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Keywords:

  • Abies chensiensis ;
  • Abies fargesii ;
  • allopatry;
  • genetic divergence;
  • natural selection;
  • parapatry

Abstract

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References

Because of introgressive hybridization, closely related species can be more similar to each other in areas of range overlap (parapatry or sympatry) than in areas where they are geographically isolated from each other (allopatry). Here, we report the reverse situation based on nuclear genetic divergence between two fir species, Abies chensiensis and Abies fargesii, in China, at sites where they are parapatric relative to where they are allopatric. We examined genetic divergence across 126 amplified fragment length polymorphism (AFLP) markers in a set of 172 individuals sampled from both allopatric and parapatric populations of the two species. Our analyses demonstrated that AFLP divergence was much greater between the species when comparisons were made between parapatric populations than between allopatric populations. We suggest that selection in parapatry may have largely contributed to this increased divergence.


Introduction

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References

Introgression commonly occurs between closely related species in areas where their distributions overlap (Anderson and Hubricht 1938; Rieseberg and Wendel 1993; Sullivan et al. 2004; Mehner et al. 2010). This can lead to two species being genetically more similar in areas of range overlap (parapatry or sympatry) than in areas where they are geographically isolated from each other (allopatry) (Palme et al. 2004; Behm et al. 2010; McKinnon et al. 2010). Alternatively, selection can act to minimize resource competition or reproductive interference between closely related species in parapatry (or sympatry), thereby promoting exaggerated interspecific divergence and thus enabling them to coexist (Pfennig and Pfennig 2010). Accordingly, a distinct pattern of increased interspecific differentiation between closely related species in parapatry (or sympatry) compared with that in allopatry has been reported for ecological and reproductive traits in a number of animals and plants (Levin 1978; Sætre et al. 1997; Grant and Grant 2006; Niet et al. 2006; Kay and Schemske 2008; Smith and Rausher 2008; Urbanelli and Porretta 2008; Kirschel et al. 2009; Grossenbacher and Whittall 2011). This process of divergence of characters between species in response to selection is usually termed “character displacement” (Brown and Wilson 1956; Pfennig and Pfennig 2009).

Although empirical and theoretical work on character displacement has illuminated the role of selection in promoting divergent evolution and triggering speciation (Pfennig and Pfennig 2009; Hoskin and Higgie 2010; Hopkins and Rausher 2011), relatively little work has explored the extent to which selection could potentially reduce gene flow and contribute further to genetic divergence across the genome (Hoskin et al. 2005; Hopkins et al. 2012; Nosil et al. 2012). The analysis of genomic patterns of divergence between incipient species experiencing secondary contact represents a powerful approach to address these questions. In this study, we focus on two fir species, Abies chensiensis and Abies fargesii from central China. Most populations of these two species are allopatric, but in some areas the species co-occur (Fu et al. 1999). In allopatry, both species usually grow at elevations from 1500 to 3000 m, but in areas of parapatry A. chensiensis is more abundant at lower elevations, whereas A. fargesii tends to occupy sites at higher altitudes (Guan 1982; Zhang 2001). Morphologically, the two species are distinguished by the color of branchlets and seed cones, the morphology of bracts, and the shape and color of leaf needles (Fu et al. 1999) (Fig. 1). Accordingly, A. chensiensis and A. fargesii have been grouped into two different sections on the basis of the most widely recognized classifications (Liu 1971; Farjon and Rushforth 1989). Nevertheless, a lack of genetic differences between them for both chloroplast (cp) and mitochondrial (mt) DNA sequences indicates that the two fir species are in fact closely related and might represent an incipient stage of speciation, with insufficient divergence time having occurred for complete lineage sorting of ancestral polymorphisms (Wang et al. 2011).

image

Figure 1. The photo shows phenotypic differences between Abies chensiensis and Abies fargesii.

