The spatial and temporal periodicity of somite formation is controlled by the segmentation clock, in which numerous cells cyclically express hairy-related transcriptional repressors with a posterior-to-anterior phase delay, creating ‘traveling waves’ of her1 expression. In zebrafish, the first traveling wave buds off from the synchronous oscillation zone in the blastoderm margin. Here we show that the emergence of a traveling wave coincides with the anterior expansion of Fgf signaling and that transplanted Fgf8b-soaked beads induce ectopic traveling waves. We thus propose that as development proceeds, the activity of Fgf signaling gradually expands anteriorly, starting from the margin, so that cells initiate her1 oscillation with a posterior-to-anterior phase delay. Furthermore, we suggest that Fgf has an essential role in establishing the period gradient that is required for the her1 spatial oscillation pattern at the emergence of the traveling wave.

Keywords:
Fgf, her1, Oscillation, Segmentation clock, Traveling waves, Zebrafish

The periodic formation of vertebrate somites is governed by the segmentation clock, a congregation of cells that exhibit oscillating expression of hairy-related transcriptional repressors (her1 and her7 in zebrafish) through a negative-feedback loop. In zebrafish, a somite is formed every 30 minutes, and the segmentation clock cyclically exhibits a dynamic spatial pattern of hairy gene expression in the presomitic mesoderm (PSM) with the same periodicity (Fig. 1A, left). Previous reports have demonstrated that the phases of cellular oscillation are highly coordinated in a spatial manner, which results in traveling waves that repeatedly bud off from the synchronized oscillation zone in the posterior PSM, sweep anteriorly, and stop around the future segmentation point (Fig. 1A, middle) (Gajewski et al., 2003; Henry et al., 2002; Holley et al., 2000; Holley et al., 2002; Horikawa et al., 2006; Jiang et al., 2000; Oates and Ho, 2002; Palmeirim et al., 1997; Pourquie, 2003; Saga and Takeda, 2001; Sawada et al., 2000). The traveling waves are the result of phase differences among the oscillating cells in a posterior-to-anterior direction; cells with nuclear dots, with cytoplasmic signals and with no signal are detected sequentially from anterior to posterior, corresponding to transcribing cells, translating cells and non-transcribing cells, respectively (Fig. 1A, right). This pattern of oscillation is maintained throughout segmentation and is referred to as the ‘mature’ pattern. Although many studies have addressed the mechanisms of the mature segmentation clock, very few investigations have focused on the initiation of the segmentation clock (Riedel-Kruse et al., 2007) and little is known about how the traveling wave emerges. In the present study, we investigate this early mechanism through in vivo and in silico experiments using zebrafish as a model system.

In situ hybridization

Whole-mount in situ hybridization (Nikaido et al., 1997) and fluorescent in situ hybridization (Horikawa et al., 2006) were performed as previously described.

Fgf bead transplantation and SU5402 treatment

Fgf8b-soaked bead transplantation and SU5402 treatment were performed as described (Sawada et al., 2001). Bead transplantation was performed at the 30% epiboly stage (~5.0 hpf, as indicated in Fig. S1A in the supplementary material). SU5402 (Calbiochem) treatment was performed at 0.2 mg/ml for 8 minutes (strong treatment in Fig. 2B) or 4 minutes (weak inhibition in Fig. 3A). Then, the embryos were incubated in Ringer's solution for 2 hours.

Time-lapse imaging

Embryos transplanted with Alexa488-injected cells were mounted in 1% agarose. Images were collected at 10-minute intervals with a MZFLIII fluorescence microscope (Leica). Cell tracking and quantification were performed with ImageJ (NIH).

Morpholino injection

Antisense morpholino oligonucleotides for her1/7 were designed as described previously (Henry et al., 2002). Morpholinos were injected at 0.25 mM into single-cell stage embryos.

Emergence of the traveling waves

The traveling wave in an anterior direction first appears at ~70% epiboly [7.8 hours post-fertilization (hpf)], long (~3 hours) before segmentation takes place (Fig. 1B-E; see Fig. S1A in the supplementary material) (Riedel-Kruse et al., 2007). Until this point, her1 oscillation is restricted to the blastoderm margin and is synchronized among cells in this area as reported previously (Riedel-Kruse et al., 2007). At the initiation of the traveling wave, phase delay in an anterior direction is observed, indicating that the traveling wave is created mainly by sequential initiation of her1 oscillation from posterior to anterior. During the synchronous oscillation in the margin, gastrulation movement towards the anterior occurs (see Fig. S1B in the supplementary material) (Warga and Kimmel, 1990), indicating that the marginal cells, which transiently expressed her1, attain a transcription-negative state when the cells exit the marginal area and form the hypoblast layer. This was further supported by a comparison between expression of the PSM marker papc (pcdh8 – Zebrafish Information Network) and her1 (see Fig. S1B in the supplementary material). her1/7 morpholino injection also revealed that the suppression of her1 in the hypoblast depends on its own negative feedback: the her1 expression domain was found to be broadened in morpholino-injected embryos, whereas it was restricted to the marginal area in control embryos (7.0 hpf) (Fig. 1F,G). We did not observe the horizontal waves from ventral to dorsal previously reported (Riedel-Kruse et al., 2007), although we performed precise time-course analysis of her1 expression using embryos of strictly controlled stages (see Fig. S1A in the supplementary material). In the following experiments we focus on the mechanism underlying the emergence of the first traveling wave.

