Segmentation is a common feature of disparate clades of metazoans, and its evolution is a central problem of evolutionary developmental biology. We evolved in silico regulatory networks by a mutation/selection process that just rewards the number of segment boundaries. For segmentation controlled by a static gradient, as in long‐germ band insects, a cascade of adjacent repressors reminiscent of gap genes evolves. For sequential segmentation controlled by a moving gradient, similar to vertebrate somitogenesis, we invariably observe a very constrained evolutionary path or funnel. The evolved state is a cell autonomous ‘clock and wavefront’ model, with the new attribute of a separate bistable system driven by an autonomous clock. Early stages in the evolution of both modes of segmentation are functionally similar, and simulations suggest a possible path for their interconversion. Our computation illustrates how complex traits can evolve by the incremental addition of new functions on top of pre‐existing traits.
Many metazoans are segmented, that is, their body plan is based on the repetition of metameric units (e.g. segments in arthropods, vertebrae in vertebrates).
Segments originate from the localized expression of segmentation genes in early embryogenesis. However, the specific mechanisms of segmentation are very different among species, raising the question of their independent evolutionary origin (Peel et al, 2005). In long‐germ insects, segments appear in parallel, under the control of static morphogen gradients––such as bicoid in Drosophila that is established maternally (Rivera‐Pomar and Jäckle, 1996). In short‐germ insects and vertebrates, segments are produced sequentially from a posterior growth zone (Pourquié, 2003; Liu and Kaufman, 2005a, 2005b). For the case of vertebrate somitogenesis, segmentation has been shown to be controlled by dynamic morphogen gradients expressed at the tail bud (such as FGF8 (Dubrulle and Pourquié, 2004) or Wnt3a (Aulehla et al, 2003)) coupled to a segmentation clock supposed to control the timing of formation of segments (Palmeirim et al, 1997).
We have previously designed an evolutionary algorithm (François and Hakim, 2004) that generates networks of interacting genes and proteins implementing a predefined function in a single cell. Here, we modify this algorithm to evolve patterning mechanisms in a simulated multicellular embryo, and investigate the possible origin and mechanisms of segmentation. The algorithm acts on a population of organisms where the dynamics of a morphogen gradient G are prescribed. With the help of a mutation/selection process, it randomly builds networks. Stripes are defined by the expression domain of a reporter gene E and selection acts to increase the number of stripes: the more the stripes in the embryo, the fitter the organism.
We first tested this strategy for simulated embryos under the control of static morphogen gradients. Networks evolved toward cascades of adjacent repressors, suggestive of topologies observed in the Drosophila segmentation network (Figure 3C and G) (Kraut and Levine, 1991a, 1991b). For instance, in the created network displayed on Figure 3G the reporter gene E is repressed by two repressors R1 and R2, and R2 is repressed by R1. This produces two stripes of expression of E, on both sides of a broad domain of expression of R2 controlled by repressor R1. This topology is reminiscent of eve (E) stripes 3–7 and 4–6 regulation in Drosophila by hunchback (R1) and central knirps (R2) (Clyde et al, 2003). Interestingly, we observe in the simulations the repeated creation of a specific feed‐forward motif (Figure 3B) that allows the localized expression of a protein at middle concentrations of a morphogen (Green, 2002) and appears widely used in actual patterning processes.
For segmentation under the control of a dynamic morphogen gradient G, the evolutionary process converged toward networks coupling bistable networks to oscillators. The observed evolutionary pathway is very constrained: first, a bistable system evolves upstream of the reporter gene E. This is a necessary step for the network to remember positional information once the dynamic morphogen gradient has disappeared (Figure 4B). The following evolutionary move is to create a repressor R that restricts the expression of the protein E and produces a localized stable stripe of E expression (Figure 4C). In the next event, R can negatively regulate itself with a delay creating a clock controlled by the moving morphogen gradient (Figure 4D). Temporal oscillations of protein R yield a striped spatial expression of protein E: when R is downregulated, E repression is lifted, and E can stabilize to a high concentration steady state; while when R is at high concentration, E is repressed and converges toward the low concentration steady state. Coupling of these temporal dynamics to the moving morphogen front implements in a simple way the ‘clock and wavefront model’ (Cooke and Zeeman, 1976): the oscillation phase is encoded in a binary way and rendered permanent by the bistable dynamics of E as the morphogen G decreases to 0.