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Based on the distribution of cpDNA and mtDNA diversity within and between both species, it has been suggested that parapatric populations likely represent secondary contact zones between the species, which formed after the penultimate glacial period (Wang et al. 2011). Because introgression frequently occurs in conifers, especially in secondary contact zones (Liepelt et al. 2002; Petit et al. 2005; Semerikova et al. 2011), we might expect that introgression will have reduced genetic divergence between these two species in parapatric compared with allopatric sites. Alternatively, speciation in parapatry may have been facilitated or even finalized by the evolution of reproductive barriers through the process of character displacement (Pfennig and Pfennig 2010; Abbott et al. 2013; Hopkins 2013). If this is correct, loci under divergent selection (plus neutral sites tightly linked to them) may exhibit enhanced genetic divergence in parapatry relative to other parts of the genome subject to weak or no selection, and where lineage sorting is incomplete and/or where the homogenizing effects of gene flow are more extreme (Nosil et al. 2009; Hopkins et al. 2012). Divergent selection may also reduce gene flow globally across the genome, facilitating the accumulation of genome-wide divergence between parapatric populations, although the degree of divergence might still be substantially heterogeneous across the genome depending on the distribution of selected sites (Nosil et al. 2008; Feder et al. 2012; Flaxman et al. 2013). The goals of this study were (1) to determine whether there is increased or reduced genetic differentiation between parapatric populations compared with allopatric populations of these two recently diverged fir species; (2) to explore how genetic differentiation is distributed throughout the genome and whether regions of divergence are concentrated in just a few ‘genomic islands’ or is widespread across the genome.

Materials and Methods

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References

Sampling

We sampled indigenous, phenotypically pure populations of A. chensiensis and A. fargesii from almost the entire range of the two species in China. In total, five populations of A. chensiensis and 10 populations of A. fargesii were sampled from allopatric sites, while four populations of each species were sampled from sites where they were parapatric (Table 1; Fig. 2). We specified populations as parapatric if the two species grew together in the same valley or on the same mountain with A. fargesii occurring above 2200 m, and A. chensiensis at lower elevations. Fresh needles of individuals, spaced at least 100 m apart, were collected from each population and dried in silica gel. Representative vouchers were made from each population and deposited in the Lanzhou University herbarium.

Table 1. Description of allopatric and parapatric populations sampled in Abies chensiensis and Abies fargesii.
PopulationLocationRegionLatitude(N)Longitude(E)Altitude (m) N % polymorphic loci H e
  1. N, number of individuals analyzed; % polymorphic loci, the percentage of loci that are polymorphic out of the total 126 loci; He, mean expected heterozygosity.

  2. HN, Henan; GS, Gansu; SX, Shanxi; HB, Hebei; SC, Sichuan.

A. chensiensis
1Neixiangxian HNAllopatry33°02.415′111°50.578′25163100.00.229
2Yiwaxiang GSAllopatry34°11.652′103°11.810′27761442.10.210
3Lazikou GSAllopatry33°48.285′103°41.583′2441895.20.199
4Zhouqu GSAllopatry33°33.467′104°20.738′2058694.40.246
5Lueyang SXAllopatry33°27.842′106°27.638′1380594.40.254
6Foping SXParapatry33°15.075′107°59.491′1986793.70.281
7Ningshanxian SXParapatry33°31.455′108°21.111′1366891.30.213
8Ningshanxian SXParapatry33°47.172′108°20.227′2012588.10.246
9Shennongjia HBParapatry31°48.037′110°30.101′18091293.70.284
Subtotal     68  
A. fargesii
10Shennongjia HBParapatry31°42.347′110°39.157′2256483.30.199
11Shennongjia HBParapatry31°27.108′110°17.011′26501691.30.242
12Ningshanxian SXParapatry33°47.172′108°20.227′2573584.90.196
13Foping SXParapatry33°15.075′107°59.491′24201332.50.169
14Zhouzhi SXAllopatry33°51.058′107°50.355′21894100.00.303
15Meixian SXAllopatry34°09.546′107°50.383′2680794.40.204
16Xinjiashan SXAllopatry34°16.219′106°31.562′20971095.20.223
17Huoyanshan GSAllopatry34°22.546′106°14.201′25631293.70.226
18Lintan GSAllopatry34°54.407′103°41.351′2945592.10.217
19Diebu GSAllopatry34°08.232′103°53.022′2600893.70.234
20Lianhuashan GSAllopatry34°56.453′103°45.470′3196790.50.233
21Wenxian GSAllopatry32°57.522′104°38.076′2357589.70.242
22Chuanzhusi SCAllopatry32°46.407′103°37.220′2688592.90.292
23Huanglong SCAllopatry32°45.011′103°49.133′32913100.00.287
Subtotal     104  
Total     172  
image

