Skip to main content
Download PDF
  • Research article
  • Open access
  • Published:

Temporal diversification of Central American cichlids

BMC Evolutionary Biology volume 10, Article number: 279 (2010) Cite this article

Abstract

Background

Cichlid fishes are classic examples of adaptive radiation because of their putative tendency to explosively diversify after invading novel environments. To examine whether ecological opportunity increased diversification (speciation minus extinction) early in a species-rich cichlid radiation, we determined if Heroine cichlids experienced a burst of diversification following their invasion of Central America.

Results

We first reconstructed the Heroine phylogeny and determined the basal node to use as the root of Central American Heroine diversification. We then examined the influence of incomplete taxon sampling on this group's diversification patterns. First, we added missing species randomly to the phylogeny and assessed deviations from a constant rate of lineage accumulation. Using a range of species numbers, we failed to recover significant deviations from a pure-birth process and found little support for an early burst of diversification. Then, we examined patterns of lineage accumulation as nodes were increasingly truncated. We assumed that as we removed more recently diverged lineages that sampling would become more complete thereby increasing the power to detect deviations from a pure-birth model. However, truncation of nodes provided even less support for an early burst of diversification.

Conclusions

Contrary to expectations, our analyses suggest Heroine cichlids did not undergo a burst of diversification when they invaded from South America. Throughout their history in Central America, Heroine cichlids appear to have diversified at a constant rate.

Background

Patterns and rates of speciation vary tremendously among clades. Vertebrate groups such as coelecanths or bowfin fishes that were once species rich, underwent bouts of extinction, and now are represented by few extant species [1]. Alternatively, diversification (speciation minus extinction) in other clades such as cichlid fishes can be explosive. In several instances, cichlids have diversified incredibly rapidly resulting in species assemblages that dominate many freshwater habitats [2–4]. Both intrinsic and extrinsic forces could underlie the tendency of cichlids to rapidly diversify. Intrinsic factors such as innovations in jaw structure [5, 6] and reproductive phenotypes like mouth brooding [7] have been suggested to drive rapid diversification in these fishes. However, in the largest of the East African Rift lakes, extrinsic factors such as the ecological release these cichlids encountered upon colonizing Lakes Tanganyika, Victoria, and Malawi could have fueled their bursts of unparalleled diversity [3, 8]. The absence of predators or competitors in these three massive, relatively old lakes could have been the key to the rapid filling of niches with the hundreds of endemic cichlid species that now occur sympatrically in each lake. However, it is generally unclear how important the invasion of novel habitats is to cichlid diversification [9] and if cichlids presented with novel ecological circumstances frequently experience a burst and subsequent slow-down in cladogenesis. To examine the hypothesis that novel ecological opportunity facilitates an increase in cichlid diversification rate, we determined whether Heroine cichlids underwent a burst of diversification following their invasion of Central America.

Central American (CA) Heroine cichlids are thought to represent an adaptive radiation that like many other cichlid radiations could have undergone a burst of diversification early in their history. Based on one taxonomic database [10] and recent species descriptions [11–13] there are 122 named species in this clade with 114 of these inhabiting the region north of the Panamanian Isthmus. These fishes are also extremely trophically diverse and exhibit an incredible array of putatively adaptive jaw morphologies [14–18]. The Heroines are nested phylogenetically within a more evolutionarily disparate group of cichlids [19] that has occupied South America since at least the Eocene, 40-55 million years ago [20]. The diversity in CA Heroines has been attributed in part to the paucity of Central American representatives of groups like catfish and characiform fishes that dominate South American freshwater ecosystems [21, 22]. Additionally, the few other cichlid lineages that occur north of the Panamanian Isthmus, Geophagus and Acarichthys, have only a few Central American species and likely did not colonize Central America until the emergence of the Isthmus of Panama, 3 million years ago [23]. Because of the lack of competing fish lineages, Central America likely offered a huge opportunity for adaptive divergence when Heroine cichlids invaded this region from South America. However, it is unclear if the adaptive diversity and species richness of the CA Heroines is largely a result of an early burst of explosive speciation as is predicted under many scenarios of adaptive radiation [24, 25].

There are several microevolutionary studies that suggest that the diversification of CA Heroines continues to occur rapidly. This radiation contains some of the best-documented cases of intraspecific trophic polymorphism in vertebrates [26, 27]. For example, species such as Herichthys minckleyi and Amphilophus citrenellus exhibit polymorphic jaw morphologies that allow individuals within the same populations to exploit highly different prey types [27, 28]. Some of the most thoroughly examined cases of sympatric speciation also occur in this radiation [29–31]. These cases of on-going divergence in the Heroine cichlid radiation suggest that speciation in these fish is strongly influenced by ecological opportunity. Also, these instances of recent divergence could be used to argue diversification in the CA Heroine radiation has not slowed since the Heroine invasion of Central America.

Many large radiations like the CA Heroines exhibit clear patterns of slowdown in diversification towards the present [32, 33]. Evaluating the patterns of diversification during a clade's history requires the ability to assess the temporal patterns of cladogenesis. Recent advances in the ability to estimate phylogenies and branch lengths have made evaluating temporal patterns of speciation feasible [34–38]. Lineage through time (LTT) studies also depend on time-calibrated phylogenies [34] and a determination of which ancestral node is relevant to begin examining the effects of novel conditions on clade diversification. Fortunately, an increasingly robust view of the interrelationships of CA Heroine cichlids is coming to light. Also, because of the ability to reconstruct ancestral areas, such as inhabiting Central America or not, and the relatively clear colonization of CA Heroines from South America, determining which cichlid clades to include in a LTT analysis should be feasible. If Heroine cichlids underwent an explosive phase of lineage diversification when they colonized Central America, this pattern should be detectable.

When evaluating the temporal variation in diversification rate of an adaptive radiation like the CA Heroines it is critical to account for incomplete sampling of lineages [35]. Species in a molecular phylogeny can be incompletely sampled because of unavailability of DNA sequences for known lineages and/or taxonomic inaccuracies in the delineation of species diversity. Simulations can be used to correct for an incomplete sampling of lineages in a phylogeny via the creation of null distributions that generate random trees and subsequently prune lineages from phylogenies [35, 37]. Both underestimation of the number of "true" lineages [39] and overestimation of the number of species can also lead to inaccurate estimation of species diversity [40, 41]. This taxonomic inaccuracy likely influences the evaluation of recent LTT patterns most. To remedy this problem, many LTT studies have somewhat arbitrarily truncated the most recent 2 million years of the topology to reduce the influence of taxonomic inaccuracy on the estimation of recent diversification [42]. Pruning a range of times or nodes from a topology to assess how taxonomic inaccuracies influence deviations from null expectations would provide an even more robust method to account for taxonomic inaccuracies. If Heroine cichlids underwent an explosive phase of lineage diversification when they colonized Central America, this pattern should be detectable with analyses that account for uncertainty in the number of extant lineages.