Fig. 1.
Overview of the segmentation clock in the zebrafish embryo. Anterior to top, posterior to bottom. Green, her1 mRNA in situ hybridization; magenta, nuclear counterstain. (A) Subcellular localization of her1 mRNA in the traveling wave during the segmentation stage. (B-E) Emergence of the traveling wave at the blastula stage. The boxed regions are enlarged in the panels beneath. (F,G) Control and her1/7 morpholino-injected samples. The injected morpholino was designed against the first ATG and her1 transcripts were detected with the intron probe; thus, the signals detected cannot result from mRNA stabilized by morpholino binding. Scale bar: 50 μm.
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Overview of the segmentation clock in the zebrafish embryo. Anterior to top, posterior to bottom. Green, her1 mRNA in situ hybridization; magenta, nuclear counterstain. (A) Subcellular localization of her1 mRNA in the traveling wave during the segmentation stage. (B-E) Emergence of the traveling wave at the blastula stage. The boxed regions are enlarged in the panels beneath. (F,G) Control and her1/7 morpholino-injected samples. The injected morpholino was designed against the first ATG and her1 transcripts were detected with the intron probe; thus, the signals detected cannot result from mRNA stabilized by morpholino binding. Scale bar: 50 μm.

Fig. 1.
Overview of the segmentation clock in the zebrafish embryo. Anterior to top, posterior to bottom. Green, her1 mRNA in situ hybridization; magenta, nuclear counterstain. (A) Subcellular localization of her1 mRNA in the traveling wave during the segmentation stage. (B-E) Emergence of the traveling wave at the blastula stage. The boxed regions are enlarged in the panels beneath. (F,G) Control and her1/7 morpholino-injected samples. The injected morpholino was designed against the first ATG and her1 transcripts were detected with the intron probe; thus, the signals detected cannot result from mRNA stabilized by morpholino binding. Scale bar: 50 μm.
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Overview of the segmentation clock in the zebrafish embryo. Anterior to top, posterior to bottom. Green, her1 mRNA in situ hybridization; magenta, nuclear counterstain. (A) Subcellular localization of her1 mRNA in the traveling wave during the segmentation stage. (B-E) Emergence of the traveling wave at the blastula stage. The boxed regions are enlarged in the panels beneath. (F,G) Control and her1/7 morpholino-injected samples. The injected morpholino was designed against the first ATG and her1 transcripts were detected with the intron probe; thus, the signals detected cannot result from mRNA stabilized by morpholino binding. Scale bar: 50 μm.

Fgf signaling triggers her1 oscillation and formation of the traveling wave

Intercellular communication through the Notch pathway is dispensable for the initiation of traveling waves as revealed both by Notch mutants (Jiang et al., 2000) and inhibitor experiments (see Fig. S2A-C in the supplementary material). Furthermore, other types of communication might not be required as our preliminary data suggest that wild-type cells initiate her1 expression when they are surrounded by non-oscillating mutant cells (see Fig. S2D,E in the supplementary material). It is also unlikely that the anterior movement of the mesoderm plays any role, as it would result only in a phase advance towards the anterior and not in a phase delay. These facts led us to speculate that the traveling wave is generated by an extracellular factor that triggers her1 oscillation. Previous studies have shown that Fgf signaling is necessary for clock oscillation in mouse and that Fgf actually induces Hes1 oscillation in murine cultured cells (Nakayama et al., 2008; Niwa et al., 2007; Wahl et al., 2007). Fgf signaling is also known to control the spatial pattern of hairy gene oscillation in zebrafish and chick (Dubrulle et al., 2001; Sawada et al., 2001). However, the role of Fgf in initiating the traveling wave has not been studied. We therefore examined its role in the emergence of the traveling wave in zebrafish embryos.