Two aspects of these results appear specially worth emphasizing. First, although the gene network responsible for somitogenesis is certainly more complex than the networks created by the evolutionary algorithm, they provide simple and conceptually useful models: segmentation can directly follow from a cell‐autonomous transition between oscillation and bistability.
Delayed negative feedback has already been proposed (Lewis, 2003) as a mechanism for the segmentation clock with genes in the hairy/E(spl) family playing the role of the repressor R, and partition of the anterior PSM into Notch1/Dll1 high‐ and low‐activity domains (Morimoto and Saga, 2005) is suggestive of bistability. This new molecular model may be useful for other patterning process coupled to growth, such as short‐germ segmentation (Liu and Kaufman, 2005a, 2005b) or limb bud growth (Pascoal et al, 2007a, 2007b). A second remarkable feature is the spontaneous and constrained evolutionary creation of oscillatory/bistable networks since the scoring function does not contain any particular element to favor them, beyond the production of a segmented pattern. Although the computer description is very simplified, this strongly suggests that evolution of this mode of segmentation is not especially difficult and may have appeared several times in metazoan evolution in convergent ways.
We show that it is computationally feasible to evolve genetic networks producing multicellular patterns, taking segmentation in a morphogen gradient as an example.
For segmentation under the control of a static gradient, computational evolution led to networks with cascades of repressors, similar to that observed in Drosophila. Evolutionary pathways include the early creation of a feed‐forward motif which serves to express a gene at an intermediate morphogen concentration and appears widely used in actual biological networks.
For segmentation under the control of a dynamic gradient, computational evolution spontaneously created network topologies coupling bistability and oscillations, implementing a “clock and wavefront” reminiscent of that observed in vertebrate somitogenesis. This provides a general class of molecular models for patterning coupled to growth.
Although only a minority of the around 30 bilaterally symmetric animal phyla display a segmental anterior–posterior body plan, examples can be found in each of the three major clades of bilaterians (Tautz, 2004). Thus the question, did segmentation appear once in some putative ‘urbilaterian’ and was then lost from most phyla or did it evolve several times? The great variety of embryonic patterning mechanisms found among insects, annelids, and vertebrates argues for the later alternative. The appearance of similar genes in the segmentation networks of diverse phyla (Peel et al, 2005) raised the question of whether this was independent recruitment or common ancestry. In this study, we simulate the evolution of transcriptional regulatory networks subject to a fitness function favoring segments. We find the repeated emergence of networks sharing a common structure that resembles what is observed in nature.
The segmented bodies of insects and the somites of vertebrates are the two best characterized segmentation networks. Insects divide into long‐germ band species such as Drosophila that create all segments in parallel, and short‐germ species such as Tribolium that segment the head and thorax first and pattern the abdomen later, together with the elongation of the posterior growth zone (Liu and Kaufman, 2005b). Segmentation is under the control of morphogen gradients, for example, the anterior activator bicoid (bcd) in Drosophila that is established maternally. Segments of long‐germ band insects are carved from broad domains of activation by short‐range repression due to gap genes (Rivera‐Pomar and Jäckle, 1996). The genes responsible for these patterns can change, most famously bcd is not present in other long‐germ band insects such as mosquito, though its functions of anterior activation and translational repression of caudal (cad) mRNA are subsumed by other genes (Liu and Kaufman, 2005b).