We combined phylogenetics, ancestral state reconstruction, and simulations to assess the temporal patterns of CA Heroine diversification. We first reconstructed the phylogeny of CA Heroines and subsequently used likelihood reconstruction to determine the basal node from which to estimate patterns of diversification. Then, we used simulations and the truncation of nodes to examine Heroine deviations from a null distribution of diversification expected under a pure-birth, constant rate model. We combined these analyses to examine if patterns of Heroine diversification were consistent with rapid lineage accumulation coincident with their invasion of Central America.

Results

Phylogeny Reconstruction

The phylogenetic relationships recovered with the 17 new cytochrome b sequences (Table 1) analyzed in a Bayesian framework do not differ greatly from previous analyses using the cytochrome b gene [43, 44]. The clade of three Greater Antillean Heroines and the South American Australoheros, that in some phylogenetic analyses [45–47] have been recovered as nested within the CA Heroines, fell phylogenetically just outside of the CA Heroine clade here (Figure 1). These groups would not be considered as primarily diversifying in Central America so their phylogenetic position inferred here was also convenient for our analyses. None of the previously sequenced species that we re-sequenced here to better estimate branch-lengths exhibited novel relationships.

Table 1 Species sequenced for cytochrome b for this study.
Full size table
Figure 1
figure 1

Chronogram of CA Heroine diversification. Likelihood ancestral areas are reconstructed at nodes as either Central American (white) or South American + Greater Antilles (black). The tips as well as many of the nodes in the phylogeny are only one color and therefore are reconstructed with virtually 100% probability as one state. The pie diagrams that exhibit both colors represent ambiguous likelihood reconstructions of the area at that node and are depicted at larger sizes. Posterior probabilities of nodes are shown on the branch preceding the nodes and are indicated with an * if there is 100% Bayesian support for the node. Other numbers behind the nodes represent the percentage that that node was recovered among topologies saved in the Bayesian analysis. Only support values above 50% are depicted. The node calibrated with divergence of 7.5 million years before present (mybp) around the Punta del Morro is shown with an X. A temporal scale running from 15.0 mybp to the recent is shown below the chronogram. An image of a typical Central American Heroine cichlid, Herichthys cyanoguttatus, is shown nested within the phylogeny.

Full size image

For species that were not previously sequenced but fell within the 90 included CA Heroine species, we recovered several interesting relationships. Thorichthys socolofi was found to be sister to T. aureus, and T. affinis was recovered as sister to T. meeki. Interestingly, the species Archocentrus spinosissimus was placed as sister to Rocio octofasciata although the length of the branch separating these two species suggests they are highly divergent. Parachromis friedrichstahlii was recovered as sister to the clade containing Parachromis motaguensis and Parachromis loiselli. The two species Cryptoheros cutteri and C. chetumalensis that were recently taxonomically split out of Cryptoheros spilurus [12] formed a monophyletic group with C. cutteri being the most phylogenetically distinct.

Chronogram

The root of the CA Heroine clade examined was estimated to be 16.2 million years before present (mybp), but there are several CA Heroine clades that appear to have diversified within a relatively recent timeframe (< 3 mybp). The Amphilophus citrenellus + Am. labiatus + Am. hogaboomorum clade forms a polytomy that likely includes a substantial number of species [31] that diverged very recently. The newly erected species Cryptoheros chetumalensis is also highly genetically similar to its sister C. spilurus. Thorichthys meeki and T. affinis as well as Vieja melanura and V. synspila are not genetically very distinct. Likewise, Vieja hartwegi + V. bifasciata + V. breidohri show very little sequence divergence. The sister clade to the polymorphic cichlid Herichthys minckleyi that includes H. cyanoguttatus, H. deppi, H. carpintis, and H. tamasopoensis also diverged within the last 3 million years.

Ancestral Area Reconstruction

The likelihood reconstruction of ancestral areas indicates that there is greater than 95% probability that the ancestral lineage leading to the basal node in Figure 1 began diversifying in Central America. The estimated Mk1 rate parameter was 0.007 indicating a generally low rate of transition between Central America and either the Greater Antilles or South America. Because the three species of Greater Antilles cichlids fell outside of this clade it suggests they did not colonize this region by first occupying Central America. Our ancestral reconstruction also supports two instances of the CA Heroines re-colonizing and experiencing limited diversification in South America. The Caquetaia clade of three species as well as the clade composed of Cichlasoma festae + C. atromaculatum + C. umbrifera clade are both reconstructed here as re-colonizing South America. Retention of all of these species in the LTT analysis should not be problematic because analyses that pruned these species (results not shown) did not differ substantially from those we present. Also, these South American species represented relatively few species, their speciation times did not seem skewed in any particular direction, and there was some ambiguity (Figure 1) about where (i.e. South America vs. Central America) the speciation events at particular ancestral nodes took place.

CA Heroine Lineages Through Time

The lineage-through-time (LTT) plot provides no obvious excess of lineages early in the history of the Heroine cichlid radiation (Figure 2). The simulation of 10000 lineages using a pure-birth model to create a 95% CI for the expectation of diversification showed that during their entire diversification the accumulation of lineages in the CA Heroine clade fell within this null expectation. The only component of the Heroine radiation that might be skewed towards faster than expected diversification contains lineages originating within the last five million years. The virtual linear accumulation of species through time (Figure 2) is highly suggestive of a pure birth process governing diversification in CA Heroines.

Figure 2
figure 2

The lineage-through-time (LTT) plot of CA Heroine diversification. The black dots represent actual numbers of Heroine lineages estimated at a given time frame from the reconstructed phylogeny. The grey lines form an ellipse of simulated pure-birth phylogenies of 90 species used to compare to the CA Heroines. The dotted lines represent the 95% confidence interval of the number of lineages expected from the simulated pure-birth phylogenies. The CA Heroine LTT lies within the 95% null distribution expected for a radiation diversifying via a pure-birth process.

Full size image

Based on the values of γ, the inference that there is a burst of diversification early in the clade of Heroine cichlids also depends upon how complete our taxon sampling of lineages is (Figure 3). If our phylogeny contains all of the species in Central America and all un-sampled lineages are merely synonyms of the 90 species currently sampled, then the chronogram of CA Heroines would exhibit a significant deviation from a pure-birth process. If this were true, CA Heroines might exhibit a slight burst of diversification early in the clade's history. However, this is unlikely, and if there are in fact 122 species of Heroine cichlids in this clade as current taxonomy suggests, this group does not show a burst of diversification early during its radiation.

Figure 3
figure 3

Species number and γ statistic. We used null distributions to test if γ exceeded the value of -1.645 (the critical value for α = 0.05) with a range of "true" total numbers of CA Heroine species in the clade. We examined γ with 90 species, the number of taxa sampled in the phylogeny, to 120 species. Increasing the number of species resulted in lower and lower probability of there being a burst early in the phylogeny. We therefore could not reject the hypothesis that CA Heroine cichlids exhibited a pure-birth model of constant lineage diversification if there are 122 species as current taxonomy suggests.