We found that fgf8a is expressed at the expected stages and location (Fig. 2A). We first confirmed in zebrafish that Fgf is necessary for her1 expression. Treatment of whole embryos with SU5402, a chemical inhibitor of Fgf signaling, abolished the intrinsic traveling waves as well as the marginal her1 oscillation at early stages (Fig. 2B), consistent with previous findings in mouse (Niwa et al., 2007; Wahl et al., 2007). We then asked whether ectopic activation of Fgf signaling would induce her1 oscillation in the embryo. We transplanted Fgf8b-soaked beads into embryos at the stage before the emergence of the traveling wave (see Fig. 2C for ectopic Fgf activity), and then examined their effect on her1 expression 0.5-1.5 hours after transplantation. The results were striking in that the ectopic her1 expression gradually expanded with time, forming a band of her1 expression around the bead in 9 out of 22 dorsally transplanted samples (Fig. 2D), whereas the remainder exhibited ectopic non-band-like expression of her1 around the beads. We confirmed that this ectopic her1 stripe was actually a traveling wave by observing a spatial transcriptional delay in the direction away from the bead: the cells at the transcription-negative, translational and transcriptional states were detected in sequence starting from the site of bead transplantation (Fig. 2E,F). The induced traveling waves were however restricted to the dorsal side and to the mesodermal layer, forming an incomplete circle (Fig. 2G). This suggests the presence of other permissive factors for her1 expression in the future PSM, before the endogenous wave emerges.

One possible mechanism for creating traveling waves by Fgf signaling is that Fgf activity gradually expands in the anterior direction so that it induces her1 oscillation in sequence with a phase delay. To monitor the activity of Fgf signaling, we examined the expression of sprouty 4 (spry4), one of the well-known downstream genes of Fgf signaling, and found that Fgf activity indeed gradually expands anteriorly from the restricted region of the margin (Fig. 2H; see Fig. S1B in the supplementary material). The timing of spry4 expansion correlated well with the emergence of the first traveling wave (Fig. 2H-J; see Fig. S1B in the supplementary material). The mechanism that expands Fgf activity at this stage remains elusive, although endocytosis could regulate this process (Scholpp and Brand, 2004). Taken together, we conclude that the anterior expansion of Fgf activity triggers the first traveling wave that leaves the marginal expression domain.

Fig. 2.
her1 oscillation is induced by Fgf. (A) Expression of fgf8a at the mid (left) and late (right) epiboly stage. (B) her1 expression disappears following treatment with the Fgf inhibitor SU5402. Left and right panels show her1 expression at the stage before (7.0 hpf) and after (9.0 hpf) the emergence of the traveling wave, respectively. (C-G) Ectopic Fgf induces an ectopic her1 traveling wave. (C) Ectopic expression of spry4 was induced by Fgf8b-soaked bead implantation (arrowhead). (D) Ectopic her1 expression (arrow) is first detected in close vicinity to the Fgf bead (left, 0.5 hours after transplantation) and tends to gradually expand with time, forming a band-like expression domain (right, 1.5 hours after transplantation). (E,F) Subcellular localization of induced her1 expression. (Ga-c) Induction of the traveling wave by Fgf bead transplantation occurs only in the hypoblast. Optical sections of the sample shown in E,F along the z-axis (Ga), x-axis (Gb) and y-axis (Gc). x- and y-axes are shown by white and red lines, respectively, in Ga. Hypoblast and epiblast are indicated by arrowheads and asterisks, respectively. (H,I) The regions of Fgf activity, as indicated by spry4 (H), and her1 expression (I) are almost identical. (J) Time-course analysis of the width (in cells) of spry4 and her1 expression. The number of cells showing nuclear signals was manually counted in samples subjected to high-resolution in situ hybridization (images not shown). Error bars indicate s.d. Scale bar: 50 μm.
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her1 oscillation is induced by Fgf. (A) Expression of fgf8a at the mid (left) and late (right) epiboly stage. (B) her1 expression disappears following treatment with the Fgf inhibitor SU5402. Left and right panels show her1 expression at the stage before (7.0 hpf) and after (9.0 hpf) the emergence of the traveling wave, respectively. (C-G) Ectopic Fgf induces an ectopic her1 traveling wave. (C) Ectopic expression of spry4 was induced by Fgf8b-soaked bead implantation (arrowhead). (D) Ectopic her1 expression (arrow) is first detected in close vicinity to the Fgf bead (left, 0.5 hours after transplantation) and tends to gradually expand with time, forming a band-like expression domain (right, 1.5 hours after transplantation). (E,F) Subcellular localization of induced her1 expression. (Ga-c) Induction of the traveling wave by Fgf bead transplantation occurs only in the hypoblast. Optical sections of the sample shown in E,F along the z-axis (Ga), x-axis (Gb) and y-axis (Gc). x- and y-axes are shown by white and red lines, respectively, in Ga. Hypoblast and epiblast are indicated by arrowheads and asterisks, respectively. (H,I) The regions of Fgf activity, as indicated by spry4 (H), and her1 expression (I) are almost identical. (J) Time-course analysis of the width (in cells) of spry4 and her1 expression. The number of cells showing nuclear signals was manually counted in samples subjected to high-resolution in situ hybridization (images not shown). Error bars indicate s.d. Scale bar: 50 μm.