The segmented structures of the vertebrate body, such as the vertebrae and skeletal muscles arise from the somites, blocks of paraxial mesoderm cells partitioned into anteroposterior domains by segmentation of the pre‐somitic mesoderm (PSM). Somites are produced from the posterior growth zone or tail bud (Pourquié, 2003), through the interaction of time‐periodic gene expression or a ‘clock’ with a morphogen wavefront that moves along with posterior growth, as insightfully proposed 30 years ago by Cooke and Zeeman (1976). Candidates for the morphogen include signaling molecules such as FGF8 (Dubrulle and Pourquié, 2004) and Wnt3a (Aulehla et al, 2003). While many cycling genes are known, including a homolog to the Drosophila pair‐rule gene hairy (Dequéant et al, 2006), much less is known about the segmentation clock than other genetic oscillators such as the circadian clock. The transition between the oscillating posterior PSM and the more anterior segmented part is also still under investigation (Morimoto and Saga, 2005).
We have previously designed an evolutionary algorithm (François and Hakim, 2004) that generates networks of interacting genes and proteins that implement a predefined function in a single cell. The simulations successfully produced circuits very similar to circadian clocks when subject to selection that favored periodic behavior. We evolved segmentation in silico using a suitably adapted version of this procedure to investigate its possible origin and mechanisms. In the following, we show that for a static morphogen gradient, segmentation networks evolve toward cascades of repressors. When the gradient becomes dynamic, they evolve toward molecular networks implementing a ‘clock and wavefront’ mechanism in a new way.
Evolution in silico
The evolutionary procedure is similar to the one described in François and Hakim (2004). The strategy is to evolve genetic networks by repeated rounds of selection, growth, and mutation.
The algorithm evolves a population of transcriptional regulatory networks. We represent the binding of a transcription factor A to the regulatory region of gene encoding a protein P by a Michaelis function, with an equilibrium binding constant, AP and a Hill coefficient n to represent cooperative effects. A gene is described by a maximum protein production rate, SP, a time delay, τP, (to represent all the steps between transcription and the appearance of new protein (Lewis, 2003; Monk, 2003)) and a decay rate, δP. The rate of protein production defined by the regulatory interactions in Figure 1 is described mathematically as follows:
When multiple activators are present as in Figure 1, their combined output is defined by the maximum of their activities. Repressors are combined multiplicatively. This is analogous to using an OR between activators and an AND between repressors in discrete systems. Gene regulation is vastly more complex than our simple model, yet if one were to measure protein production in response to changing levels of activators and repressors, the trends would be captured by our model.
Each network is evaluated in an ‘embryo’, which consists of a linear array of cells (typically 100) sharing the same genetic network. The embryo is one‐dimensional: there is only one cell for each anteroposterior position x along the embryo. Cells are independent and cannot communicate with each other. A protein G provides positional information to these cells. We impose the dynamics of this ‘effector protein’, which we assume to reflect the effect of a morphogen gradient. For simplicity, we call G the morphogen in the following. The only difference between cells in the same embryo is through their exposure to G, which is a prescribed function of x and the same in all embryos. A reporter gene E, whose product defines the segments, is introduced into the system. Selective pressure acts on the final profile of this protein.
Integration of the gene network equations in each embryo then allows us to rank the genetic networks according to a predetermined scoring or fitness function that counts the number of boundaries in the profile between low and high states of E (see below).
A hundred networks are followed in parallel. The first generation network for all the simulations is the morphogen G and uncoupled from it the reporter E. At each step of the algorithm, after the fitness function is computed, the 50 best networks are retained; then each is copied and mutated. Mutations can create or destroy genes, add or remove transcriptional regulatory linkages (e.g. G activates E), and change any parameter. After the mutation step, the entire process is iterated. A ‘generation’ is one iteration of this selection/growth/mutation process, and corresponds to many generations in a real organism since we are only concerned with mutations in the one network under study. An overview of the algorithm is provided in Figure 2.
The fitness function is a crucial ingredient in our evolution of segmentation. Darwin originally proposed that a complete eye could have evolved from a simple sensor if gradual changes increased the ability to derive information about the environment from light and were inheritable (Darwin, 1859; Nilsson and Pelger, 1994). This argument potentially applies to any complex trait; if there is a sequence of small steps each increasing the fitness that lead to the desired trait, then evolution can be rapid. It thus appears reasonable to assume that segmentation arose from the potential benefit of more specialization and modularity in the body plan.