Full size image

The truncation of nodes (Figure 4) indicates there is little support for a burst of diversification especially as one proceeds back into the CA Heroine phylogeny. Sampling of lineages should become more complete as one moves towards the root of the phylogeny, and therefore, the results of this truncation should test how robust our results are. If incomplete taxonomic sampling at the tips were skewing our inferences away from detection of a burst of diversification, we would expect that the γ values would become, or remain, more significant as nodes were truncated. However, we recovered the opposite. After nodes at an age of approximately 3.5 mybp were removed, the remaining γ values were clearly not above the critical threshold value of -1.645 that statistically marks the 95% expectation of a constant diversification rate. At 4.0 mybp and deeper in the phylogeny, the fact that γ did not exceed this critical value indicates there was not an early burst of diversification in CA Heroines. As nodes were truncated from our taxonomically incomplete chronogram, the γ values approached the expectation under a constant rate, pure-birth model of diversification. Both our simulations accounting for our incomplete phylogenetic sampling of the named Heroine species in Central America and pruning the topology back in time are concordant in suggesting there was no early burst of diversification in CA Heroine cichlids.

Figure 4
figure 4

Node truncation and stability of γ. Nodes were truncated from the present to the root of the CA Heroine phylogeny in order to assess the stability of γ using our empirically estimated 90 species phylogeny. Because lineage sampling should become more complete towards the root of the phylogeny, truncation of nodes closer to the present should reduce the influence of incomplete lineage sampling on inferences made from γ. Node removal and γ recalculation is depicted temporally based on the last removed node's time-calibration from the CA Heroine chronogram. Importantly, once nodes from the present to 3.5 mybp are removed, γ is clearly not significant in our empirical phylogeny. Therefore, analyses of only the deeper nodes in the CA Heroine phylogeny cannot reject a pattern of pure-birth lineage diversification.

Full size image

The expected rate of lineage accumulation under a constant-rate model of diversification cannot be rejected for the Heroine cichlids. Additionally, the model fitting approach failed to favor any of the rate variable models examined over a pure-birth model of lineage diversification. Regardless of the expected number of terminal taxa (90-122) in the clade, a pure-birth model (no extinction) could not be rejected for CA Heroine cichlids.

Discussion and Conclusion

There was no dramatic burst of speciation as Heroine cichlids colonized Central America. The phylogenetic inclusion of several species further resolved the phylogeny of the entire clade, but did little to change the overall topology of the tree recovered in previous studies. The temporal estimates of the root node of Heroine cichlids as being close to 16 mybp is also consistent with most other molecular clock estimates derived from mitochondrial DNA markers for these fishes [44, 48]. These studies, largely based on cytochrome b suggest an age of between 15 and 22 mybp for Heroine diversification. However, several recent studies indicate that Heroines and other cichlids groups are much older than previously thought [40, 49, 50]. These studies suggest that the reciprocally monophyletic diversification in the Neotropics and Africa is generally consistent with a Gondwanan split and divergence time estimates for each continental radiation of around 65-85 mybp. If this is true, Heroine cichlids could have begun diversifying in Central America almost 30 mybp [50]. Regardless, if our dates are close to realistic, it suggests that there are several clades in the CA Heroines that have likely diverged relatively recently (< 3 mybp). Nevertheless, our analyses do not provide substantial support for an increased rate of diversification at the base of the CA Heroine phylogeny.

This phylogenetic analysis is the most thoroughly sampled species-level analysis of Heroine cichlid relationships. However, it is unclear how incomplete the taxonomic sampling of the phylogeny is currently. Future studies of the alpha taxonomy of CA Heroines could substantially increase the number of named species in this group. There remain regions of Central America such as the flooded forests of the Moskitia in Honduras and Nicaragua where the diversity of freshwater cichlids has not been extensively documented [23]. Also, substantial numbers of CA Heroine lineages could be described by taxonomically splitting currently recognized species [12]. For instance, the species 'Cichlasoma' uropthalmus that is represented in our phylogeny by a single lineage has 11 currently recognized species/subspecies [51]. If they form a recently evolved monophyletic group as is likely, the addition of these species to our phylogeny would further decrease support for a burst of diversification at the base of the CA Heroine radiation. The number of cichlid species in the crater lakes of Lake Nicaragua is also debated but the speciation times for these groups are clearly recent as well [31]. A complete tally of CA Heroines will undoubtedly recognize more lineages and generally increase the number of recent nodes towards the tips of the phylogeny rather than at the base of the radiation. Additional Heroine species descriptions will not skew diversification patterns toward detection of a burst of diversification at the base of this clade.

If there are in fact 122 species of Heroine cichlids in this clade, this group's diversification does not show a significant deviation from a pure-birth process (Figure 3). However, the inference that there could have been a burst of diversification in Heroine cichlids depends in part on the completeness of our taxon sampling. If our phylogeny contains all of the species in Central America and all un-sampled lineages are merely synonyms of the 90 species currently sampled, then the phylogeny of Central American cichlids would exhibit a significant deviation from a pure-birth process. However, because current taxonomy suggests there are 122 evolutionarily independent lineages, Heroine cichlids probably did not exhibit a burst of diversification concordant with their invasion of Central America. There is also no empirical support for a substantial amount of extinction (i.e. birth-death model) or temporal change (rate variable model) during the diversification of CA Heroine cichlids. The comparison of the LTT plot to null distributions and truncation of nodes provide little support for Heroine diversification deviating significantly from a pure-birth process. In fact, node truncation suggests that as one proceeds back in time, the historical pattern of CA Heroine diversification becomes less and less compatible with an early burst of diversification.

There remain a few caveats to this study. First, the use of a mitochondrial marker like cytochrome b could show saturation and thus underestimate the branch lengths connecting deeper nodes in the tree [52]. However, this would only bias analyses towards detection of a burst of speciation at the base of the radiation because of underestimation of older branch lengths. Hybridization could also mislead the inferences we are making with respect to CA Heroine phylogeny. However, hybridization is likely more important during the first few million years of diversification within clades of cichlids [53]. Therefore, the possibility of recent hybridization should not obscure our inferences of a lack of rapid lineage diversification in Heroine cichlid lineages that diverged around 16 mybp or even earlier. Analyses of more genes will undoubtedly provide an increasingly robust view of the phylogenetic relationships among this diverse clade. But, we have no reason to believe that the marker used here provides an exceptionally biased view of the diversification history of CA Heroines.

This study could call into question the general importance of ecological opportunity to cichlid diversification. However, one way that hypotheses aimed at elucidating the importance of ecological release to diversification could be refined is to more explicitly incorporate the history of these radiations into their particular environmental frameworks. There are several reasons the ecology of the African Great Lakes might better facilitate obvious bursts of diversification compared to other freshwater systems cichlids inhabit. Unlike rivers, the African Great Lakes contain archipelagos of small rocky islands [3] that favor rapid isolation and divergence. Additionally, the cichlid radiations in the African Great Lakes diversified in an exceptionally sympatric context. The radiation of CA Heroine cichlids likely involved a much more allopatric mode of diversification in the numerous river basins that dissect Central America. Lake Tanganyika is also likely well over 10 million years old [54] and could be as old as 20 million years [49]. Although Lake Victoria is less than a million years old [54] and Lake Malawi is likely close to 3 million years old [40, 50], most of the lake and riverine habitats in Central America are young and geologically dynamic [55, 56] as compared to the African Great Lakes. The extensive bathymetry of the African Great Lakes also create stratified light environments that appear to influence sexual selection and rapid reproductive isolation among lineages [53]. The exceptional number of herbivores and planktivores in the African Great Lakes [3, 8] likewise could indicate there are ecological opportunities available in these habitats that are largely absent from other aquatic systems. Perhaps it is the particular types of ecological conditions and their stability over time that facilitated the explosive diversification of cichlid lineages inhabiting the East African Rift Lakes [9].

