MRC Centre for Developmental Neurobiology, Kings College London, Guys Campus, London SE1 1UL, UK
*Author for correspondence (e-mail: andrew.lumsden{at}kcl.ac.uk)
Accepted April 9, 2001
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SUMMARY |
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Key words: Anteroposterior patterning, Hindbrain, Segmentation, Retinoic acid, Morphogen, Chick
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INTRODUCTION |
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The spatial and temporal nature of retinoid influence on gene expression depends on a large number of parameters. These include the local availability of retinoic acid (RA) receptors (RAR, ß,
and RXR
, ß,
) which transduce the retinoid signal, enzymes necessary for RA synthesis and/or catabolism, and intra- or intercellular carrier proteins (Chambon, 1996; Duester et al., 1998). The distribution of RA in the early embryo correlates with the opposing action of the two main RA metabolic enzymes: Raldh2 (Maden et al., 1998a; Niederreither et al., 1997; Berggren et al., 1999), which converts retinaldehyde into RA, and Cyp26, a cytochrome P450 that oxidatively inactivates RA (Swindell et al., 1999; de Roos et al., 1999; Fujii et al., 1997). Raldh2 is strongly expressed in the somites adjacent to the caudal hindbrain and cervical spinal cord (Swindell et al., 1999; Berggren et al., 1999), whereas Cyp26 is strongly expressed in the fore- and midbrain region of the neural plate (Swindell et al., 1999). It has yet to be shown that a posterior-to-anterior gradient of RA exists during hindbrain patterning, but the expression of Raldh2 and Cyp26 is suggestive of a source and sink that would be required to set up such a gradient.
Recent genetic analysis in the mouse has revealed that Raldh2 (Aldh1a2 Mouse Genome Informatics) is crucial for regulating patterning events in the posterior hindbrain. However, the phenotype of Raldh2 knockout mice differs from that described for the VAD quail, as r4 molecular markers are still expressed in these embryos (Niederreither et al., 1999; Niederreither et al., 2000). In female rats, complete VAD leads to reproductive failure, whereas a partial deficiency leads to variable hindbrain defects in the progeny (White et al., 1998; White et al., 2000). Targeted disruption of murine RAR genes also provides information on the roles of RA in anteroposterior patterning. Interestingly, the RAR:RARß compound mutant embryos have normal anterior rhombomeres (r1-r4), but posterior hindbrain markers expand in a posterior direction (Dupé et al., 1999). Similarly, overexpression of dominant negative retinoic acid receptors partially anteriorises the posterior rhombomeres of Xenopus embryos (Blumberg et al., 1997; Kolm et al., 1997; Van der Wees et al., 1998). Targeted disruption of Hoxa1 and Hoxb1 RA response elements (RAREs) reveal further levels of complexity in the actions of RA in anteroposterior patterning (Dupé et al., 1997; Studer et al., 1998). Collectively, these results are not easy to interpret, given the wide disparity of phenotype. In the case of both knockout and dominant negative receptor experiments, uncertainty arises on account of the incomplete inactivation of RA signalling. For both of these approaches, as for the VAD embryos, uncertainty also surrounds the timing of an RA requirement for different aspects of patterning, as RA signalling is depleted throughout development. An approach that could potentially resolve both uncertainties would be to block RA signalling completely or partially at successive, defined stages of development.
Thus, in order to investigate the diverse roles of RA signalling during anteroposterior nervous system patterning, and to explore the exact timing of RA actions, we have used a culture system in which a staged series of chick embryos are exposed to various concentrations of an antagonist that blocks activation of all three RAR isotypes (Wendling et al., 2000). We find that the entire posterior hindbrain develops as a default r4 in absence of RA. Consequently, RA is the transforming signal involved in the specification of posterior hindbrain structures from stage 5 to stage 10+. These actions take place through the regulation of hindbrain segmentation genes in an environment of a retinoid activity gradient. More generally, we have made a thorough analysis of the early RA functions during chick hindbrain patterning.
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MATERIALS AND METHODS |
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The pan-RAR synthetic retinoid antagonist BMS493 (Bristol-Myers-Squibb, Princeton, NJ, USA), diluted in ethanol, was added to the Liebovitz medium at various concentration (10-5M to 10-8M). In control embryo cultures, vehicle (ethanol) was added at the same final dilution.