Fig. 2.
her1 oscillation is induced by Fgf. (A) Expression of fgf8a at the mid (left) and late (right) epiboly stage. (B) her1 expression disappears following treatment with the Fgf inhibitor SU5402. Left and right panels show her1 expression at the stage before (7.0 hpf) and after (9.0 hpf) the emergence of the traveling wave, respectively. (C-G) Ectopic Fgf induces an ectopic her1 traveling wave. (C) Ectopic expression of spry4 was induced by Fgf8b-soaked bead implantation (arrowhead). (D) Ectopic her1 expression (arrow) is first detected in close vicinity to the Fgf bead (left, 0.5 hours after transplantation) and tends to gradually expand with time, forming a band-like expression domain (right, 1.5 hours after transplantation). (E,F) Subcellular localization of induced her1 expression. (Ga-c) Induction of the traveling wave by Fgf bead transplantation occurs only in the hypoblast. Optical sections of the sample shown in E,F along the z-axis (Ga), x-axis (Gb) and y-axis (Gc). x- and y-axes are shown by white and red lines, respectively, in Ga. Hypoblast and epiblast are indicated by arrowheads and asterisks, respectively. (H,I) The regions of Fgf activity, as indicated by spry4 (H), and her1 expression (I) are almost identical. (J) Time-course analysis of the width (in cells) of spry4 and her1 expression. The number of cells showing nuclear signals was manually counted in samples subjected to high-resolution in situ hybridization (images not shown). Error bars indicate s.d. Scale bar: 50 μm.
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her1 oscillation is induced by Fgf. (A) Expression of fgf8a at the mid (left) and late (right) epiboly stage. (B) her1 expression disappears following treatment with the Fgf inhibitor SU5402. Left and right panels show her1 expression at the stage before (7.0 hpf) and after (9.0 hpf) the emergence of the traveling wave, respectively. (C-G) Ectopic Fgf induces an ectopic her1 traveling wave. (C) Ectopic expression of spry4 was induced by Fgf8b-soaked bead implantation (arrowhead). (D) Ectopic her1 expression (arrow) is first detected in close vicinity to the Fgf bead (left, 0.5 hours after transplantation) and tends to gradually expand with time, forming a band-like expression domain (right, 1.5 hours after transplantation). (E,F) Subcellular localization of induced her1 expression. (Ga-c) Induction of the traveling wave by Fgf bead transplantation occurs only in the hypoblast. Optical sections of the sample shown in E,F along the z-axis (Ga), x-axis (Gb) and y-axis (Gc). x- and y-axes are shown by white and red lines, respectively, in Ga. Hypoblast and epiblast are indicated by arrowheads and asterisks, respectively. (H,I) The regions of Fgf activity, as indicated by spry4 (H), and her1 expression (I) are almost identical. (J) Time-course analysis of the width (in cells) of spry4 and her1 expression. The number of cells showing nuclear signals was manually counted in samples subjected to high-resolution in situ hybridization (images not shown). Error bars indicate s.d. Scale bar: 50 μm.

Fgf signaling is responsible for the period gradient of the traveling wave

In the mature segmentation clock, the stripes of her1 become narrower as they move anteriorly. This characteristic oscillation pattern has been considered to result from a gradient in the oscillation period along the anterior-posterior (AP) axis (Giudicelli et al., 2007; Gomez et al., 2008; Morelli et al., 2009; Palmeirim et al., 1997; Uriu et al., 2009), which is shorter in the posterior and longer in the anterior PSM. We also confirmed this idea using the phase oscillator model (see Fig. S3 in the supplementary material). This idea appears to hold true at the emergence of the traveling wave because the first traveling wave also becomes narrower as it moves. Furthermore, the Fgf activity gradient (higher in the posterior PSM) is known to affect the spatial oscillation pattern of her1 (Dubrulle et al., 2001; Sawada et al., 2001). These facts raise the possibility that early Fgf signaling regulates the period, as well as the timing of initiation, of her1 oscillation at the emergence of the traveling wave. To directly test this possibility, we weakly inhibited gastrulating embryos with SU5402, in which the gradient of Fgf activity was expected to be uniformly decreased. When the stripe first appeared (for control, t=60; for SU5402 treated, t=90), the her1 stripe in treated embryos became narrower and was formed at a more posterior site than that in control embryos (Fig. 3A). Under our experimental conditions, the mesoderm was maintained after SU5402 treatment, but the PSM was reduced in size along the AP axis (see Fig. S4A in the supplementary material). The reduction in PSM size, however, might not account for the narrower and posteriorly shifted her1 expression band in SU5402-treated embryos because the her1 expression pattern is thought to depend primarily on the oscillation dynamics of unit oscillators (e.g. the period) (Giudicelli et al., 2007; Gomez et al., 2008; Morelli et al., 2009; Palmeirim et al., 1997; Uriu et al., 2009). Furthermore, the effect of SU5402 treatment on cellular movement was limited (Fig. 3B; see Fig. S4B in the supplementary material). Taken together, we conclude that the observed change in her1 stripes induced by SU5402 treatment was mainly attributable to the altered dynamics of her1 oscillation.