Many models and empirical studies suggest that adaptive radiations should be characterized by a burst of diversification early in their history [25]. We found no evidence that the CA Heroine cichlids exhibit a burst early in their history. However, we cannot exclude the possibility that CA Heroines are indeed undergoing rapid diversification and are still in the "early" stage of their radiation where it is impossible to detect a slowdown in diversification at this time because it has not yet occurred. If density dependence among members of a clade governs the rate of diversification [57], CA Heroines could also simply be far from the carrying capacity for the number of cichlid lineages that can co-exist. Currently, the maximum number of CA Heroine species that occur sympatrically is approximately 12 species [4]. This is far less than the 100 or more cichlid species that can occur sympatrically in some habitats in Lake Malawi [58]. The dynamic nature of the largely riverine and geologically active Central American landscape relative to the East African Great Lakes could have enforced a relatively slow fuse on the explosive diversification rate of CA Heroines.

Furthermore, although the rate of diversification in some East African Rift Lakes is clearly high [54, 59–64], only diversification patterns in the oldest of the lakes, Lake Tanganyika, has been tested extensively in a LTT framework. Somewhat counter to what we find here for CA Heroines, diversification rate does appear to have slowed slightly towards the present in Lake Tanganyika. However, this slowdown was not as marked as one might expect and it is clear that the diversification rate is not especially rapid for the cichlids inhabiting this lake [64]. However, the diversification rates in Lake Victoria and Lake Malawi are unquestionably fairly rapid [64]. If CA Heroines are in fact only 16 million years old, diversification in this group of over 100 species has been rapid compared to many fish radiations [65, 66]. However, if this clade is as old as 30 million years as some calibrations suggest [40, 49, 50], the diversification rate is likely to be more in line with many other fish groups. With multiple genes and multiple temporal calibrations, whether CA Heroines exhibit a relatively rapid diversification rate per million years could be tested. Additionally, ecological divergence in CA Heroines is substantial [4, 15, 17] and the rate of adaptive phenotypic and ecological divergence in this radiation could well be extraordinary. General processes, both intrinsic and extrinsic, that are responsible for generating diversity in adaptively diverging clades should come to light as radiations like the CA Heroine cichlids are examined in more explicit evolutionary and ecological detail.

Methods

DNA Sequencing

Gene sequence for the cytochrome b gene (1137 bp) for 17 Heroine species (see Additional file 1) were combined with sequence for numerous species previously analyzed [43, 44]. All species sequenced in this study were collected from the wild except for Archocentrus spinossimus that was purchased commercially. Collection localities are available in Table 1. All new sequences were submitted to Genbank [Genbank: HM193438-HM193454]. Because we were interested in efficiently resolving a bifurcating topology and estimating branch lengths only one complete sequence per currently named species was utilized in our analyses.

For sequencing, total genomic DNA was isolated from axial muscle using Puregene© extraction. A 1 μl aliquot of this solution was used to provide a DNA template for polymerase chain reaction (PCR). The entire cytochrome b gene was PCR amplified using primers in Hulsey et al. [43]. Amplifications were carried out using standardized PCR protocols. The PCR volume was 25 ml (18 ml H2O, 2.75 ml MgCl2 PCR buffer, 1.25 ml MgCl2, 2.0 ml dNTPs (10 mM), 1.25 ml of each primer (10 mM), 0.25 ml Taq and 0.5 ml DNA; approx. 15-20 ng). Thermal cycling conditions consisted of an initial denaturation step of 94°C (2.0 min), 54°C (1.0 min) and 72°C (1.5 min). A final incubation of 72°C for 4 min was added to ensure complete extension of amplified products. Subsequently, the 1.4 kb PCR products were separated from unincorporated primers and dNTPs using electrophoresis in agarose gels run in Tris-acetate buffer (pH 7.8). Ethidium bromide (1.5 mg/ml) was added to the gels for visualization. Positively amplified DNA was then purified using an enzymatic combination of 1 μl of Exonuclease I and 1 μl shrimp alkaline phosphatase per 10 μl of PCR product. Complete gene sequences were assembled from individual sequencing reactions using the program Sequencher version 4.1 (Gene Codes, Ann Arbor, MI).

Phylogeny Reconstruction

A combined total of 111 species' sequences were examined in the phylogenetic analysis (Additional file 1). Prior to the analyses, it was unclear exactly which species should be included in the CA Heroine clade and therefore a large number of potential outgroups were included. The putative outgroups utilized that are all from South America were Acarichthys heckelii, Aequidens coeruleopunctatus, Cichla monoculus, Cleithracara maronii, Heros appendiculatus, Hoplarchus psittacus, Hypselecara coryphaenoides, Mesonauta festivus, M. insignis, Pterophyllum scalare, Symphysodon aequifasciata, and Uaru amphiacanthoides. Their Genbank accession numbers are included (Additional file 1). For the Bayesian analyses, sequences were aligned using Clustal X [67] and codon positions were defined using MacClade 4.0 [68]. ModelTest 3.06 [69] was used to identify the best model of molecular evolution for each codon site. A model of GTR + I + gamma was found to be the best model for all three positions. The Bayesian analyses were executed to find approximations of the maximum likelihood tree using MrBayes 3.0 [70]. The analyses treated the transition-transversion matrices, number of invariant sites, and gamma shape parameters as unlinked or independent for each codon site. Flat prior probability distribution for all parameters were assumed before analysis. We ran three separate Bayesian analyses for 5,000,000 generations with four Markov chains in each run. We sampled trees from the Markov Chain Monte Carlo (MCMC) search algorithm every 1000 generations. At the end of each analysis, the log-likelihood scores were plotted against generation time to identify the point at which log likelihood values reached a stable equilibrium. In all three, the equilibrium appeared to be reached at approximately 100,000 generations, and therefore, sample points prior to generation 100,000 in each run were discarded as "burn-in" samples. The remaining samples from all runs combined were used to produce a majority rule consensus tree in PAUP* 4.0b10 [71]. The percentage of trees that recovered a particular clade (the clade's posterior probability) was depicted on the single best likelihood tree topology found during the Bayesian analyses.

Chronogram

To generate a time-calibrated chronogram of CA Heroine diversification, we utilized penalized-likelihood implemented in the program r8s [72]. Optimal smoothing parameters that compensate for rate heterogeneity were estimated using cross validation implemented in r8s. Using the optimal rate smoothing parameter of 0.001 derived from the cross-validation, r8s generated a time-calibrated ultrametric tree that was utilized in the subsequent analyses.