Molecular analyses
Whole-mount in situ hybridisation with digoxigenin-labelled riboprobes was performed as described by Wilkinson (Wilkinson, 1992), using probes from template plasmids produced in our laboratory (for Hoxb1, follistatin, Cepu-1 and Hoxa1) (Guthrie et al., 1992; Graham and Lumsden, 1996; Jungbluth et al., 2001) or kindly provided by D. Wilkinson (Krox-20) (Wilkinson et al., 1989), J. Dodd (Wnt-8c) (Hume and Dodd, 1993) and I. McKay (MafB/kr).
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RESULTS |
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Exposure of stage 4 (full-length primitive streak) and stage 5 (head process) embryos to a high concentration (5x10-6 M) of antagonist resulted in all embryos developing a shorter anteroposterior axis with smaller and poorly defined somites compared with controls. Treated embryos examined at stage 11 show expanded Krox-20 expression in the r3 domain, with a posterior limit that is not well defined, and lack the characteristic stripe of expression in r5 as well as the neural crest cells (NCC) migrating from r5/r6 (Fig. 1a). Furthermore, the characteristic stripe of Hoxb1 expression in r4 disappears, with Hoxb1 being continuously expressed from a region just rostral to the first somite down to the posterior neuropore (Fig. 1k,l). Corresponding with the posterior limit of Krox-20 expression, the rostralmost region of Hoxb1 expression lacks a sharp border and contains patches of unlabelled cells. The characteristic expression of MafB/kr in r5 and r6 is absent (compare Fig. 1i with 1j). Identical results were obtained using a higher concentration of antagonist (10-5 M).
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When treated with the antagonist at stage 6+, embryos have normal r3 Krox-20 expression but display patches of Krox-20-positive cells in the r5 region, although these patches extend posteriorly beyond the expected r5 territory (Fig. 1c,d). This patchy expression of Krox-20 may represent the appearance of r5-like cells. Indeed, in embryos treated at stage 6+, we observed patches of Hoxb1-negative cells at the expected axial level of the r5 region (compare Fig. 1n with Fig. 1c,d). Hoxb1 expression domains such as this are not seen when embryos are treated slightly earlier (stage 6). MafB/kr expression also appears in scattered patches, but the staining does not appear more extended than that of Krox-20, indicating that, at this stage of treatment, r6-like identity is absent (Fig. 1e).
Embryos treated at stage 7 (one-somite stage) display a normal r3 and the number of Krox-20-positive cells in the most posterior domain is increased; their anterior limit corresponds to a normal anterior r5 boundary, whereas their posterior limit extends beyond the expected location of r5/r6 boundary (Fig. 1f). At this stage of treatment, Hoxb1 expression in r4 is normal (data not shown).
Treatment of stage 7+ and 9- embryos (two- to six-somite stages; n=12) does not affect the size of r4, but r5 is markedly enlarged, as shown by the expression of Krox-20 (Fig. 1g). follistatin expression at stage 13 in embryos treated between stage 7+ and 9- confirms the expansion of the morphologically recognisable r5, and shows abnormal caudal expansion of putative r6 and r7 (Fig. 1p). However, follistatin expression is not detected in the neural tube posterior to the sixth somite. MafB/kr expression is also extends beyond the expected location of r6/r7 boundary (data not shown).
Embryos treated between stage 9 and 9+ (seven- to eight-somite stages) have normal expression of Krox-20 in r3 and r5 but, as shown by follistatin expression, they have an enlarged r6 and r7 (Fig. 1q). Again, this expanded expression in the neural tube is not found beyond somite 6.
In embryos treated between stage 10- and 10+ (nine- to 11-somite stages), only the r7 is expanded, reaching the 3rd somite, as MafB/kr expression is normal and the characteristic weak expression domain of follistatin in r7 is enlarged (data not shown). From stage 11-, the presence of antagonist in the culture medium no longer affects patterning of the hindbrain.
These data implicate RA in the specification of rhombomere boundaries from stage 5 to 10+. Furthermore, this RA dependency is lost progressively from anterior to posterior as development proceeds.
Establishment of hindbrain boundaries is dependent on RA concentration
To test the idea that a graded RA concentration could mediate hindbrain patterning, we applied various concentrations of the antagonist to cultured embryos at stage 4, and used Krox-20, follistatin, MafB/kr and Hoxb1 to reveal the size of rhombomeres. As a function of the concentration used, we have obtained a range of phenotypes that we have classified in six arbitrary types from very affected embryos, as described previously for a 5x10-6 M concentration, to normal embryos (Table 1).