Since we were unable to determine directly whether the results obtained by SU5402 treatment were the consequence of an altered oscillation period, we instead assessed the effect of altered period on the spatial oscillation pattern in a mathematical simulation, using the phase oscillator model (see Fig. S3 in the supplementary material). For control embryos, we set the intrinsic frequency (the frequency intrinsically given to each virtual oscillator) as the green line in Fig. 3Ca, so that the observed frequency (the actual frequency in simulation, which is not identical to the intrinsic frequency as a result of cellular coupling) also forms a similar gradient as indicated by the green line in Fig. 3Cb. This reproduced the normal emergence of traveling waves in silico (Fig. 3Cc, left). We then examined the spatial oscillation pattern when the gradient of the intrinsic frequency is uniformly decreased, a situation expected to occur when embryos are treated with SU5402 (Fig. 3Ca,b). Under this condition, the phenotype obtained in vivo is clearly reproduced in the simulation, resulting in a posteriorly shifted and narrower stripe (Fig. 3Cc, right). Furthermore, the opposite phenotype was obtained with Fgf bead transplantation (see Fig. S5 in the supplementary material). All these data support the idea that the oscillation period is controlled by Fgf signaling.

Fig. 3.
Effect of Fgf inhibition on the her1 oscillation period. (Aa-d) Effect of compromised Fgf signaling on the spatial oscillation pattern of her1. (a) Time series of her1 expression in control (upper) and SU5402-treated (lower) zebrafish embryos. We set the 50% epiboly stage as t=0. The boxed regions, in those images taken at the time points that the her1 stripe first appears, are enlarged to the right. Brackets indicate the first her1 stripes. (b) The length of the her1 stripe (line b) and the distance between the her1 stripe and the posterior end of the PSM (line c) were measured and normalized by embryonic size (line a). (c,d) The normalized length of the her1 stripe and the normalized distance of the her1 stripe from the posterior end of the PSM in SU5402-treated embryos were significantly shorter than in the control; **, P<0.01 (n=12 for control embryos and n=11 for SU5402 treatment). Error bars indicate s.d. (Ba-c) The effect of SU5402 treatment on gastrulation cell movement was limited. (a) Time-course images of the labeled cells with or without SU5402 treatment. The cellular movement was then tracked every 10 minutes (b) and quantified (c). The mean net displacement towards the posterior direction (n=25 cells from three embryos for control and n=34 cells from three embryos for SU5402 treatment) reveals no significant difference in gastrulation movement following the treatment (c). Error bars indicate s.d. (Ca-c) Simulation of a decreased frequency gradient. (a,b) The intrinsic (a) and observed (b) frequency. n indicates the number of cells that were given the gradient of intrinsic frequency. The intrinsic frequency for the SU5402-treated case was fixed at 0 in the cells i=1-30 (a, red) (see Fig. S3 in the supplementary material). (c) The simulated stripe pattern of her1 expression when the stripe first appeared in each condition. n and t beneath the panels indicate the number of cells that were given the gradient of intrinsic frequency and the elapsed time, respectively. Coupling between non-oscillatory cells (n=0-30 in the SU5402-treated case) and oscillatory cells was maintained in this simulation, but we confirmed that the same trend was obtained in the absence of coupling.
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Effect of Fgf inhibition on the her1 oscillation period. (Aa-d) Effect of compromised Fgf signaling on the spatial oscillation pattern of her1. (a) Time series of her1 expression in control (upper) and SU5402-treated (lower) zebrafish embryos. We set the 50% epiboly stage as t=0. The boxed regions, in those images taken at the time points that the her1 stripe first appears, are enlarged to the right. Brackets indicate the first her1 stripes. (b) The length of the her1 stripe (line b) and the distance between the her1 stripe and the posterior end of the PSM (line c) were measured and normalized by embryonic size (line a). (c,d) The normalized length of the her1 stripe and the normalized distance of the her1 stripe from the posterior end of the PSM in SU5402-treated embryos were significantly shorter than in the control; **, P<0.01 (n=12 for control embryos and n=11 for SU5402 treatment). Error bars indicate s.d. (Ba-c) The effect of SU5402 treatment on gastrulation cell movement was limited. (a) Time-course images of the labeled cells with or without SU5402 treatment. The cellular movement was then tracked every 10 minutes (b) and quantified (c). The mean net displacement towards the posterior direction (n=25 cells from three embryos for control and n=34 cells from three embryos for SU5402 treatment) reveals no significant difference in gastrulation movement following the treatment (c). Error bars indicate s.d. (Ca-c) Simulation of a decreased frequency gradient. (a,b) The intrinsic (a) and observed (b) frequency. n indicates the number of cells that were given the gradient of intrinsic frequency. The intrinsic frequency for the SU5402-treated case was fixed at 0 in the cells i=1-30 (a, red) (see Fig. S3 in the supplementary material). (c) The simulated stripe pattern of her1 expression when the stripe first appeared in each condition. n and t beneath the panels indicate the number of cells that were given the gradient of intrinsic frequency and the elapsed time, respectively. Coupling between non-oscillatory cells (n=0-30 in the SU5402-treated case) and oscillatory cells was maintained in this simulation, but we confirmed that the same trend was obtained in the absence of coupling.