Although it is not necessary to analyze LTT plots using absolute rates of time, we chose to calibrate the topology with what is likely a temporally realistic geologic calibration. To calibrate the topology we used the formation of the Punta del Morro an extension of the Mexican Neovolcanic Plateau to the Gulf of Mexico. This boundary was thought to have formed between 5 and 10 million years ago [73]. We used the "set age" command in r8s to fix the age of the divergence for the two cichlid sister-clades that spanned the formation of this boundary at 7.5 million years, the average of geologic estimates for the Punta del Morro formation. In the Heroine cichlids, only the Herichthys species are located north of this region [43]. We therefore used the node separating a representative of these species, Herichthys cyanoguttatus, and the species Vieja fenestrata, a member of the sister group to Herichthys, as the node calibrated by the formation of the Punta del Morro.

Ancestral Area Reconstruction

To determine the ancestral node in the Heroine phylogeny from which to measure patterns of speciation, we reconstructed the ancestral areas of nodes on the CA Heroine chronogram generated above. All species present in mainland Central America were coded as 1 and all species that occur primarily in South America or in the Greater Antilles were coded as 0. Using the program Mesquite [74], likelihood ancestral state reconstruction of presence in these two areas was estimated. The Markov k-state 1 parameter model (Mk1) was implemented to reconstruct the likelihood of ancestral states at nodes [75]. This type of optimization assumes equal probabilities of transitions and therefore estimates a single parameter for transitions between Central America and other regions. It is important to note that our estimate of the Central American ancestral node is likely biased towards reconstructing a relatively deep node as mostly Central American as there are several hundred South American cichlid outgroups not included in our estimate of the ancestral area. However, most of these outgroups are fairly distantly related to the Central American Heroines, and therefore, they should have limited influence on ancestral area estimation. Ancestral state reconstruction is always sensitive to groups not included in the analysis due to processes such as extinction and exclusion of species [75]. However, the likelihood that this ancestral area would be reconstructed as Central American would never be negligible as the three nodes closer to the present all subtend primarily Central American groups. Furthermore, all phylogenetic studies to date have recovered this group of CA Heroines as largely monophyletic [47]. We depicted the likelihood of the ancestral states we estimated using pie diagrams showing the estimated probabilities that speciation at each reconstructed node on the chronogram took place in either Central America or outside of Central America.

CA Heroine Lineages Through Time

If CA Heroines underwent an explosive bout of diversification following their colonization of mainland Central America, this pattern should be evidenced by deviations from a constant rate pattern of cladogenesis. Several approaches were used to explore diversification rate variation in the CA Heroine chronogram. First, we used Pybus and Harvey's [35] constant rate (CR) test, which examines the accumulation of lineages through time using the test statistic gamma (γ). Under a pure-birth model of diversification, γ follows a standard normal distribution. Thus, values of γ < -1.645 (the critical value for a one tailed test at α = 0.05) indicate a deviation from a pure-birth model where diversification decreases towards the present as one would expect if CA Heroines underwent a burst of diversification early in their history.

However, the CR test assumes complete taxon sampling. Based on species names available in Fishbase [10] and several recent taxonomic revision [11–13], we included all but 32 of the currently 122 named species in the CA Heroine radiation in our analysis (Additional file 2). To compensate for this incomplete sampling, we generated random topologies for the total number of taxa thought to be extant in the clade and then pruned them to the number of species empirically sampled. We examined γ over a range of expected terminal taxa (i.e., species richness). We used species richness values between 90, which assumes our current tree contains all species, to 122 species, the number current taxonomy suggests is in the clade. This approach provided us with a range of lineage values to examine the sensitivity of our statistical inferences to taxonomy. Our null distributions of γ were obtained using 10000 simulated pure-birth trees with taxon sampling generated with the program Phylogen [76].

When examining variation in diversification rate, incomplete taxon sampling can also increase type I error rates because it effectively results in nodes near the tips of the tree being pruned [77]. Not including the other 32 named species of CA Heroines in our phylogeny could result in erroneously finding an apparent high rate of diversification early in the clade's history. To help alleviate this problem, we also examined the values of the γ statistic as our empirical tree containing 90 species was truncated node by node serially back in time. As the tree was truncated, lineage sampling should become increasingly more complete thereby reducing error in inferences based on the value of γ. To examine the resulting changes in the γ statistic as nodes were truncated, we graphed γ, recalculated for the number of lineages remaining in the phylogeny, versus the time-calibrated estimate of the most recent node removed. As one moved towards the root of the CA Heroine phylogeny, γ would be expected to become more negative if an under-sampling of lineages was obfuscating an early burst of diversification in CA Heroines.

Because there was some ambiguity in our ancestral state reconstructions and relatively low support for some of the deeper nodes in the topology, we also re-examined all of the above analyses in the two major subsections of the CA Heroine clade. This allowed us to determine if our results were heavily contingent upon inferences concerning the deepest nodes. Our results from these analyses of subsets of the phylogeny were consistent with those recovered for the entire topology (results not shown).

If a pure-birth model was the best fit to the lineage accumulation of CA Heroines through time, it would suggest CA Heroines did not experience a burst of diversification when they colonized Central America. By comparing models that incorporate additional rate parameters of lineage accumulation, we determined the best model for the empirically observed pattern of CA Heroine diversification rate variation through time. We fit two candidate rate-constant models, pure-birth (yule process) and birth-death (birth and extinction), and three rate variable models (density dependent exponential, density dependent logistic, and Yule two-rate) to the vector of branching times obtained from the CA Heroine chronogram. These models test several types of alternative patterns of speciation and extinction through time [38]. We calculated the likelihood of each model given the data as implemented in the R-package LASER (version 2.2) [37]. Subsequently, we examined the Akaike Information Criterion (AIC) to evaluate which was the best model given the data. We chose the best model based on the distribution of differences between the AIC scores of all of the rate-constant and rate-variable models using a critical difference in AIC scores of α = 0.05 [57]. These fits were derived from comparisons to 10000 simulated pure-birth trees with taxon sampling generated by the program Phylogen [76].

References

  1. Patterson C: Bony fishes. Major Features of Vertebrate Evolution. Edited by: D.R. Prothero S, R.M. 1994, Knoxville, TN: University of Tennessee Paleontological Society, 57-84.

    Google Scholar 

  2. Greenwood PH: Explosive speciation in African lakes. Proceedings of the Royal Institute of Great Britain. 1964, 40: 256-269.

    Google Scholar 

  3. Fryer G, Iles TD: The cichlid fishes of the Great Lakes of Africa. 1972, Edinburgh, UK: Oliver and Boyd

    Google Scholar 

  4. Winemiller KO, Kelso-Winemiller LC, Brenkert AL: Ecomorphological diversification and convergence in fluvial cichlid fishes. Environmental Biology of Fishes. 1995, 44: 235-261. 10.1007/BF00005919.

    Article  Google Scholar 

  5. Liem KF: Evolutionary strategies and morphological innovations - cichlid pharyngeal jaws. Systematic Zoology. 1973, 22: 425-441. 10.2307/2412950.