To test this scenario in our computations, segmentation was simply defined as the spatial alternation between high and low concentrations of the test protein E. We then chose as a fitness function the number of boundaries (transitions in either direction between low and high) or ‘steps’ in the concentration of E. This mathematically represents the general evolutionary pressure that an increase in the number of segments is beneficial without making arbitrary assumptions such as insisting on predefined levels of E or rewarding only seven segments in the case of Drosophila. These more specific functions not only contravene the notion of genericity and gradualism, they also greatly slow the evolution, which reduces to a random search through a vast space with no clues indicating proximity to the desired state (see Figures S1–S3 in Supplement).
The second crucial ingredient in our evolutionary computation is the choice of the dynamics of the morphogen G. We explore two possibilities. In a first introductory set of simulations, we take G to be a static gradient as in the fly (Figure 3). For the more complicated case of sequential segmentation, we take a uniformly translating (sweeping) exponential step (Figure 4B–E) decreasing from a constant concentration to a concentration that is effectively 0 (i.e. smaller than relevant binding affinities). This mimics formation of a signaling gradient upon exit from a growth zone, similar to what happens in the PSM during somitogenesis. Therefore, it is not necessary to model growth of the tail bud, and for computational convenience, we just extend the (constant) morphogen over all the posterior cells. The number of boundaries in E is counted after the morphogen front has run down the row of cells and is close to zero everywhere.
Static gradient: in silico evolution produces cascades of repressors
To test the relevance of the method on a simplified example, we first considered the in silico evolution of segmentation under the control of a static morphogen gradient. Two typical examples of simulations are displayed in Figure 3A–C and D–G with the major stages of their evolutionary pathway.
Both evolutionary pathways begin in the same way: after few generations, the gene E is put under the control of the graded morphogen, and is transcriptionally activated when the morphogen G exceeds some level (Figure 3A and D).
A few generations later, the next event creates R1, a repressor of E, only active in the region where the morphogen is highest. As a result, this creates a second boundary (E from high to low) in the region of R1 activity (Figure 3B and E).
The evolutionary processes then fork for the later generations. In the first case, a second repressor R2 is created, which represses R1 in regions of yet higher concentration of the morphogen. This creates a new region of E activity, where R2 lifts R1 repression (Figure 3C), so that E is expressed in two broad domains.
In the second case, a second repressor R2 is created by neutral evolution, at an intermediate concentration of the morphogen G, and is repressed by R1 in regions of higher concentration of G. Then, R2 represses E, which increases the fitness by splitting the broad stripe of Figure 3E into two smaller stripes, delimitated by the regions of high repressor (Figure 3F). Later in the evolution, mutual repression between repressors R2 and R1 is selected to sharpen the boundary of one stripe (Figure 3G and Supplementary Figure S4).
Each stage in this evolutionary process creates new boundaries by repressing or derepressing E. In the example of Figure 3C, the evolutionary pathway creates a cascade of repressors. Cascades were often found by the algorithm, since cross‐regulating repressors create adjacent regions of expression of E. Such networks, based on a cascade of repressors, are suggestive of some part of the actual Drosophila gap‐gene regulation network as discussed below.
Dynamic gradient: spontaneous evolution of a ‘clock and wavefront’ mechanism
Since the algorithm succeeded in creating some simple networks controlling localized expression of genes in a static gradient, we allowed the gradient to sweep to create a dynamic morphogenetic profile.
An example of a network with the corresponding evolutionary pathway is displayed in Figure 4.
The first stage in the evolution of the sequential segmentation simulation (Figure 4) is always activation of E at some intermediate level GE of the initial gradient and then positive feedback of E onto itself so that high values are self sustaining while low values decay to zero. This generates one step after the morphogen gradient runs over the cells and G equals 0 everywhere (Figure 4B). Bistability is the first functionality to evolve.
The next event is to create a repressor, R, of E that itself is induced only for morphogen levels G greater than GE. This can occur either by placing a pre‐existing repressor of E under the control of G or adding repressor function to some other gene controlled by G.