Figure 2. Sampling localities and distributions of Abies chensiensis (marked by black solid triangle and red dashed line) and Abies fargesii (marked by black solid circle and black dashed line) in central China (in the upper right corner). Sampled populations (details in Table (1).) in this study include both allopatric and parapatric populations of Abies chensiensis (marked by white and black triangles) and A. fargesii (marked by white and black circles). Parapatric areas are shown in three independent dashed squares.

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DNA extraction and AFLP genotyping

Genomic DNA was extracted from approximately 20 mg of silica gel-dried, needle material per sample according to a cetytrimethyl ammonium bromide (CTAB) procedure (Doyle and Doyle 1987). Amplified fragment length polymorphism profiles were generated using a protocol modified slightly from Vos et al. (1995). An initial screening of selective primers was performed on six individuals from six populations, using 20 primer combinations with three selective nucleotides. We selected three EcoRI/MseI primer pairs producing the most repeatable and unambiguously scorable profiles. Fluorescence-labeled fragments were separated on a CEQ 8000 capillary sequencer (Beckman Coulter), with an internal size standard. All loci between 100 and 500 bp were then visually inspected in all individuals. Only unambiguously scorable loci and individuals were included in the analysis, and peaks found in <3% of individuals were excluded. In total, 172 individuals were scored for 126 AFLP markers, with all scoring being performed blind to population of origin. To ensure high repeatability of analyzed AFLP loci, we ran a subset of 30 individuals twice from the preselective amplification step. The average per-locus genotyping error rate for the AFLP data, measured as recommended by Bonin et al. (2004), was 2.6%.

Genetic diversity and population structure

To assess genetic diversity in each population, the percentage of polymorphic fragments and Nei's expected heterozygosity (He) were determined. We also estimated total diversity (HT), within-population diversity (HS), between-population diversity (HB), and population differentiation (FST) for allopatric and parapatric populations of each species, taken separately and in combination, using the method of Lynch and Milligan (1994) as implemented in the program AFLP-SURV version 1.0 (Vekemans et al. 2002). Because the inbreeding coefficient (f) cannot be calculated directly due to the dominant nature of AFLPs, we employed an alternative Bayesian approach developed by Holsinger et al. (2002) to estimate an FST analogue (designated by θB) for dominant markers, which accounts for uncertainty in f and simultaneously provides accurate and reliable estimates of genetic differentiation (Holsinger and Wallace 2004; Holsinger and Lewis 2007). Using the program HICKORY version 1.1 (Holsinger and Lewis 2007), we ran three models separately: (1) full model (both θB and f are unknown); (2) = 0 model (θB is unknown and no inbreeding occurs); (3) f-free model (f was not estimated but was chosen at random from the prior distribution). The posterior distribution of θB was estimated through Markov Chain Monte Carlo (MCMC) methods by HICKORY v1.1, with a burn-in of 5000 iterations and a sampling run of 25,000 iterations from which every fifth sample was retained for posterior calculations. The deviance information criterion (DIC) was subsequently used to determine the model showing the best fit to the data (Holsinger and Wallace 2004). To reveal differentiation patterns, we calculated pairwise FST and θB values between a priori defined groups based on various combinations of species (A. chensiensis and A. fargesii) and population type (allopatric and parapatric) using AFLP-SURV 1.0 and HICKORY 1.1. The significance of FST values was calculated based on comparison with values obtained from 10,000 randomly permuted individuals among the populations and/or between groups. We then constructed a neighbor-joining (NJ) tree with the program NEIGHBOR incorporated in the software package PHYLIP version 3.6 (Felsenstein 2004). Bootstrap support for internal nodes was estimated with a 10,000 distance matrix of replicates generated by AFLP-SURV 1.1, and a consensus tree was generated with CONSENSE in PHYLIP.

