafted cells in the streak may retain information on the periodicity of somites to be formed. An alternative possibility is that as the CNH ectoderm is much smaller than the primitive streak, the grafted cells may include the progenitors of entire somites, effectively creating a heterotopic graft of lateral somite precursors to a location where cells normally exit to medial somites.
In contrast to CNH, TBM is only capable of populating short axial stretches that corresponds to a distance of a few somites. It shows a low frequency of incorporation in axial tissue, and fails to contribute to tail bud. The capacity of TBM cells to contribute to anterior axial positions has also been studied by Tam and Tan (Tam and Tan, 1992), who grafted of small numbers of cells from the tail bud of embryos up to 13.5 d.p.c. These grafts are capable of contributing to much more anterior positions than they would have done in situ. As these authors do not distinguish CNH from TBM in the grafts, it may be that it is a small population of CNH cells included in their grafted population that retain potency, especially to contribute to the tail bud. The relatively low frequency observed by these authors of grafted cell retention in the tail bud (around 20% of embryos) supports this idea. Alternatively, the smaller number of grafted cells used by Tam and Tan (Tam and Tan, 1992
) may intermingle more extensively with the host cells than the TBM grafts in the present study. Larger TBM grafts may therefore be subject to greater community effects that preserve either specification as mesoderm or anteroposterior information. As recently ingressed mesoderm earlier in gastrulation is more restricted in potency than the cells from the ectoderm that produced it (Tam et al., 1997
), it is likely that TBM cells that have undergone ingression from the posterior neural plate, are also restricted in potency.
Serial passage of axial progenitors
When CNH cells are passaged through a second and third generation of embryos in culture, at least some cells retain the capacity to colonise the axis in an identical manner to first generation CNH. These results show that the primitive streak/tail bud can retain descendants of cells initially located near the node over a total of around 90 somites made by the hosts, and strongly suggests that a stem cell population resides in the CNH. When we tested TBM in the same way, this showed the same pattern of incorporation as grafts from fresh 10.5 d.p.c. TBM, albeit a slight increase in the frequency of grafts that incorporate in the axis (compare TBM grafts in Tables 1 and 3). However, this subpopulation of TBM cells that originated from anterior streak does not show any greater tendency for retention in the tail bud than the bulk population of TBM, and argues against stem cells residing in any part of the TBM.
It is interesting to note that the grafts that gave rise to three generations of incorporation in the axis and CNH were descended from initial node grafts that showed contribution to both notochord and paraxial mesoderm. This, together with the observation that many node grafts did not show such contribution, suggests that it is not the node itself, but cells immediately abutting it that were included with the grafted tissue, that demonstrate stem cell-like properties. This would correspond well with the hypothesis, discussed earlier, that the ventral layer of the node contains committed notochord progenitors, while cells in its vicinity in the ectoderm layer constitute less committed (stem cell) progenitors. An interesting parallel to these experiments is seen in studies of the chick node and anterior streak (Charrier et al., 1999). The junction of Hensens node and the anterior primitive streak (the axial-paraxial hinge) shows overlapping expression of genes characteristic of the node (Hnf3b and chordin) and those characteristic of the streak (chicken Tbx6l). Cells from this region are capable of generating notochord, neural tube or somites. Normally this contribution is limited to small regions of the axis, and cells are retained in the tail bud. Deletion of the bulk of Hensens node (excluding the axial-paraxial hinge) results in the interruption of notochord formation, but this resumes further posteriorly. However, deletion of the axial-paraxial hinge results in embryos in which notochord formation continues for a short distance, but is followed by axial truncation. These results imply that this region is important as a signalling centre allowing maintenance of axial elongation, and/or that it contains stem cells for the axis. This is consistent with lineage data in the chick that places progenitors contributing to the entire mediolateral extent of all somites at the anterior end of the streak, in a region overlapping with notochord precursors (Psychoyos and Stern, 1996
).
The hypothesis that stem cells are highly localised at the anterior streak, however, presents a paradox. If stem cells are so highly localised, why do fate maps show that most cells in the anterior streak close to the node give rise only to the medial portion of somites? The precursors of lateral somites lie more posteriorly in the streak at 8.5 d.p.c. (Wilson and Beddington, 1996). Descendants of these also contribute to the tail bud after 24-48 hours culture (Wilson and Beddington, 1996
) (results not shown). However, they do not contribute to the CNH, but instead lie ventrally in the TBM. In contrast, the CNH can generate ventral tail bud mesoderm (Fig. 3A,D; Fig. 7A,K). Therefore, the cells in more posterior regions of the 8.5 d.p.c. streak may represent progenitors already committed to a mesoderm fate, which have themselves arisen earlier from a stem cell population near the node. Nonetheless, the contribution of cells in posterior regions of the 8.5 d.p.c. streak to relatively long axial distances without generating a population in which we can demonstrate extensive potency leaves open the possibility that not all of the postcranial axis is generated by node/streak border and CNH derived-stem cells.
The stem cell progenitors suggested by Nicolas and colleagues for the myotome and spinal cord may therefore reside close together in the regions we have identified: the junction of the node and streak at 8.5 d.p.c., and the CNH at 10.5-12.5 d.p.c. (Fig. 8). Their close physical proximity raises the possibility that a single multipotent axial stem cell type may exist, consistent with the observation that some cells in the Xenopus CNH appear to contribute to neurectoderm, somites and notochord (Davis and Kirschner, 2000). In the myotome, stem cell-derived clones are almost exclusively bilateral (Nicolas et al., 1996
), consistent with our observation that CNH cells contribute bilaterally to host embryos. Our analysis also suggests a location for progenitor cells that contribute to up to six consecutive somites (either unilaterally or bilaterally) in the myotome observed by Nicolas et al. (Nicolas et al., 1996
). The present study would locate such clones posterior to the axial-paraxial hinge at 8.5 d.p.c., and in the TBM from 10.5 d.p.c. Like these progenitors identified by Nicolas et al. (Nicolas et al., 1996
) TBM derived cells contributed to one or both sides of the midline (results not shown). Our identification of the position of putative stem cells in the node/streak junction and the CNH will make it possible to characterise their potency in more detail via single cell transplantation or other forms of clonal analysis.
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ACKNOWLEDGMENTS |
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