Several conditions should be met for R to create a second boundary of E expression without destroying the first one. First, to preserve the boundary from low to high E expression:
R should turn on later than E while the morphogen is sweeping past, so that E has time to autoactivate before being repressed. Typically R turns on for higher value of G than E, but the opposite could be true if R turns on much more slowly than E.
the high value of E in the bistable system should be stable (persist) for low values of R. Weak induction of R by the exponential tail of G should not destroy the stable high value of E.
The creation of a second boundary, from high to low E concentration, requires that full expression of R should repress E expression strongly enough to prevent its autoactivation, thereby creating a limited domain where E concentration is high.
When these conditions are satisfied, R drives E to zero well ahead of the morphogen front, while in the morphogen‐decaying tail, an island of autoactivated E remains (Figure 4C and Supplementary Figure S5).
Subsequent evolution creates, however, a more spectacular improvement (Figure 4D) and a large fitness increase. In addition to repressing E, the protein R becomes a transcriptional repressor of its own gene. This negative feedback loop produces temporal oscillations in R so long as G is large enough to induce R. The oscillations in R produce islands of E for the same reasons as before. The oscillation phase is encoded in a binary way and rendered permanent by the bistable dynamics of E as G decreases to 0. Figure 5 illustrates this mechanism at the level of individual cells. As a consequence of this process (and with the exception of the very first segments), all segments are of the same size as can be seen in Figure 4E: segment size is simply given by the product of the velocity of the front times the period of the clock. Bistability further implies sharp boundaries between domain of high and low E expression. There are only two possible concentrations for E at steady state and therefore E concentration profile jumps abruptly from one cell to the next.
After several dozen evolution experiments for a variety of mutation parameters, the only networks that produced more than one or two stripes always displayed a clock coupled to a bistable system (see several examples in Supplementary Figures S6–S11). However, some variability in the detailed sequence of events was observed, most often in the final stage (R represses itself) when sometimes multiple repressors would appear, as in Figure 6 (evolutionary pathway is displayed in Supplementary Figure S8). Each repressor creates a single additional step in E, until finally an oscillator (similar in principle to the engineered ‘repressilator’; Elowitz and Leibler, 2000) is created for a big increase in fitness. An interesting property of this repressilator network is that delays are not required for it to work efficiently and to produce many stripes (even though delays are needed along the evolutionary pathway leading to it).
To investigate the generality of these conclusions and the ubiquity of the path leading to the clock and wavefront model, we did 20 additional simulations with identical parameters and stopped them after a fixed number of generations (Table I). Five of the simulations consisted of a clock coupled to a bistable system. In one, the oscillations were damped, and in network 17 a repressilator‐like clock evolved (as illustrated in Supplementary Figure S12), slightly different from the one displayed in Figure 4. Interestingly, all networks evolved at least a bistable system, and several others one or more repressors, for example, network 7 had a cascade of repressors and two others stopped at the stage displayed in Figure 2C.
When we increased the rate of topology‐changing mutations relative to those that changed parameters, the evolutionary path remained the same but the fraction of high fitness ‘clock and bistable’ systems increased. Finally, we chose random mutation rates and repeated the evolution using the same dynamic morphogen and the same fitness function. Again we found only networks with topologies coupling clock and bistable systems or ones on the path leading to it, as detailed in Table II. In this sense, there is a common path or fitness funnel that all systems traverse as their fitness increases.
The evolved cascades of repressors resemble some modules of Drosophila segmentation network
Both terminal networks in Figure 3 have approximate analogs in selected modules of the Drosophila system with E a pair‐rule gene such as even‐skipped (eve), and the various repressors acting as gap genes. From Figure 3C, knirps (kni) and giant (gt) are known to be complementary and mutually repress in the anterior part of the embryo (Kraut and Levine, 1991a). gt defines the anterior border of the central Krüppel (Kr) domain (Kraut and Levine, 1991b) and possibly splits it off from the weak and dynamic Kr anterior domain (e.g. Figure 2 of Wu et al, 1998).