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At a lower concentration of antagonist (10-6 M), we observed new phenotypes, the most significant of which was the appearance of Krox-20-expressing cells in ectopic posterior positions. Indeed, of the embryos treated at 10-6 M, 45% developed either patches of Krox-20-expressing cells or a continuous domain of Krox-20 expression with poorly defined boundaries (Fig. 2a, Table 1). The anterior limit of this ectopic Krox-20 expression lies as far posterior as the level of the second somite, whereas the posterior limit can reach the level of the 6th somite. We never observed Krox-20 expression in the neural tube posterior to somite 6. This ectopic expression of Krox-20 may represent the appearance of a greatly enlarged r5-like territory in a more caudal region. In this case, the large unstained region of the hindbrain between the r3 caudal border and the level of somite 2 would correspond to r4. Indeed, we found Hoxb1 to be expressed throughout the expanded Krox-20-negative region between r3/r4 and somite 2, and to be absent from the expanded Krox-20-positive domain between somite 2 and somite 6 (Fig. 2g). Therefore, the elongated anterior stripe of Hoxb1 expression does correspond molecularly to an enlarged r4.
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When the concentration of antagonist was reduced to 2.5x10-7 M, all of the embryos had a more clearly defined r5 and the proportion of embryos with slightly enlarged r4, r5, r6 and r7 decreased to 27%. Interestingly, at this concentration, 41% of the embryos had a slightly enlarged r4, whereas r5, r6 and r7 were of normal size (Table 1). This is shown by expression domains of Krox-20, Hoxb1 and follistatin. Furthermore, some embryos developed bilaterally asymmetric phenotypes, with an enlarged r4 and r5 on one side of the hindbrain and a less enlarged r4 and almost normal r5 on the other (Fig. 2d).
At 10-7 M antagonist, 46% of the embryos had a slightly enlarged r4 (Fig. 2e,h,m), whereas 44% had a normal hindbrain segmentation; at 5x10-8 M antagonist, only 14% had a slightly enlarged r4, whereas 86% had a normally segmented hindbrain; at 10-8 M antagonist, we saw no effects at all (Table 1).
RA acts as a posteriorising signal
During the formation of rhombomere boundaries, Hoxb1 is selectively expressed in the developing r4 in rodents, quail and chick (e.g. Sundin and Eichele, 1990; Murphy et al., 1989). In contrast to rodents, where Hoxb1 disappears from the rest of the neural tube, expression persists in the stage 11 chick and quail embryos all along the neural tube posterior to r7 (Sundin and Eichele, 1990). The expression of Hoxb1, Krox-20 and MafB/kr in VAD quail embryos led Maden et al. (Maden et al., 1996) to conclude that r4 was absent in these animals. Conversely, Hoxb1 expression in VAD rat embryos and Raldh2 knockout mouse embryos suggests that r4 is still present, but enlarged (White et al., 2000; Niederreither et al., 2000).
In order to determine whether or not r4 had totally disappeared in antagonist-treated chick embryos, we have used additional hindbrain markers. Embryos exposed to highly concentrated antagonist (5x10-6 M or 10-5 M) at stage 4 and allowed to develop to stage 11, display an extended expression of follistatin in r2 (Fig. 3b). Surprisingly, in these embryos, follistatin is strongly expressed in the neural tube from the r3 caudal boundary into the spinal cord down to the axial level of somite 6 (Fig. 3b). Furthermore, there is a strong downregulation of follistatin expression in the anterior mesencephalon of treated embryos (Fig. 3b).
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CEPU-1 is a cell-adhesion molecule that is specifically expressed in r3 and r4 during early hindbrain segmentation (Fig. 3e) (Jungbluth et al., 2001; Spaltmann and Brummendorf, 1996). Embryos exposed to antagonist (5x10-6 M) at stage 4 and allowed to develop to stage 10, display a considerably extended expression domain of Cepu-1 in the parasomitic neural tube (Fig. 3f). As for Wnt8c, this expanded expression of Cepu-1 in the neural tube extends posteriorly as far as somite 6, but no further. As the enlarged r3 is morphologically distinguishable at this stage, we conclude that the neural tube posterior to this rhombomere expressing Cepu-1 has acquired an r4-like identity down to the level of the sixth somite.