Fig. 3.
Effect of Fgf inhibition on the her1 oscillation period. (Aa-d) Effect of compromised Fgf signaling on the spatial oscillation pattern of her1. (a) Time series of her1 expression in control (upper) and SU5402-treated (lower) zebrafish embryos. We set the 50% epiboly stage as t=0. The boxed regions, in those images taken at the time points that the her1 stripe first appears, are enlarged to the right. Brackets indicate the first her1 stripes. (b) The length of the her1 stripe (line b) and the distance between the her1 stripe and the posterior end of the PSM (line c) were measured and normalized by embryonic size (line a). (c,d) The normalized length of the her1 stripe and the normalized distance of the her1 stripe from the posterior end of the PSM in SU5402-treated embryos were significantly shorter than in the control; **, P<0.01 (n=12 for control embryos and n=11 for SU5402 treatment). Error bars indicate s.d. (Ba-c) The effect of SU5402 treatment on gastrulation cell movement was limited. (a) Time-course images of the labeled cells with or without SU5402 treatment. The cellular movement was then tracked every 10 minutes (b) and quantified (c). The mean net displacement towards the posterior direction (n=25 cells from three embryos for control and n=34 cells from three embryos for SU5402 treatment) reveals no significant difference in gastrulation movement following the treatment (c). Error bars indicate s.d. (Ca-c) Simulation of a decreased frequency gradient. (a,b) The intrinsic (a) and observed (b) frequency. n indicates the number of cells that were given the gradient of intrinsic frequency. The intrinsic frequency for the SU5402-treated case was fixed at 0 in the cells i=1-30 (a, red) (see Fig. S3 in the supplementary material). (c) The simulated stripe pattern of her1 expression when the stripe first appeared in each condition. n and t beneath the panels indicate the number of cells that were given the gradient of intrinsic frequency and the elapsed time, respectively. Coupling between non-oscillatory cells (n=0-30 in the SU5402-treated case) and oscillatory cells was maintained in this simulation, but we confirmed that the same trend was obtained in the absence of coupling.
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Effect of Fgf inhibition on the her1 oscillation period. (Aa-d) Effect of compromised Fgf signaling on the spatial oscillation pattern of her1. (a) Time series of her1 expression in control (upper) and SU5402-treated (lower) zebrafish embryos. We set the 50% epiboly stage as t=0. The boxed regions, in those images taken at the time points that the her1 stripe first appears, are enlarged to the right. Brackets indicate the first her1 stripes. (b) The length of the her1 stripe (line b) and the distance between the her1 stripe and the posterior end of the PSM (line c) were measured and normalized by embryonic size (line a). (c,d) The normalized length of the her1 stripe and the normalized distance of the her1 stripe from the posterior end of the PSM in SU5402-treated embryos were significantly shorter than in the control; **, P<0.01 (n=12 for control embryos and n=11 for SU5402 treatment). Error bars indicate s.d. (Ba-c) The effect of SU5402 treatment on gastrulation cell movement was limited. (a) Time-course images of the labeled cells with or without SU5402 treatment. The cellular movement was then tracked every 10 minutes (b) and quantified (c). The mean net displacement towards the posterior direction (n=25 cells from three embryos for control and n=34 cells from three embryos for SU5402 treatment) reveals no significant difference in gastrulation movement following the treatment (c). Error bars indicate s.d. (Ca-c) Simulation of a decreased frequency gradient. (a,b) The intrinsic (a) and observed (b) frequency. n indicates the number of cells that were given the gradient of intrinsic frequency. The intrinsic frequency for the SU5402-treated case was fixed at 0 in the cells i=1-30 (a, red) (see Fig. S3 in the supplementary material). (c) The simulated stripe pattern of her1 expression when the stripe first appeared in each condition. n and t beneath the panels indicate the number of cells that were given the gradient of intrinsic frequency and the elapsed time, respectively. Coupling between non-oscillatory cells (n=0-30 in the SU5402-treated case) and oscillatory cells was maintained in this simulation, but we confirmed that the same trend was obtained in the absence of coupling.

Taken together, our findings suggest that at the emergence of the traveling wave, the initiation timing and the oscillation period of her1 are simultaneously controlled by Fgf and co-operatively establish the posterior-to-anterior phase delay in the oscillatory field. In wild-type embryos, the traveling waves appear in a highly coordinated manner despite dynamic morphogenesis during gastrulation. The global control of cellular oscillators by secreted factors, such as Fgfs, could be crucial in this situation. The mechanism by which Fgf signaling modulates her1 negative feedback to induce her1 oscillation and alter the her1 oscillation period remains to be established. Further effort aimed at direct measurements of each reaction step in the her1 negative-feedback loop in response to Fgf will help to identify the Fgf target step, and improve our current understanding of the basic principles governing the emergence of the traveling wave.