The situation in Figure 3G is loosely like eve stripes 3–7 or 4–6 in that one module creates two stripes with two repressors, one central kni and the other hunchback (hb) defining the outer boundaries of the pair of stripes (Clyde et al, 2003). The analogy is incomplete in that the eve stripes are created from a uniform activator, while we have a spacial gradient and the simulation simply uses the limit of the activator domain in place of hb to define the anterior boundary of the anterior stripe. Mutual repression seen between R1 (hb) and R2 (kni) occurs in the evolved system when a small term favoring sharp boundaries is added to the fitness.
The algorithm is therefore able to generate small modules with topology close to gap genes interaction generating localized expression domains. The complete Drosophila patterning system involves both anterior‐ and posterior‐anchored morphogens, hence is much more complex than what we have simulated. Drosophila segmentation network is also a highly derived and hierarchical system (Peel et al, 2005), presumably from more primitive (short germ) insects, so that evolution of a complete long‐germ band segmentation system may require steps passing through a dynamic mode of segmentation (see below). The networks presented here only suggest possible building blocks for formation of gap or segmentation gene domains (or anterior patterning in short‐germ band insects).
More uniform domains of expression could be obtained if a subsidiary term were added to our primary fitness function favoring that feature (see for an example, Supplementary Figure S13). Uniform stripes in the fly may be a vestige of its presumed short‐germ band ancestor where uniform segments arise naturally from a clock and wavefront system. Simply counting boundaries as we do, leaves the spacing, shape, and intensity of the segmentation marker completely unregulated. In reality, selection will further play on these features while leaving the topology of the network unchanged.
Finally, note that the network topology displayed in Figure 3B (and also in Figure 4C) is a very general mechanism to create a limited zone of expression of a protein E at intermediate concentration of an effector G. There are several examples in contexts other than segmentation where one signal activates a protein over a threshold and shuts it down at higher concentration via activation of a repressor. For instance, in Xenopus development, the gradient of Activin induces Brachyury (Xbra) and then Goosecoid (Gsc), that in turn represses Xbra (Green, 2002).
Network evolution suggests new models of sequential segmentation
Somitogenesis has long been the subject of quantitative modeling (reviewed in Baker et al, 2006). The model suggested by the evolutionary algorithm is characterized by a combination of two features: (1) a cell autonomous clock dependent on the morphogen and (2) an independent bistable system driven both by the morphogen and clock, which we identify as the anterio‐posterior somite marker. Most existing models focus on more specific aspects of somitogenesis. Lewis (2003) proposed a clock based on delayed negative feedback among genes in the hairy/E(spl) family and demonstrated its robustness against changes in transcription rate and mRNA levels. The evolved network extends this model and suggests that a bistable system may provide a discrete encoding of the phase and sidestep the more subtle task of remembering the continuous phase suggested in Kerszberg and Wolpert (2000). Evidence for some bistability in single cells comes from experiments where elimination of one of several delta paralogs is thought to desynchronize oscillations, and yields a salt and pepper pattern for an anterior somite marker (Jiang et al, 2000). We find partition of the anterior PSM into Notch1/Dll1 high and low activity domains suggestive of our bistable ‘gene’ E (Morimoto and Saga, 2005).
Another model (Baker et al, 2006) mathematically describes the behavior in the transition zone by imposing thresholds on the moving morphogen front. This is only part of the problem, and our evolved network by construction gives a full model transforming the prepattern into a static array of segments. Meinhardt (1986) was the first to suggest an explicit model of the complete process and proposed that diffusion or long‐range inhibition between cells played an essential role in segmentation. Our model is situated in the opposite limit and is purely cell autonomous.
The sweeping of the morphogen step ties segmentation to the growth of new tail bud. In a static gradient, each segment requires a new inhibitory interaction as can be seen in Figure 3. Therefore, it is hard to generate more than a few segments. In contrast, in a temporal gradient, the addition of a clock to a series of one or more repressors appears as the highly favored way to create many segments within our simulations.