The abnormal expression patterns of follistatin, Wnt8c and Cepu-1 in RA-deficient chick embryos collectively indicate that cells with r4 molecular expression characteristics form a defined domain from the r3/r4 border to the region of the neural tube at the axial level of the sixth somite. Thus, in the absence of RA signalling the posterior hindbrain (including the posteriormost, parasomitic region) is anteriorised and has an r4-like identity.
Hoxa1 is downregulated in antagonist-treated embryos
During early gastrulation, Hoxa1 mRNA expression extends from the posterior end of the embryo along both the neurectodermal and mesodermal layers up to the presumptive r3/r4 boundary (Fig. 4a). At early somite stages, Hoxa1 expression begins to regress caudally, later becoming localised to the tailbud (Sundin et al., 1990). The product of Hoxa1 is essential during hindbrain segmentation. Hoxa1-knockout mice have an enlarged r3 and it has been shown that expression of Hoxa1 posterior to the prospective r3 is regulated through RAREs during the presomite stage (Dupé et al., 1997; Studer et al., 1998). In order to determine if the enlarged r3 observed in antagonist-treated embryos is due to downregulation of Hoxa1, we exposed stage 4 embryos to 5x10-6 M antagonist and allowed them to develop to stage 7. This treatment downregulates Hoxa1 expression anteriorly, with the anterior limit of high level expression retreating posteriorly from the expected r3/r4 boundary (Fig. 4b). This abnormal Hoxa1 expression is not observed in embryos treated with a 5x10-7 M and 10-7 M of the antagonist.
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DISCUSSION |
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Abrogation of RA signalling results in the enlargement of r4
Treating chick embryos at stage 4 with the 5x10-6 M antagonist, produces a hindbrain phenotype that is identical, in terms of morphology and molecular marker expression, to that described for VAD quail embryos that have a complete absence of endogenous RA (Maden et al., 1996; Maden et al., 1998b). Embryos develop a shorter AP axis with smaller and poorly defined somites (Fig. 3b,f). Furthermore, patterning of the r2-r7 region is profoundly altered, with enlarged r2 and r3, absence of the r5 Krox-20 expression, loss of MafB/kr expression, and with Hoxb1 expressed continuously throughout the posterior hindbrain and spinal cord (Figs 1, 3). Interestingly, the few rat embryos obtained under conditions of absolute retinoid deficiency exhibit similar Hoxb1 expression (White et al., 2000).
However, the phenotype of the VAD quail and that resulting from the blockade of RA signalling by the BMS493 antagonist are interpreted differently. In their studies on VAD quail embryos, Maden et al. concluded that r4 is absent (Maden et al., 1996; Maden et al., 1997; Maden et al., 1998b). This was on the basis of Hoxb1 expression, which, in the neural tube of VAD quail embryos, extends caudally from just anterior to the first somite in these embryos; the distinctive r4 stripe of Hoxb1 expression is absent but the continuous posterior domain looks similar to the cervical spinal cord domain of Hoxb1 in normal embryos (see fig. 3 in Maden, 1996). In the absence of other r4 markers, the reasonable conclusion by Maden et al. (Maden et al., 1996) was that r4 is lost, and that r3 abuts spinal cord. We see an identical pattern of Hoxb1 expression in the antagonist-treated embryos but, by contrast, we offer a different interpretation of the upper reaches of the parasomitic domain, arguing that it is not spinal cord but hindbrain. Specifically, it is r4. Thus, we have shown that in antagonist-treated embryos, follistatin is expressed posterior to the enlarged r3 down to the level of the 6th somite, indicating that this region has a hindbrain identity. Furthermore, expression of the r4 marker Wnt8c in antagonist-treated embryos shows that as early as stage 8, presumptive r4 cells are not restricted to a stripe, as in control embryos, but are found in parasomitic neural tube down to the level of somite 6. Finally, Cepu-1, another r4 marker, is also expressed down to the level of somite 6. We conclude, therefore, that the blockade of RA signalling in chick does not result in the loss of r4; rather, it results in the formation of an enlarged r4. In the light of this observation, the hindbrain phenotypes observed in RA-deficient chick and VAD quail and rat are actually similar to the one observed in Raldh2-knockout mouse, where Hoxb1- and Wnt8-expressing cells expand posteriorly into the spinal cord region (Niederreither et al., 1999; Niederreither et al., 2000).