To visualize the relative genetic relationships between individuals and populations of A. chensiensis and A. fargesii, we conducted a principal coordinate analysis (PCoA) on a genetic distance matrix generated from the binary presence–absence matrix as implemented in GENALEX 6.2 (Peakall and Smouse 2006). Principal coordinate model clustering (PCO-MC), which couples PCoA with a clustering procedure, was used to further determine significant population structure in the AFLP dataset following Reeves and Richards (2009) and http://lamar.colostate.edu/~reevesp/PCOMC/PCOMC.html. Rather than only visualizing the first two or three principal coordinate axes, this method simultaneously takes into consideration information for all axes of a PCoA and offers an object way to determine whether clusters found in the PCoA are significant using NTSYS and the MODECLUS procedure in SAS 9.1. In addition, hierarchical partitioning of genetic diversity was estimated by performing analyses of molecular variance (AMOVA) (Excoffier et al. 1992) on populations grouped according to population type (allopatric and parapatric) within each species, and/or according to species (A. chensiensis and A. fargesii) as implemented for dominant markers in GENALEX 6.2 (Peakall and Smouse 2006), with significance tested by a nonparametric permutation procedure with 9999 permutations.

We checked whether genetic structure between parapatric and allopatric populations of A. chensiensis and A. fargesii was correlated with geographical distance, according to a pattern of isolation by distance (IBD). Pairwise genetic distance between populations was estimated using the Slatkin's linearized FST values (FST/1−FST) in ARLEQUIN 3.5 (Rousset 1997; Excoffier and Lischer 2010). Then, a Mantel test was performed on pairwise values of linearized FST and log-transformed geographical distances. The significance of these correlations was evaluated with 1000 permutations using the VEGAN package in R (R Development Core Team 2013). To compare the overall distribution of genetic differentiation across the genome between parapatric and allopatric populations of these two species, we used the Bayesian method of Foll and Gaggiotti (2008) to calculate locus-specific estimates of FST, which allows for the estimation of both population-specific effects (βj) and locus-specific effects (αi) on genetic differentiation and has been shown to be robust to complex demographic models.

Results

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References

Of a total of 126 AFLP loci surveyed, 101 (80.2%) were polymorphic. Values of average gene diversity (He) per population ranged between 0.199 and 0.284 for A. chensiensis, and between 0.169 and 0.303 for A. fargesii (Table 1). In each species, average within-population diversity (HS) was much higher than average between-population diversity (HB) for both allopatric and parapatric populations whether considered separately or together (Table 2). For all estimates of θB, the full model showed the best fit to the data, having the lowest DIC value (data not shown), and thus, we only present the θB values from the full model. Population differentiation (FST and θB) between parapatric or allopatric populations treated separately in both species was much lower than values of FST and θB obtained when all populations within species were considered together (Table 2). Estimates of genetic differentiation between A. chensiensis and A. fargesii in terms of FST and θB were much lower when allopatric populations were compared (FST = 0.0455, θB = 0.0533) than when comparisons were made only between parapatric populations (FST = 0.4053, θB = 0.4742) (Table 3). It was also the case that allopatric populations of Afargesii were more similar to parapatric populations of Achensiensis (FST = 0.1323, θB = 0.1904), than were allopatric populations of Achensiensis to parapatric populations of Afargesii (FST = 0.4040, θB = 0.4741). There was greater divergence between allopatric and parapatric populations in A. fargesii (FST = 0.3685, θB = 0.4411) than within Achensiensis (FST = 0.1559, θB = 0.2178) (Table 3). A neighbor-joining tree constructed with Nei's genetic distances calculated for the entire AFLP dataset revealed that relationships between allopatric populations of both species were generally poorly resolved (bootstrap value <50) (Fig. 3B). By contrast, populations in parapatry were clearly structured into two distinct and highly supported clades (bootstrap value = 100) corresponding to the two species (Fig. 3B).