Thus, it is tempting to speculate that in short‐germ insects or in myriapods, a clock will be found to complement the moving morphogen gradient implicit in the elongating posterior growth zone (Peel et al, 2005). Recently, a gradient of mkp3 has also been observed during chick limb bud growth (Pascoal et al, 2007a) and cyclic hairy2 expression has been demonstrated (Pascoal et al, 2007b). Interestingly, the period of the limb bud formation clock is much longer than in the segmentation clock. These results suggest that similar clock and wavefront mechanisms, based on different molecular players, may apply to other sequential segmentation processes.
Simple as it is, our evolved model suggests biochemical interactions (such as the need of bistability to fix the pattern) that may be checked experimentally. It admits refinement, such as cell–cell communication, that may be necessary to keep the phase of the different oscillators synchronized and makes the somite boundary straight in the direction perpendicular to the morphogen gradient, and deals with the bilateral symmetry. Such elaborations need not destroy the core cell autonomous dynamics and the basic synchrony imposed on a field of cells by the morphogen will enhance the efficacy of cell–cell communication. Other variants can display additional features of the experiments that did not spontaneously evolve such as the traveling waves posterior to the front (Palmeirim et al, 1997; Dequéant et al, 2006). Such phase waves could be simulated if one allowed the period of the clock (mainly under control of the transcriptional delay in R in the network displayed on Figure 4) to vary along the oscillatory region, for instance under control of a secondary gradient. Further work is needed to explore more precisely the interplay among the clock, bistability and morphogen interactions in our system.
Our simulations and recent experiments suggest a possible evolutionary path between short‐ and long‐germ insects. In the basal short‐germ insect Oncopeltus, Liu and Kaufman (2005a) show that the prototype fly pair‐rule gene eve actually feeds back and activates the anterior gap genes hb and Kr. The situation is very suggestive of the evolved network in Figure 6. The cascade of repressors is common to what we found for a static morphogen, and eve is one target of that cascade. The feedback of eve into this cascade (i.e. E activates R3 in Figure 6) could create an oscillator and thus drive sequential segmentation. The early anterior gap‐like expression of eve in Drosophila could be a vestige of this feedback interaction, which could be a key transition linking short‐ and long‐germ band insects. A recent reassessment of the phylogeny among the major groups of Holometabolous insects (Savard et al, 2006) makes the Hymenoptera (which includes the long‐germ band wasp Nasonia (Lynch et al, 2006)) an outgroup with respect to Diptera (which includes long‐germ band insects) and Coleoptera (which includes short‐germ species such as Tribolium). Thus interconversion between these two modes of development has occurred multiple times, and evolutionary simulations suggest a possible pathway for the evolution.
Incremental evolution produces complex networks from a generic fitness function
How can a numerical simulation performed in complete ignorance of the actual mutation rates hope to capture even a cartoon version of actual evolutionary pathways? The key assumption, we believe, is the incremental increase in fitness, and the contingency imposed on subsequent stages of evolution by the earlier ones.
Evolutionary simulations for segmentation under the control of static gradients spontaneously evolved toward cascades of repressors. New segment boundaries arose by the addition of new proteins to the cascade, which restrict the domain of expression of the downstream proteins. Evolution of sequential segmentation seems much more constrained. The first stage that couples bistability to a moving front of G is the only way to create one persistent step. A single cell sees a temporal pulse of G, and from that stimulus has to assume either the high or low state. This defines bistability.
Adding one or more repressors creates additional high/low E boundaries just as it did for a static gradient G. A negative feedback oscillator is then only one mutation away from the repressor itself. Note that repression accomplishes both the regulation of E and the oscillations, so one protein can perform both functions. In conformity with ideas about the evolution of biochemical pathways (Horowitz, 1945), somitogenesis in our simulation evolves by adding functionality upstream to an existing, less fit, process.
The strict serial construction of a network renders the process independent of rates of mutation. Numerically correct rates become important when there are several parallel routes to the same end; then the one realized depends on the rates evolution explores them. A computational reconstruction of evolution is most likely to succeed when real biological networks are built serially. This may only be true on the macro‐scale that we have modeled, while there may be many ways of making a bistable system and negative feedback oscillator and the one chosen depends on numbers.