On the basis of the interpretation by Maden et al. of the VAD quail (Maden et al., 1996), where RA signalling is completely absent, it has recently been suggested that the Raldh2 mutants may have residual RA signalling (Gavalas and Krumlauf, 2000). Our analysis, however, suggests that there is a complete deficiency of RA in the Raldh2 mutant hindbrain. It is therefore reasonable to assume that the RA implicated in hindbrain patterning is produced exclusively by Raldh2 activity.
As early as stage 4, Raldh2 is expressed lateral to the primitive streak with a sharp anterior boundary. At stage 7, transcripts are abundant in the paraxial mesoderm and display an anterior boundary at the level of the first somite (Berggren et al., 1999; Swindell et al., 1999), corresponding with the future location of the r6/r7 boundary. A similar anterior boundary of RA production has been shown by Maden et al. in the chick using a RA reporter cell assay (Maden et al., 1998a). It has been proposed that RA synthesised at high levels in the first and subsequent somites diffuses anteriorly through the hindbrain at early stages and contributes to establishment of Hox gene expression patterns (Swindell et al., 1999; Berggren et al., 1999; Maden, 1999; Grapin-Botton et al., 1998). As Raldh2 is detectable in cervical somites but not in the more rostral unsegmented paraxial mesoderm, and because our results are consistent with Raldh2 being the sole source of RA in hindbrain patterning, the RA effects we and others have described must be long range.
The posteriorising effect of RA is restricted to the hindbrain
Our results show that proper specification of the post-otic neural tube also requires RA. Interestingly, only the region of neural tube down to level of the sixth somite is anteriorised by abrogating RA signalling. Indeed, we never saw expression of hindbrain markers posterior to the sixth somite. What might be distinct between the neural tube regions anterior and posterior to the sixth somite? There is no obvious correlation with weaker expression of Raldh2 in the somites, as those posterior to somite 6 also express the gene (Swindell et al., 1999; Berggren et al., 1999). However, there is known to be a fundamental change of neurectodermal cell fate and potential at this juncture in the neural tube, with particular respect to the neural crest. Rostral to somite 7, the neurogenic crest is fated to form enteric ganglia whereas caudal to somite 5 it is fated to give rise to sympathetic neurons (Le Douarin and Kalcheim, 1999). That the cells rostral to this point have the broad ectomesenchymal potentials of cephalic crest, which are lacking from more caudal crest (Nakamura and Ayer-le Lievre, 1982), is perhaps an even more significant difference. Fate-mapping studies have shown that the avian skull is derived from neural crest ectomesenchyme, together with paraxial mesoderm, down to the level of the fifth somite (Couly et al., 1993), the scelerotome of the upper cervical somites being incorporated into the occipital region of the skull. Although the neural tube of this region acquires a dorsoventral cell pattern that is characteristic of spinal cord, it is contained within the skull; it is thus properly designated as hindbrain rather than spinal cord, thus corresponding to the rhombomere 8 described by Lumsden and Keynes (Lumsden and Keynes, 1989; see also Cambronero and Puelles, 2000). In summary, it appears that dependency on RA for correct anteroposterior patterning is restricted to the hindbrain, by this strict anatomical definition, and that in embryos that completely lack RA signalling, the posterior hindbrain (r5-r8), takes on the identity of a large r4 region by default.
RA is implicated in the specification of hindbrain borders in a stage-dependant manner
We have shown that RA is required for proper hindbrain segmentation from stage 5 to stage 10+. Furthermore, the specification of gene expression borders, and presumably future rhombomere boundaries, has an RA dependency that is lost progressively in an anterior-to-posterior sequence as development proceeds. The results of producing a deficiency of RA signalling at successive stages of early hindbrain development are summarized in Table 2. The first action of RA appears to be at stage 5, as we observed the same hindbrain phenotype when embryos are treated (5x10- M antagonist) at stage 4 or 5. In embryos treated at stage 6, Krox-20 expression is normal in r3, suggesting that RA is no longer required for maintaining the r3/r4 border after stage 6. Our results also indicate that RA is no longer required for maintaining the r4/r5 border after stage 7+, the r5/r6 border after stage 9, the r6/r7 border after stage 10- and the r7/r8 border after stage 10+ (Table 2). However, Gale et al. were able to rescue the hindbrain phenotype of VAD quails by treating the embryos with RA as late as stage 8 (Gale et al., 1999), showing that the hindbrain has enough plasticity to respond to RA until this stage.