Table 2. Genetic diversity statistics for Abies chensiensis, Abies fargesii, and for allopatric and parapatric populations within each species.
Species H T H S H B F ST θ B
  1. HT, total population diversity; HS, average within-population diversity; HB, average between-population diversity; FST and θB, the population differentiation (θB with 95% credibility intervals in parentheses); NS, not significant.

  2. a

    Significant at < 0.001.

A. chensiensis
Allopatric populations0.22970.22780.00200.0084NS0.0310 (0.0076–0.0633)
Parapatric populations0.27160.25600.01560.0573a0.1009 (0.0641–0.1459)
Total0.27050.24030.03020.1112a0.1688 (0.1363–0.2036)
A. fargesii
Allopatric populations0.25630.24610.01020.0398a0.0671 (0.0428–0.0957)
Parapatric populations0.21410.20160.01250.0580a0.0609 (0.0294–0.1008)
Total0.29860.23340.06530.2197a0.2992 (0.2670–0.3325)
Table 3. Matrices of pairwise FST (below diagonal) and θB (above diagonal) for comparisons of allopatric and parapatric populations between and within species.
PopulationsSpeciesAllopatricParapatric
A. chensiensis A. fargesii A. chensiensis A. fargesii
  1. a

    Significant at < 0.001. θB with 95% credible intervals in parentheses following estimates.

Total loci
Allopatric A. chensiensis 0.0533 (0.0319–0.0819)0.2178 (0.1509–0.2996)0.4741 (0.4043–0.5395)
A. fargesii 0.0455a0.1904 (0.1339–0.2632)0.4411 (0.3658–0.5119)
Parapatric A. chensiensis 0.1559a0.1323a0.4742 (0.4053–0.5354)
A. fargesii 0.4040a0.3685a0.4053a
image

Figure 3. (A) Principal coordinate analysis of AFLP marker variation among 172 individuals in Abies chensiensis and Abies fargesii. The variance explained by PC1 and PC2 is 53.4% and 19.4%, respectively. The three clusters that were found to be significant in the PCO-MC analysis are circled by different color. (B) Unrooted neighbor-joining tree based on Nei's genetic distance between populations of Abies chensiensis and Abies fargesii. Populations are labeled as in Fig. 1, and branches are color-coded as in (A). Bootstrap values over 50 are shown next to the corresponding branches.

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A plot of individual scores against the first two principal coordinates extracted from the PCoA and accounting for 53.4% and 19.4% of the variance, respectively, divided the dataset into three significantly distinct clusters as identified by PCO-MC analysis (circled in Fig. 3A). The largest of these clusters mainly comprised allopatric individuals of the two species, while the second cluster was mainly composed of parapatric individuals of Achensiensis, and the third cluster consisted of only parapatric Afargesii individuals. In general, these patterns of divergence were confirmed by the results of AMOVA, which showed that while only 5% of total variation was accounted for by interspecific differences between allopatric populations, 52% of total variation was due to differences between species when parapatric populations were compared (Table 4). Furthermore, 25% and 48% of total variance was partitioned between allopatric and parapatric populations within Achensiensis and Afargesii, respectively. The percentage of genetic diversity measured among populations within population types (allopatric or parapatric) was very low in all comparisons (Table 4).

Table 4. Analysis of molecular variance (AMOVA) for AFLP variation within and between Abies chensiensis and Abies fargesii when individuals were grouped according to population type, that is, allopatric or parapatric.
Species/RegionsSource of variationdfSSEst. variance% VarianceValueP value
  1. df, degree of freedom; SS, sum of squares.