Certain of our ‘genes’ such as the bistable E may be pre‐existing modules that are just recruited by the morphogen G. The composite nature of our ‘genes’ does not matter, evolution merely has to stitch pieces together. The relationships among the nodes of our network, such as bistability and negative feedback, could be realized no matter what the actual molecular interactions are.
The choice of fitness is crucial, and it is noteworthy that separate bistable and oscillatory modules evolved in response to a fitness function that only scored the number of boundaries in E. Both observations and theory support our choice of a nonspecific fitness function. Although somite number is a characteristic of an organism, it is notably disassociated from other taxonomic features (Richardson et al, 1998). Temperature shock can change somite number (Primmett et al, 1988), and local environment can shift the segment number of centipedes (Arthur and Kettle, 2001). Once the topology of the somitogenesis system is established, the number or spacing of somites can be varied with the clock period or front velocity as occurs between the backbone and tail of a mouse (Richardson et al, 1998). Our function describes a component of fitness common to all metazoans that favors segmentation. For a particular phylum, there will be additional terms that are hard to deduce a priori that favor a particular number and size of segments. Mathematical search is efficient when one can move continuously uphill and arrive at the optimum. Similarly, biological evolution is rapid when positive selection controls the succession of states realized. Our fitness function, since it is parameter free and rewards only ‘topological’ properties of the solution, provides just such a smooth bias to facilitate, in a natural way, the evolutionary search.
Robustness and evolution of genetic networks
Screening for parameter independence has been used to select among biological networks. The one which realizes the known transformation (taken from an extant organism) for the widest range of parameters is considered as the most plausible (von Dassow et al, 2000; Eldar et al, 2002).
This implicitly corresponds to a mode of evolution in big jumps, each one creating a complex network (with associated parameters); the first one that works is selected. However, searching through all possible networks takes much longer than building them incrementally. When evolution progresses by small fitness‐increasing increments, purifying selection will control deleterious changes in the values of sensitive parameters (see also Galis et al, 2002) once there is a workable network topology.
For sequential segmentation, we found an almost unique evolutionary path from an unsegmented ancestor to a species embodying a novel version of the clock and wavefront model of somitogenesis. We term this a fitness funnel and note that it is an argument for convergent evolution. Conversely, the observation of networks with similar topology realized by non‐homologous genes is evidence for convergent evolution.
The traditional strategy for modeling a biological system is to start with a network defined by genetics, obtain constants for the interactions (from diverse sources), and then hope it works. However, this strategy does not shed light on the invariant dynamical structure that a particular set of genes implement. This structure is important to understand since it can be implemented by different genes in different species. For instance, rather surprisingly, there appears to be only a small overlap when comparing the genes that oscillate during somitogenesis in the chick and mouse (O Pourquié, private communication). Evolving a network as we have done inverts this procedure. A logically complete dynamical model comes first, lacking all connections to the genes. These models are compact or condensed in comparison to the number of genes implicated in the processes. Thus if correct, multiple genes will impact each model variable, allowing for non‐trivial predictions or at least a principled organization of the genes into a network.
If the topology of biological networks can be deduced by evolutionary simulations from a generic fitness function that gives rise to a fitness funnel, then evolution should be viewed more as a learning process than an optimization process. Networks that can be learned quickly are what we observe, even if they are not the global optimum of some fitness function specific to an organism and an environment.
Materials and methods
The evolutionary algorithm used in this study is similar to the one described in François and Hakim (2004). Further details on this are provided in the Supplementary information.
We thank Cori Bargmann, Eric Davidson, Claude Desplan, Ariel Levine, Alin Vonica and the anonymous referees for their useful comments on the manuscript. This study was supported by the CNRS and the National Science Foundation Grant DMR‐0517138 to EDS.
Supplementary Information [msb4100192-sup-0001.pdf]
↵† Order of authors is alphabetical.
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