We thank Dr Sharron Amercher for providing her1/7 deletion mutants; Dr Julian Lewis for advice and helpful discussions; and the National BioResource Project, Zebrafish, NBRP/Brain Science Institute, RIKEN for zebrafish supply. This work was supported in part by Grants-in-Aid for Scientific Research Priority Area Genome Science and Scientific Research (A and B) and Global COE Program (Integrative Life Science Based on the Study of Biosignaling Mechanisms) from the Ministry of Education, Culture, Sports, Science and Technology (MEXT) of Japan. K.I. was supported by Research Fellowships for Young Scientists from the Japan Society for the Promotion of Science.

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Competing interests statement

The authors declare no competing financial interests.

© 2010.
2010

Supplementary information

Supplemental Figure S1

Fig. S1. Time-course analysis of expression patterns of her1, spry4, papc, no-tail and the process of gastrulation. (A) To minimize individual differences at developmental stages, we collected embryos by the following method. Embryos that spawn within 10 minutes were collected. Embryos that failed to reach or remain at the 4-, 8- and 16-cell stages within 5 minutes at the fixed time were removed so that the developmental time difference was less than 5 minutes. Ten embryos were then fixed every 10 minutes from 5 hours post-fertilization (hpf) to 8.7 hpf. All procedures were performed in a temperature-controlled room at a fixed 28.5°C. Until 7 hours 50 minutes post-fertilization, her1 oscillation occurs only in the margin area, as reported previously (Riedel-Kruse et al., 2007); the intensity of fluorescence of the her1 mRNA signal repeatedly became stronger and weaker in unison. Then, a traveling wave in a posterior to anterior direction was observed. Under our experimental conditions, traveling waves in a ventral to dorsal direction, as previously reported (Riedel-Kruse et al., 2007), were not observed. (B) The stages of the embryos were strictly controlled as described in A. Gastrulation starts prior to the emergence of the traveling wave and to the anterior expansion of Fgf signaling, indicating that the gastrulation movement is not the primary cause of both events; gastrulation starts at ∼6.0 hpf and the emergence of the traveling wave and the anterior expansion of Fgf signaling begins at ∼8.0 hpf. The anterior limit of gastrulating mesoderm is indicated by yellow arrowheads in live embryos (top). The emergence of the traveling wave of her1 and the anterior expansion of Fgf signaling occur at the same stage (8.0 hpf). In addition, both her1 and spry4 are first detected at the same stages (5.0 hpf), suggesting that the early oscillation of her1 also depends on Fgf signaling. papc expression (a marker for the PSM) gradually becomes broader as gastrulation proceeds, while her1 expression remains restricted to the marginal area, supporting the idea that involuting mesoderm cells transiently express her1 before they leave the marginal area and then become negative. no-tail expression (a pan-mesodermal marker) is not identical to that of her1 (the no-tail expression domain is wider than that of her1), indicating that Fgf signaling differentially regulates mesoderm maintenance and clock oscillation.

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Supplemental Figure S2

Fig. S2. The emergence of the traveling wave does not depend on intercellular communication. (A-C) Inhibition of Notch signaling by DAPT does not affect the emergence of the traveling wave. (A) To examine whether the onset of the her1 traveling wave depends on Notch-dependent intercellular signaling, embryos were treated with the Notch signaling inhibitor DAPT as described previously (Horikawa et al., 2006). (B) An embryo treated with DAPT until the emergence of the traveling wave. The traveling wave was created in the absence of Notch signaling. (C) An embryo treated with DAPT after the emergence of the traveling wave. The spatial pattern of the traveling wave is disturbed, with several transcribing cells detected in the transcription-negative area (arrow). This treatment was performed as a positive control to confirm that DAPT treatment was effective. The two experiments were performed under the same conditions, with the exception of the timing of treatment. Although the horizontal oscillation phase is not exactly the same in the traveling wave at the earlier stage, the occurrence of the traveling wave in the absence of Notch signaling indicates that this wave is not the one relayed from marginal oscillation through Notch signaling. (D,E) We performed transplantation experiments to examine whether unknown intercellular coupling plays a significant role in relaying the marginal her1 oscillation to create the traveling wave. Wild-type cells were transplanted into the her1/7 deletion mutant, which lacks the her1/7 genomic region and thus does not produce any type of her1 oscillation, including the marginal one. If the traveling wave does not depend on intercellular signaling triggered by the margin, the transplanted normal cells can initiate her1 oscillation in the mutant background. (D) Schematic of the cell transplantation assay at the blastula stage. Transplantation was performed at the stage before the onset of her1 marginal oscillation. (E) The transplanted cells show her1 expression with proper phase delay. Since her1/7 mutant cells never express her1, the cells with her1 mRNA signal should be donor cells. The arrowheads indicate cells with her1 transcription, whereas the arrows indicate cells with her1 translation, indicating that the transplanted wild-type cells initiate her1 oscillation with proper phase delay. This result excludes the idea that the traveling wave is triggered by the marginal oscillation through intercellular coupling. Scale bar: 50 µm.