A. chensiensis Among population type (allopatric vs. parapatric)1119.913.0825ΦRT = 0.2460.001
Among populations within population type798.440.756ΦPR = 0.0790.001
Within populations59514.358.7269ΦPT = 0.3050.001
Total67732.7112.55   
A. fargesii Among population type (allopatric vs. parapatric)1428.028.5248ΦRT = 0.4780.001
Among populations within population type12168.840.794ΦPR = 0.0850.001
Within populations90766.268.5148ΦPT = 0.5230.001
Total1031363.1317.83   
Allopatric populationsAmong species137.270.55ΦRT = 0.0530.001
Among populations within species13163.110.637ΦPR = 0.0700.001
Within populations87730.468.3988ΦPT = 0.1190.001
Total101930.839.53   
Parapatric populationsAmong species1399.2610.9352ΦRT = 0.5240.001
Among populations within species6104.181.045ΦPR = 0.1050.003
Within populations62550.168.8743ΦPT = 0.5740.001
Total691053.6020.84   

Despite the strong population structure observed in both Achensiensis and Afargesii, there was no evidence for isolation by distance (Mantel test: = −0.022, = 0.499, and = −0.069, = 0.514, for allopatric and parapatric populations, respectively). The lack of evidence for IBD in both allopatric and parapatric populations of each species (Fig. 4) indicates that the strong genetic differentiation between parapatric populations is likely not caused by neutral demographic processes associated with range expansion. Moreover, an examination of the distribution of locus-specific FST values between allopatric and parapatric populations of both species showed that it was strongly “L-shaped”, with most loci showing little or no divergence between allopatric populations (Fig. 5). In contrast, FST values for adjacent parapatric populations were shifted to the right of this distribution (Fig. 5). In line with this, parapatric populations exhibited significantly higher average values of FST relative to allopatric populations (Wilcoxon rank sum test, < 0.001, mean FST = 0.038 for allopatric populations and FST = 0.240 for parapatric populations). Thus, rather than being restricted solely to outlier loci, it appears that interspecific divergence in parapatry is characterized by widespread genetic differentiation across the genome.

image

Figure 4. Comparison of isolation by geographical distance between populations. Black and red dots indicate interspecific comparisons between allopatric populations and parapatric populations, respectively, whereas green and blue dots indicate intraspecific comparisons between allopatric populations and parapatric populations, respectively.

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image

Figure 5. Frequency distributions of locus-specific FST values for comparisons between allopatric (black) and parapatric (red) pairs of populations. The FST distribution tended to be “L-shaped” for allopatric population pairs and shifted to the right for parapatric populations.

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Discussion

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References

In contrast to an initial expectation that genetic divergence between parapatric populations of two species of Abies, Achensiensis and Afargesii might be reduced due to introgression, we found that divergence based on amplified fragment length polymorphism was much greater between parapatric populations than between allopatric populations. This difference could result from demographic processes associated with range expansions of the two species (Freedman et al. 2010). For example, if parapatric populations of both species were derived from allopatric ones, repeated bottleneck events associated with recent expansion might have lead to increased genetic divergence between parapatric populations due to founder events and genetic drift. However, this hypothesis is inconsistent with our previous phylogeographical study of these two species (Wang et al. 2011). Based on an analysis of cpDNA and mtDNA sequence variation, we previously obtained no evidence that allopatric populations of either species had undergone range expansion to give rise to parapatric populations at least since the penultimate glacial period (Wang et al. 2011). Furthermore, strong genetic drift associated with demographic expansion would result in reduced genetic diversity, which was not evident from comparisons of expected heterozygosity made between allopatric and parapatric populations of either species (Table 1). Finally, no geographical pattern of isolation by distance (IBD) was found for either intraspecific or interspecific comparisons in allopatry and parapatry (Fig. 4), suggesting that geographical distance has played either no role or a minor role in restricting gene flow within and between these species. Because there are no physical barriers to gene flow between allopatric and parapatric populations of both species, the striking pattern of increased divergence between species in parapatry, and also between parapatric and allopatric populations of the same species, cannot result from geographical barriers to gene flow. It would seem, therefore, that neutral genetic drift or other demographic processes are unlikely to have caused the increased genetic divergence observed between the two species in parapatry, although further investigations are needed to rule out these possibilities entirely.