    Article  Google Scholar 

  6. Hulsey CD, García de León FJ, Rodiles-Hernandez R: Micro- and macroevolutionary decoupling of cichlid jaws: A test of Liem's key innovation hypothesis. Evolution. 2006, 60: 2096-2109.

    Article  CAS  PubMed  Google Scholar 

  7. Salzburger W, Mack T, Verheyen E, Meyer A: Out of Tanganyika: Genesis, explosive speciation, key-innovations and phylogeography of the haplochromine cichlid fishes. BMC Evolutionary Biology. 2005, 5 (1): 17-10.1186/1471-2148-5-17.

    Article  PubMed Central  PubMed  Google Scholar 

  8. Kornfield I, Smith PF: African cichlid fishes: Model systems for evolutionary biology. Annual Review of Ecology and Systematics. 2000, 31: 163-10.1146/annurev.ecolsys.31.1.163.

    Article  Google Scholar 

  9. Seehausen O: Evolution and ecological theory - Chance, historical contingency and ecological determinism jointly determine the rate of adaptive radiation. Heredity. 2007, 99: 361-363. 10.1038/sj.hdy.6801047.

    Article  CAS  PubMed  Google Scholar 

  10. FishBase. [http://www.fishbase.org]

  11. Stauffer JR, McKaye KR: Descriptions of three new species of cichlid fishes (Teleostei: Cichlidae) from Lake Xiloá, Nicaragua. 2002, Managua, Nicaragua: Dirección de Investigación de la Universidad Centroamericana, 1-18.

    Google Scholar 

  12. Schmitter-Soto JJ: Phylogeny of species formerly assigned to the genus Archocentrus (Perciformes: Cichlidae). Zootaxa. 2007, 1-50.

    Google Scholar 

  13. Stauffer JR, McCrary JK, Black KE: Three new species of cichlid fish (Teleostei: Cichlidae) in Lake Apoyo, Nicaragua. Proceedings of the Biological Society of Washington. 2008, 121: 117-129. 10.2988/06-37.1.

    Article  Google Scholar 

  14. Eaton TH: An adaptive series of protractile jaws in cichlid fishes. Journal of Morphology. 1943, 72: 183-190. 10.1002/jmor.1050720107.

    Article  Google Scholar 

  15. Hulsey CD, García de León FJ: Cichlid jaw mechanics: linking morphology to feeding specialization. Functional Ecology. 2005, 19: 487-494. 10.1111/j.1365-2435.2005.00987.x.

    Article  Google Scholar 

  16. Higham TE, Hulsey CD, Rican O, Carroll AM: Feeding with speed: prey capture evolution in cichilds. Journal of Evolutionary Biology. 2007, 20: 70-78. 10.1111/j.1420-9101.2006.01227.x.

    Article  CAS  PubMed  Google Scholar 

  17. Hulsey CD, Roberts RJ, Lin ASP, Guldberg R, Streelman JT: Convergence in a mechanically complex phenotype: Detecting structural adaptations for crushing in cichlid fish. Evolution. 2008, 62: 1587-1599. 10.1111/j.1558-5646.2008.00384.x.

    Article  PubMed  Google Scholar 

  18. Hulsey CD, Hollingsworth PR, Holzman R: Co-evolution of the premaxilla and jaw protrusion in cichlid fishes (Heroine: Cichlidae). Biological Journal of the Linnean Society. 2010, 100: 619-629. 10.1111/j.1095-8312.2010.01468.x.

    Article  Google Scholar 

  19. Farias IP, Orti G, Sampaio I, Schneider H, Meyer A: The cytochrome b gene as a phylogenetic marker: The limits of resolution for analyzing relationships among cichlid fishes. Journal of Molecular Evolution. 2001, 53: 89-103.

    Article  CAS  PubMed  Google Scholar 

  20. Malabarba MC, Zuleta O, Del Papa C: Proterocara argentina, a new fossil cichlid from the Lumbrera Formation, Eocene of Argentina. Journal of Vertebrate Paleontology. 2006, 26: 267-275. 10.1671/0272-4634(2006)26[267:PAANFC]2.0.CO;2.

    Article  Google Scholar 

  21. Miller RR: Geographical distribution of Central American freshwater fishes. Copeia. 1966, 773-802. 10.2307/1441406.

    Google Scholar 

  22. Myers GS: Derivation of freshwater fish fauna of Central America. Copeia. 1966, 766-773. 10.2307/1441405.

    Google Scholar 

  23. Hulsey CD, López-Fernández H: Historical biogeography of the fishes of Nuclear Central America. Neotropical Fish Biologeography. Edited by: Alber J, Reis RE. 2009, Berkeley, CA: University of California Press,

    Google Scholar 

  24. Schluter D: The ecology of adaptive radiation. 2000, New York, New York: Oxford University Press

    Google Scholar 

  25. Gavrilets S, Losos JB: Adaptive Radiation: Contrasting Theory with Data. Science. 2009, 323: 732-737. 10.1126/science.1157966.

    Article  CAS  PubMed  Google Scholar 

  26. Kornfield IL, Koehn RK: Genetic-variaion and speciation in New World cichlids. Evolution. 1975, 29: 427-437. 10.2307/2407255.

    Article  Google Scholar 

  27. Meyer A: Ecological and evolutionary consequences of the trophic polymorphism in Cichlasoma citrinellum (Pisces, Cichlidae). Biological Journal of the Linnean Society. 1990, 39: 279-299. 10.1111/j.1095-8312.1990.tb00517.x.

    Article  Google Scholar 

  28. Hulsey CD, Hendrickson DA, García de León FJ: Trophic morphology, feeding performance and prey use in the polymorphic fish Herichthys minckleyi. Evolutionary Ecology Research. 2005, 7: 303-324.

    Google Scholar 

  29. Barluenga M, Stolting KN, Salzburger W, Muschick M, Meyer A: Sympatric speciation in Nicaraguan crater lake cichlid fish. Nature. 2006, 439: 719-723. 10.1038/nature04325.

    Article  CAS  PubMed  Google Scholar 

  30. Gavrilets S, Vose A, Barluenga M, Salzburger W, Meyer A: Case studies and mathematical models of ecological speciation. 1. Cichlids in a crater lake. Molecular Ecology. 2007, 16: 2893-2909. 10.1111/j.1365-294X.2007.03305.x.

    Article  PubMed  Google Scholar 

  31. Elmer KR, Kusche H, Lehtonen TK, Meyer A: Local variation and parallel evolution: morphological and genetic diversity across a species complex of neotropical crater lake cichlid fishes. Philosophical Transactions of the Royal Society Series B. 2010, 365: 1763-1782. 10.1098/rstb.2009.0271.

    Article  Google Scholar 

  32. Kozak KH, Weisrock DW, Larson A: Rapid lineage accumulation in a non-adaptive radiation: phylogenetic analysis of diversification rates in eastern North American woodland salamanders (Plethodontidae: Plethodon). Proceedings of the Royal Society B-Biological Sciences. 2006, 273: 539-546. 10.1098/rspb.2005.3326.