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Antagonist treatment can mimic the RAR:RARß mutant phenotype
Embryos treated at stage 8- have a similar phenotype to that of the RAR:RARß compound mutant mouse embryos, which have normal anterior rhombomeres (r1-r4), but enlarged r5 and r6 (Dupé et al., 1999). This suggests that RARß and RAR
are implicated in later aspects of RA signalling in patterning the posterior hindbrain, whereas RAR
may be implicated in earlier aspects, for example, in controlling Hoxa1 expression (see below). This is underscored by the fact that RARß has an anterior limit of expression in the neural tube corresponding to the r5/6 boundary (Smith and Eichele, 1991), and RARß is downregulated in the presence of antagonist (Wendling et al., 2000; data not shown).
RA signalling plays an essential role in the specification of the r3/r4 border by regulating early Hoxa1 expression
Several anteriorly expressed Hox genes harbour RAREs in their regulatory sequences and require RA for establishment of their normal expression domains in the hindbrain (Gould et al., 1998; Marshall et al., 1994; Studer et al., 1994; Langston and Gudas, 1992; Pöpperl and Featherstone, 1993). Antagonist-treated chick embryos and Raldh2 mutant mouse embryos display altered Hoxa1 expression, similar to the effect of a targeted disruption of the Hoxa1 RARE. These mouse mutants later develop an enlarged r3, similar to that noted for our antagonist-treated embryos (Niederreither et al., 1999; Dupé et al., 1997). Activation of Krox-20 at the level of r3 is dependent on signals that must be propagated from r4, and these signals are downstream from Hoxa1 and Hoxb1. Furthermore, Hoxa1 is required for the expression of Hoxb1 in the anterior region of r4 (Helmbacher et al., 1998; Studer et al., 1998; Rossel and Capecchi, 1999; Barrow et al., 2000; Giudicelli et al., 2001). In the present work, the fact that the anterior limit of Hoxa1 expression is found at a more posterior level in treated embryos explains the enlargement of r3, as the signal is produced at a more posterior level and may not reach its normal limit. Thus, enlargement of r3 in antagonist-treated embryos is directly due to the downregulation of Hoxa1. By extension, it indicates that RA is essential for establishing the anterior limit of Hoxa1 expression at stage 5. Moreover, our culture experiments, using various concentrations of antagonist, suggest that the Hoxa1 RARE is capable, in vivo, of responding to low concentration of RA, as only a very high concentration of antagonist can lead to an enlarged r3. This is also suggested by the effect of supplementing VAD rat embryos, as a 0.5 µg/g RA diet is sufficient to shift the rostral limit of Hoxb1 expression from the level of the first somite (in the case of complete retinoid deficiency) to the region of the r3/r4 border (White et al., 2000).
A gradient based on RA responses operates in the posterior hindbrain
Krox-20 and MafB/kr are among the earliest known genes to be expressed with an anteroposteriorly restricted pattern within the hindbrain. The ectopic expression (i.e. Krox-20 in anterior r4) or downregulation (i.e. Krox-20 in r5 and MafB/kr in r5-r6) of these genes in our 5x10-6 M antagonist treated embryos, support the idea that RA signalling acts at the head of the genetic hierarchy involved in the control of the hindbrain segmentation.
Our results indicate that the normal non-expression of Krox-20 posterior to r5 and MafB/kr posterior to r6 is due to the presence of a high concentration of RA in this region. Indeed, we have seen from our experiments that a weak RA deficiency leads to upregulation of Krox-20 and MafB/kr in the parasomitic (postotic) hindbrain, and Maden et al. have shown the presence of a high level of RA in the neural tube posterior to r6 (Maden et al., 1998a). Retinoids may cooperate with fibroblast growth factors (FGFs) in this process, as it has recently been shown that FGF signalling pathways are likely to participate in the determination of the posterior limit of expression of Krox-20 and MafB/kr in the hindbrain (Marin and Charnay, 2000).