Based on our results, it seems more likely that increased genetic divergence between Achensiensis and Afargesii in parapatry may reflect the effects of divergent selection (Barton and Bengtsson 1986; Beaumont and Balding 2004; Dayan and Simberloff 2005; Storz 2005; Stinchcombe and Hoekstra 2007; Nosil et al. 2008, 2009; Pfennig and Pfennig 2009) as follows. First, it is feasible that selection may have acted to increase ecological adaptation to different habitats, so as to reduce interspecific competition in areas of species overlap (Schluter 2001; Nosil 2012). This prediction is consistent with field observations showing that while both species grow over the same range of altitude in allopatry, in parapatry, Achensiensis occurs mainly at low altitudes while Afargesii is found above 2200 m (Guan 1982; Zhang 2001). However, further investigation will be required to prove that adaptive ecological divergence has taken place, possibly involving transplant studies and the analysis of candidate genes responsible for local adaptation at parapatric sites. Second, given that hybridization between recently diverged conifer species is often recorded in the wild, we cannot rule out that selection may have acted to strengthen prezygotic isolation in parapatry (reinforcement) (Noor 1999; Servedio and Noor 2003; Servedio 2004; Petit and Hampe 2006). We have observed occasional individuals in the field exhibiting intermediate morphology to Achensiensis and A. fargesii, especially in areas of parapatry, indicating that hybridization occurs between these two species. If hybrids were formed frequently in the past and had low fitness relative to parental species, selection for reinforcement might have occurred at parapatric sites causing barriers to gene flow to strengthen (Hopkins 2013). Third, rather than being driven by interspecific interactions in parapatry, local adaptation to biotic and/or abiotic conditions existing between allopatric and parapatric sites occupied by the same species could have indirectly caused the increased genetic divergence between parapatric populations (Nosil 2012; Hopkins 2013). Although we are currently unable to discriminate among these potential selective mechanisms, future studies combining morphological, ecological, and genomic data will hopefully do so and reveal why there is increased genomic divergence between parapatric populations of A. chensiensis and A. fargesii.

The very low level of AFLP divergence recorded between species based on comparisons between allopatric populations was somewhat surprising given their morphological divergence in allopatry (Liu 1971; Farjon and Rushforth 1989). This suggests that taxonomically important morphological differences between these species might be controlled by relatively few loci and that allopatric populations are genetically similar at most loci (Fig. 5). This prediction is consistent with our previous study, which indicated that the species pair is probably at an initial stage of divergence (Wang et al. 2011). In contrast, higher levels of between species differentiation in parapatry imply that divergent selection might have reduced effective gene flow sufficiently for widespread divergence to accumulate between populations across the genome, instead of being restricted to sites tightly linked to a few loci subject to divergent selection (Feder et al. 2012; Flaxman et al. 2013). Because the distribution of selected sites can vary across the genome, a large degree of heterogeneity in levels of genetic differentiation between parapatric populations might be generated as observed in our study (Fig. 5). This pattern is consistent with one expected under “genome hitchhiking” (Feder et al. 2012). Future comparisons of the genome sequences of these two Abies species in parapatry and allopatry are now required to establish the exact level and pattern of genomic divergence, which exists between them.

Acknowledgments

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References

We thank Patrick A. Reeves for helping running the PCO-MC analysis, and we also thank Yongshui Sun for modifying the format of the paper. This research was supported by National Key Project for Basic Research (2014CB954100) and a Royal Society-NSF China International Joint Project award 2010/R4 to R. J. A. and J. Q. L. The stay of Jing Wang in Sweden was supported by the Chinese Scholarship Council.

References

  1. Top of page
  2. Abstract
  3. Introduction
  4. Materials and Methods
  5. Results
  6. Discussion
  7. Acknowledgments
  8. Conflict of Interest
  9. References