    Article  PubMed Central  CAS  Google Scholar 

  33. Weir JT: Divergent timing and patterns of species accumulation in lowland and highland neotropical birds. Evolution. 2006, 60: 842-855.

    Article  PubMed  Google Scholar 

  34. Nee S: Inferring speciation rates from phylogenies. Evolution. 2001, 55: 661-668. 10.1554/0014-3820(2001)055[0661:ISRFP]2.0.CO;2.

    Article  CAS  PubMed  Google Scholar 

  35. Pybus OG, Harvey PH: Testing macro-evolutionary models using incomplete molecular phylogenies. Proceedings of the Royal Society of London Series B-Biological Sciences. 2000, 267: 2267-2272. 10.1098/rspb.2000.1278.

    Article  CAS  Google Scholar 

  36. Nee S: Birth-death models in macroevolution. Annual Review of Ecology Evolution and Systematics. 2006, 37: 1-17. 10.1146/annurev.ecolsys.37.091305.110035.

    Article  Google Scholar 

  37. Rabosky DL: LASER: A Maximum Likelihood Toolkit for Detecting Temporal Shifts in Diversification Rates From Molecular Phylogenies. Evolutionary Bioinformatics. 2006, 2: 247-250.

    Google Scholar 

  38. Rabosky DL: Likelihood methods for detecting temporal shifts in diversification rates. Evolution. 2006, 60: 1152-1164.

    Article  PubMed  Google Scholar 

  39. Avise JC, Walker D: Pleistocene phylogeographic effects on avian populations and the speciation process. Proceedings of the Royal Society of London Series B-Biological Sciences. 1988, 265: 457-1463. 10.1098/rspb.1998.0317.

    Article  Google Scholar 

  40. Genner MJ, Seehausen O, Lunt DH, Joyce DA, Shaw PW, Carvalho GR, Turner GF: Age of cichlids: New dates for ancient lake fish radiations. Molecular Biology and Evolution. 2007, 24: 1269-1282. 10.1093/molbev/msm050.

    Article  CAS  PubMed  Google Scholar 

  41. Isaac NJB, Mallet J, Mace GM: Taxonomic inflation: its influence on macroecology and conservation. Trends in Ecology & Evolution. 2004, 19: 464-469.

    Article  Google Scholar 

  42. Phillimore AB, Price TD: Density-dependent cladogenesis in birds. PLOS Biology. 2008, 6: 483-489. 10.1371/journal.pbio.0060071.

    Article  CAS  Google Scholar 

  43. Hulsey CD, García de León FJ, Johnson YS, Hendrickson DA, Near TJ: Temporal diversification of Mesoamerican cichlid fishes across a major biogeographic boundary. Molecular Phylogenetics and Evolution. 2004, 31: 754-764. 10.1016/j.ympev.2003.08.024.

    Article  CAS  Google Scholar 

  44. Concheiro-Pérez GAC, Rican O, Orti G, Bermingham E, Doadrio I, Zardoya R: Phylogeny and biogeography of 91 species of heroine cichlids (Teleostei: Cichlidae) based on sequences of the cytochrome b gene. Molecular Phylogenetics and Evolution. 2007, 43: 91-110. 10.1016/j.ympev.2006.08.012.

    Article  Google Scholar 

  45. Chakrabarty P: Systematics and historical biogeography of Greater Antillean Cichlidae. Molecular Phylogenetics and Evolution. 2006, 39: 619-627. 10.1016/j.ympev.2006.01.014.

    Article  PubMed  Google Scholar 

  46. Rican O, Zardoya R, Doadrio I: Phylogenetic relationships of Middle American cichlids (Cichlidae, Heroini) based on combined evidence from nuclear genes, mtDNA, and morphology. Molecular Phylogenetics and Evolution. 2008, 49: 941-957. 10.1016/j.ympev.2008.07.022.

    Article  CAS  PubMed  Google Scholar 

  47. López-Fernández H, Winemiller KO, Honeycutt RL: Multilocus phylogeny and rapid radiations in Neotropical cichlid fishes (Perciformes: Cichlidae: Cichlinae). Molecular Phylogenetics and Evolution. 2010, 55: 1070-1086. 10.1016/j.ympev.2010.02.020.

    Article  PubMed  Google Scholar 

  48. Martin AP, Bermingham E: Systematics and evolution of lower Central American cichlids inferred from analysis of cytochrome b gene sequences. Molecular Phylogenetics and Evolution. 1998, 9: 192-203. 10.1006/mpev.1997.0461.

    Article  CAS  PubMed  Google Scholar 

  49. Schwarzer J, Misof B, Tautz D, Schliewen UK: The root of the East African cichlid radiations. BMC Evolutionary Biology. 2009, 9: 186-10.1186/1471-2148-9-186.

    Article  PubMed Central  PubMed  Google Scholar 

  50. Hulsey CD, Mims MC, Parnell NF, Streelman JT: Comparative rates of lower jaw diversification in cichlid adaptive radiations. Journal of Evolutionary Biology. 2010, 23: 1456-1467. 10.1111/j.1420-9101.2010.02004.x.

    Article  CAS  PubMed  Google Scholar 

  51. Hubbs CL: Fishes of the Yucatán Peninsula. 1936, Carnegie Institute of Washington Publications, 457: 157-287.

    Google Scholar 

  52. Revell LJ, Harmon LJ, Glor RE: Underparameterized model of sequence evolution leads to bias in the estimation of diversification rates from molecular phylogenies. Systematic Biology. 2005, 54: 973-983. 10.1080/10635150500354647.

    Article  PubMed  Google Scholar 

  53. Seehausen O, Terai Y, Magalhaes IS, Carleton KL, Mrosso HDJ, Miyagi R, van der Sluijs I, Schneider MV, Maan ME, Tachida H, et al: Speciation through sensory drive in cichlid fish. Nature. 2008, 455: 620-623. 10.1038/nature07285.

    Article  CAS  PubMed  Google Scholar 

  54. Seehausen O: Patterns in fish radiation are compatible with Pleistocene desiccation of Lake Victoria and 14,600 year history for its cichlid species flock. Proceedings of the Royal Society of London Series B-Biological Sciences. 2002, 269: 491-497. 10.1098/rspb.2001.1906.

    Article  Google Scholar 

  55. Rogers R, Karason H, van der Hilst R: Epirogenic uplift above a detached slab in northern Central America. Geology. 2002, 30: 1031-1034. 10.1130/0091-7613(2002)030<1031:EUAADS>2.0.CO;2.

    Article  Google Scholar 

  56. Bethune DC, Ryan M, Losilla J, Krasn M: Hydrogeology. Central America: Geology, Resources, and Hazards. Edited by: Bundschuh J, Alvarado GE. 2007, London: Taylor and Francis, 665-686.

    Google Scholar 

  57. Rabosky DL, Lovette IJ: Density-dependent diversification in North American wood warblers. Proceedings of the Royal Society B-Biological Sciences. 2008, 275: 2363-2371. 10.1098/rspb.2008.0630.