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Supplemental Figure S3

Fig. S3. Simulation of the stripe pattern with or without a period gradient. (A,B) The simulation was performed with (A) or without (B) a period gradient. Here, we used the phase oscillator model that considers a population of coupled phase oscillators, in which each oscillator has only a single variable phase (Pikovsky et al., 2001; Acebron et al., 2005). The left-hand figures show the intrinsic and observed frequency in linearly aligned cells, and the right-hand figures show temporal changes of the stripe pattern. The normal spatial pattern of her1 expression, where the her1 stripes become narrower as they move anteriorly, was reproduced when we provided the gradient of oscillation period (A). Although only the initial phase delay without intrinsic frequency gradient can also create traveling waves, the created waves travel with their width constant, which is different from the in vivo pattern (B). For details of the model, see below. To model the traveling waves at the zebrafish blastula stage, one-dimensionally coupled phase oscillators were considered as follows:

dθ1/dt1 + ε sin(θ2− θ1),

dθi/dti + ε sin((θi−1− θi) + sin(θi+1− θi)), i=2...n−1,

dθn/dtn + ε sin(θn−1− θn),

where θi and ωi are the oscillation phase and intrinsic frequency of the ith oscillator, where i is the position of the cells aligned in line, and n is the total number of cells. Coupling between cells is given by a coupling function assumed sin(.) as the simplest case and coupling strength ε. In this study, we used the following parameter sets: n=50 and ε=0.1. The coupling strength is slightly smaller than the value needed to form perfect synchronization in this system. We assigned a spatial gradient to the intrinsic frequency. For the intrinsic frequency in Fig. S4A, ωi is a line connecting ω1=0 at i=1 and ω50=0.075 at i=50. In Fig. S4B, ωi is a uniform value, ωi=0.075, at each cell.

References

Acebron, J. A., Bonilla, L. L., Pérez Vicente, C. J., Ritort, F. and Spigler, R. (2005). The Kuramoto model: a simple paradigm for synchronization phenomena. Rev. Mod. Phys.77, 137-185.

Pikovsky, A., Rosenblum, M. and Kurth, J. (2001). Synchronization: A Universal Concept in Nonlinear Sciences. Cambridge Nonlinear Science Series 12. Cambridge, UK: Cambridge University Press.

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Supplemental Figure S4

Fig. S4. Effect of SU5402 treatment on gastrulation movement and the expression of PSM markers. (A) We examined whether the differentiation and maintenance of the PSM are affected by SU5402 treatment. The presumptive PSM was monitored by the expression of tbx24 and papc. tbx24 is expressed in the anterior two-thirds of the (presumptive) PSM and papc is known to be a paraxial mesoderm marker. Their expression domains were found to posteriorly regress in the SU5402-treated embryos, indicating that SU5402 treatment affects the size of the presumptive PSM. This is not the result of compromised cellular movement because the cellular movement was not affected by SU5402 treatment (see Fig. 3B and Fig. S5B), but possibly by differentiation defects. As described in the main text, we think that the change in her1 spatial pattern in SU5402-treated embryos is not merely a result of decreased size of the presumptive PSM. (B) The anterior limit of the gastrulating mesoderm (yellow arrowheads) reaches the head region normally in the SU5402-treated embryo. This indicates that the gastrulation movement is not substantially affected by SU5402 treatment.

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Supplemental Figure S5

Fig. S5. Effect of Fgf-soaked bead transplantation on the her1 expression pattern. (A) Comparison of her1 expression pattern between control and Fgf bead transplanted sides. Each side of the same sample is shown. The anterior her1 stripe was anteriorly shifted and the posterior her1 expression domain became broadened (n=7/9). The light-blue and magenta dots represent the axial levels of the anterior stripe on control and bead transplanted sides, respectively. White arrows indicate the width of the posterior expression of her1 on each side. The transplantation was performed under the same conditions as in Fig. 2C-G except for the stage of transplantation (∼7.0 hpf). (Ba-c) Simulation of an increased frequency gradient. (a,b) The intrinsic (a) and observed (b) frequency. The intrinsic frequency for the Fgf bead transplantation case was fixed at 0.6 in the cells i=40-50 (red). (c) The simulated stripe pattern of the control (left) and bead transplanted (right) cases, when the stripe first appeared under each condition. The simulated spatial pattern recapitulates well the outcome of Fgf bead transplantation. The anterior stripe was anteriorly shifted and the posterior stripe became broader. The light-blue and magenta dots represent the position of the anterior stripe in the control and bead transplanted cases, respectively. White arrows indicate the width of the posterior stripes. The simulation is based on the same equation as in Fig. 3C. For the control simulation, the anterior non-oscillatory cells were not coupled with the posterior oscillatory cells. t under the panels indicates the elapsed time.

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