Furthermore, we have shown that RA signalling controls Krox-20 and MafB/kr in a dose-dependant way in the postotic hindbrain. Indeed, with complete RA deficiency, we lose Krox-20 and MafB/kr expression in r5 and r5/r6, respectively, and a progressive increase of RA availability results in activation of their expression in the neural tube anterior to the level of the sixth somite. Eventually, when RA signalling is unaffected, expression is suppressed in the posterior end of this domain. This indicates that only a low concentration of RA can activate Krox-20, MafB/kr and maybe other segmental genes in presumptive r7 and r8, whereas a higher concentration is necessary to obtain the normal sharpening expression of these genes (as discussed above). Interestingly, similar ectopic expression of Krox-20 was previously obtained using VAD rat embryos supplemented insufficiently with RA (White et al., 2000).
Grapin-Botton et al. have postulated the existence of a morphogen in a posterior-to-anterior decreasing gradient (Grapin-Botton et al., 1998). MafB/kr would be expressed in a window of morphogen concentration in this gradient. Using various concentration of antagonist, we saw a posterior shift of MafB/kr expression, consistent with the posterior displacement of a window of RA signalling strength. When the concentration of RA antagonist is increased, the r4/r5 region produces an enlarged r4, and the r6/r7 region has ectopic expression of MafB/kr. This is strong support for the existence of an endogenous gradient of RA activity, and that this is indeed the morphogen postulated by Grapin-Botton et al., Regulation of Krox-20 in r5 may well depend on a smaller window in the same gradient.
The existence of an RA gradient has been proposed previously, based on expression experiments involving the RA-synthetic enzyme Raldh2 and the enzyme responsible for RA inactivation, Cyp26 (Swindell et al., 1999; Berggren et al., 1999). However, in the light of our work, we have to keep in mind that the specification of the rhombomere boundaries by RA (from r3/r4 to r7/r8) is stage dependent. In this context, it is difficult to consider a continuous RA concentration gradient between the posterior and anterior extremities of the hindbrain that would also persist from stage 5+ to stage 10. Furthermore, a simple source-sink model for such a gradient may be inappropriate, considering that we and others are able to rescue the hindbrain phenotype simply by RA administration to the embryo (Niederreither et al., 2000; Gale et al., 1999; White et al., 2000; data not shown). Together, these features suggest the presence of an active mechanism that would distribute RA along the hindbrain at the appropriate concentration. This mechanism may depend on a large number of parameters, considering that the RARE-containing hindbrain patterning genes have different RAREs that respond differently to RA (Langston and Gudas, 1992; Marshall et al., 1994; Mendelsohn et al., 1991). A further complication is the distribution of CRABPI, which may act as a supplementary local source, or sink, for RA (Ruberte et al., 1991). Furthermore, the results of inactivating Cyp26A1 confirm the role of this enzyme in cleaning RA from specific embryonic areas to protect them against inappropriate RA signalling. In the context of the hindbrain, Cyp26A1 is required to generate an RA-free domain in the rostral hindbrain, defining the position of r3/r4 boundary (Abu-Abed et al., 2001; Sakai et al., 2001). In this respect, other RA-metabolising enzymes may perform additional specific hindbrain functions by modulating RA levels.
In conclusion, our results have enabled us to interpret or re-interpret some of the wide disparity of hindbrain phenotypes previously observed in various models of RA deficiency (Maden et al., 1998b; Niederreither et al., 2000; White et al., 2000; Dupé et al., 1999). Specifically, we have shown that RA signalling is required for correct patterning of the posterior hindbrain, by its wider (anatomical) definition that includes rhombomere 8 (i.e. down to the level of s6) and this entire region acquires an r4-default identity in absence of RA. In terms of RA requirement, anterior rhombomeres are established and independent of RA signalling at an earlier stage than posterior rhombomeres. Stabilisation of rhombomere pattern thus proceeds in a strict rostral-to-caudal procession. It is also clear that successively more posterior rhombomere boundaries are successively more sensitive to a RA deficiency, suggesting that they require progressively higher concentrations of endogenous RA for their correct positioning. Our work strongly supports the hypothesis of a gradient of RA activity in the hindbrain, but this gradient is likely to be a dynamic one, considering the many levels of complexity that accompany RA signalling pathways. Hindbrain development is more likely to be dependent on graded RA responses rather than on a linear RA concentration gradient.
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ACKNOWLEDGMENTS |
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