    Article  PubMed Central  Google Scholar 

  58. Danley PD, Kocher TD: Speciation in rapidly diverging systems: lessons from Lake Malawi. Molecular Ecology. 2001, 10: 1075-1086. 10.1046/j.1365-294X.2001.01283.x.

    Article  CAS  PubMed  Google Scholar 

  59. Kornfield IL: Evidence for rapid speciation in African cichlid fishes. Experientia. 1978, 34: 335-336. 10.1007/BF01923020.

    Article  Google Scholar 

  60. Meyer A, Kocher TD, Basasibwaki P, Wilson AC: Monophyletic origin of Lake Victoria cichlid fishes suggested by mitochondrial DNA sequences. Nature. 1990, 347: 550-553. 10.1038/347550a0.

    Article  CAS  PubMed  Google Scholar 

  61. Sturmbauer C, Hainz U, Baric S, Verheyen E, Salzburger W: Evolution of the tribe Tropheini from Lake Tanganyika: synchronized explosive speciation producing multiple evolutionary parallelism. Hydrobiologia. 2003, 500: 51-64. 10.1023/A:1024680201436.

    Article  Google Scholar 

  62. Verheyen E, Salzburger W, Snoeks J, Meyer A: Origin of the superflock of cichlid fishes from Lake Victoria, East Africa. Science. 2003, 300: 325-329. 10.1126/science.1080699.

    Article  CAS  PubMed  Google Scholar 

  63. Kocher TD: Adaptive evolution and explosive speciation: The cichlid fish model. Nature Reviews Genetics. 2004, 5: 288-298. 10.1038/nrg1316.

    Article  CAS  PubMed  Google Scholar 

  64. Day JJ, Cotton JA, Barraclough TG: Tempo and mode of diversification of Lake Tanganyika cichlid fishes. PLOS One. 2008, 3: 10-10.1371/journal.pone.0001730.

    Article  Google Scholar 

  65. McCune A: How fast is speciation? Molecular, geological, and phylogenetic evidence from adaptive radiations of fishes. Molecular evolution and adaptive radiation. Edited by: Sytsma TJGKJ. 1997, Cambridge, UK: Cambridge University Press, 585-610.

    Google Scholar 

  66. Bolnick DI, Near TJ: Tempo of hybrid inviability in centrarchid fishes (Teleostei: Centrarchidae). Evolution. 2005, 59: 1754-1767.

    Article  PubMed  Google Scholar 

  67. Thompson JD, Gibson TJ, Plewniak F, Jeanmougin F, Higgins DG: The CLUSTAL_X windows interface: flexible strategies for multiple sequence alignment aided by quality analysis tools. Nucleic Acids Research. 1997, 25: 4876-4882. 10.1093/nar/25.24.4876.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

  68. Maddison DR, Maddison WP: MACCLADE 4.0. 2000, Sunderland, MA: Sinauer Associates

    Google Scholar 

  69. Posada D, Crandall KA: MODELTEST: testing the model of DNA substitution. Bioinformatics. 1998, 14: 817-818. 10.1093/bioinformatics/14.9.817.

    Article  CAS  PubMed  Google Scholar 

  70. Ronquist F, Huelsenbeck JP: MrBayes 3: Bayesian phylogenetic inference under mixed models. Bioinformatics. 2003, 19: 1572-1574. 10.1093/bioinformatics/btg180.

    Article  CAS  PubMed  Google Scholar 

  71. Swofford DL: PAUP*: phylogenetic analyses using parsimony (* and other methods). beta version 4.0 edn. 2002, Sunderland, MA: Sinauer

    Google Scholar 

  72. Sanderson MJ: r8s: inferring absolute rates of molecular evolution and divergence times in the absence of a molecular clock. Bioinformatics. 2003, 19: 301-302. 10.1093/bioinformatics/19.2.301.

    Article  CAS  PubMed  Google Scholar 

  73. Byerly GR: Igneous activity. The Gulf of Mexico Basin: The Geology of North America. Edited by: Salvador A. 1991, Boulder, CO: Geological Society of America, 91-108.

    Google Scholar 

  74. Maddison WP, Maddison DR: Mesquite: a modular system for evolutionary analysis. 2009, [http://mesquiteproject.org]2.71

    Google Scholar 

  75. Schluter D, Price T, Mooers AO, Ludwig D: Likelihood of ancestor states in adaptive radiation. Evolution. 1997, 51: 1699-1711. 10.2307/2410994.

    Article  Google Scholar 

  76. Rambaut AP: PhyloGen. Oxford: Department of Zoology, University of Oxford; 2002, 1.0

  77. Nee S, Mooers AO, Harvey PH: Tempo and mode of evolution revealed from molecular phylogenies. Proceedings of the National Academy of Sciences of the United States of America. 1992, 89: 8322-8326. 10.1073/pnas.89.17.8322.

    Article  PubMed Central  CAS  PubMed  Google Scholar 

Download references

Acknowledgements

We thank B. Fitzpatrick, M. Niemiller, G. Reynolds, J. Robinson, M. Todd-Thompson, and L. Wisner for comments on an earlier version of this manuscript. Support for this project was provided through the University of Tennessee and the National Science Foundation (NSF IOS-0919459).

Author information

Authors and Affiliations

  1. Department of Ecology and Evolutionary Biology, University of Tennessee, Knoxville, TN, USA

    C Darrin Hulsey, Phillip R Hollingsworth Jr & James A Fordyce

Authors
  1. C Darrin Hulsey
    View author publications

    You can also search for this author in PubMed Google Scholar

  2. Phillip R Hollingsworth Jr
    View author publications

    You can also search for this author in PubMed Google Scholar

  3. James A Fordyce
    View author publications

    You can also search for this author in PubMed Google Scholar

Corresponding author

Correspondence to C Darrin Hulsey.

Additional information

Authors' contributions

CDH and JAF conceived of the study. PRH performed most of the sequencing and some of the phylogenetic analyses. CDH and JAH performed and analyzed the LTT analyses. All three authors contributed to the writing of the manuscript.

Electronic supplementary material

12862_2010_1495_MOESM1_ESM.DOC

Additional file 1: Included cichlid species. Cichlid cytochrome b sequences used to generate the Heroine chronogram. Generic names that are repeated in the list are followed with shortened versions of the genus using multiple letters to clarify the genus to which they are currently assigned. (DOC 42 KB)

12862_2010_1495_MOESM2_ESM.DOC

Additional file 2: Heroine species that were not included in this study. Putative Heroine species that are extant [10, 11, 13, 51] but are not included in our phylogeny are listed. (DOC 27 KB)

Authors’ original submitted files for images

Rights and permissions

This article is published under license to BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Reprints and permissions

About this article

Cite this article

Hulsey, C.D., Hollingsworth, P.R. & Fordyce, J.A. Temporal diversification of Central American cichlids. BMC Evol Biol 10, 279 (2010). https://doi.org/10.1186/1471-2148-10-279

Download citation

  • Received:

  • Accepted:

  • Published:

  • DOI: https://doi.org/10.1186/1471-2148-10-279

Keywords

BMC Ecology and Evolution

ISSN: 2730-7182

Contact us