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Phylogeography of Camellia taliensis (Theaceae) inferred from chloroplast and nuclear DNA: insights into evolutionary history and conservation

Abstract

Background

As one of the most important but seriously endangered wild relatives of the cultivated tea, Camellia taliensis harbors valuable gene resources for tea tree improvement in the future. The knowledge of genetic variation and population structure may provide insights into evolutionary history and germplasm conservation of the species.

Results

Here, we sampled 21 natural populations from the species' range in China and performed the phylogeography of C. taliensis by using the nuclear PAL gene fragment and chloroplast rpl32-trnL intergenic spacer. Levels of haplotype diversity and nucleotide diversity detected at rpl32-trnL (h = 0.841; π = 0.00314) were almost as high as at PAL (h = 0.836; π = 0.00417). Significant chloroplast DNA population subdivision was detected (GST = 0.988; NST = 0.989), suggesting fairly high genetic differentiation and low levels of recurrent gene flow through seeds among populations. Nested clade phylogeographic analysis of chlorotypes suggests that population genetic structure in C. taliensis has been affected by habitat fragmentation in the past. However, the detection of a moderate nrDNA population subdivision (GST = 0.222; NST = 0.301) provided the evidence of efficient pollen-mediated gene flow among populations and significant phylogeographical structure (NST > GST; P < 0.01). The analysis of PAL haplotypes indicates that phylogeographical pattern of nrDNA haplotypes might be caused by restricted gene flow with isolation by distance, which was also supported by Mantel’s test of nrDNA haplotypes (r = 0.234, P < 0.001). We found that chlorotype C1 was fixed in seven populations of Lancang River Region, implying that the Lancang River might have provided a corridor for the long-distance dispersal of the species.

Conclusions

We found that C. taliensis showed fairly high genetic differentiation resulting from restricted gene flow and habitat fragmentation. This phylogeographical study gives us deep insights into population structure of the species and conservation strategies for germplasm sampling and developing in situ conservation of natural populations.

Background

Crop wild relatives, which include wild progenitors of cultivated plants as well as other closely related species, are important components of natural habitats and agroecosystem [1]. They may contain desirable alleles that can enhance pest/disease resistance and abiotic adaptation, or improve nutritional values or flavour of crops, providing plant breeders with a broad pool of potentially useful genetic resources. Wild relatives have repeatedly served as important sources of useful traits for genetically impoverished crops in the past decades [2]. However, these wild species are subject to an increasing range of threats in their natural habitats [3]. To design optimal conservation and management strategies, it is necessary to trace their evolutionary histories by better investigating their population structure.

Phylogeographical studies have been emerging as a powerful tool for understanding population structure and evolution of plant species [4, 5]. By synthesizing the influence of both history and current genetic exchanges, phylogeography uses genealogical and geographical information to infer the demographic and historical processes that shaped the evolution of populations and species [5, 6]. Recent decades have witnessed increasing applications of phylogeography in economically important plants and their wild relatives [2, 712].

The genus Camellia is composed of over 110 taxa [13], of which only one species, C. sinensis (L.) O. Kuntze, is commercially used as a source of the beverage tea. C. taliensis is one of the most important wild relatives of the cultivated tea, and they together belong to the section Thea. Both them are monoecious, insect-pollinated, and outcrossing species. They differ primarily in the number of locules and the size of flowers and leaves. The number of locules per ovary is five in C. talensis, while C. sinensis has three. C. taliensis usually grows in the mountainous evergreen broad-leaved forests at altitudes from 1300 to 2700 m, and is mainly distributed in southwestern Yunnan of China, as well as adjacent regions including northern Myanmar and Thailand. Because of its close relationship with the cultivated tea and fascinated aftertaste, C. taliensis also has been consumed instead of regular tea by local people in parts of Asia, particularly in Yunnan Province of China [13]. These wild tea germplasms undoubtedly harbor abundant gene sources and thus possess great potentials to enhance genetic improvement of cultivated tea in the future. Unfortunately, recent human overexploitation to subtropical forests has unavoidably made C. taliensis suffer the degradation and fragmentation of natural habitats suitable for natural populations of the species. In particular, the well-known Pu’er tea, made from organic leaves of wild C. taliensis plants in Yunnan Province, enjoys a price 10–100 times higher than cultivated tea trees in the market. For this reason, natural populations of the species have become endangered due to over-picking driven by economic incentives. Hence, it is urgently needed to pay particular attention to making efficient germplasm conservation of C. taliensis.

The use of molecular markers derived from nuclear and chloroplast genomes provides an unprecedented opportunity to investigate genetic structure and take insights into population history of a species, particularly by means of a combined analysis of biparentally inherited nuclear and maternally inherited organelle markers [4, 5, 1416]. In order to better elucidate population genetic structure and the phylogeography of C. taliensis, nucleotide polymorphisms of a total of 21 natural populations (Table 1) were screened by using the maternally inherited cpDNA rpl32-trnL spacer and biparentally inherited nuclear PAL gene fragment. It was shown that rpl32-trnL intergenic spacer could offer higher level of variation than other 33 noncoding regions in the chloroplast, and thus has been successfully applied in phylogeography analyses of many plants [1719]. Phenylalanine ammonialyase (PAL) was reported to involve in the phenylpropanoid pathway and is encoded by a single-copy gene [20]. As a result, it has often been used to evaluate genetic diversity of cultivated tea and elucidate the differentiation among cultivars [2123]. In this study, we aim to: (i) investigate levels of genetic diversity and genetic structure of C. taliensis populations; (ii) infer evolutionary forces that might have shaped the observed population structure and determine demographic and evolutionary history; and (iii) propose efficient strategies for guiding the future germplasm preservation actions and in situ conservation management.

Table 1 The sample sizes and geographical locations of the C. taliensis populations in this study

Results

Haplotype variation and neutrality tests

cpDNA sequences from the rpl32-trnL spacer were obtained from 183 individuals of C. taliensis and aligned to be 858 bp in length. These sequences represented 12 haplotypes with 18 polymorphic sites, including five insertions/deletions (indels) and 13 substitutions (Table 2). Of the five detected indels, three were single nucleotide, while the other two had 5 and 9 bp, respectively (Table 2). Of the analyzed 21 populations, only one population (CNB) harbored two chlorotypes, while the other 20 were monomorphic (Table 3 and Figure 1). It is of interest to find that two chlorotypes, C1 and C2, were detected in the ten populations from the Langcang River region. Chlorotype C1 was fixed in six populations CNC, SJ, GM, CY, XM and BD, and occurred with a high frequency in the population CNB. With the exception of a low frequency occurred in the CNB population, however, Chlorotype C2 was unique to populations FQ, NE and YX from Lancang River region and one eastern population JC. Three chlorotypes (C4, C9 and C12) were present within populations located in eastern range of the species, while the remaining seven (C3, C5, C6, C7, C8, C10 and C11) were found in western populations.

Table 2 Twelve haplotypes of C. taliensis identified in the rpl32-trnL sequences
Table 3 Chlorotype distribution and measures of haplotype diversity in C. taliensis populations
Figure 1
figure 1

The geographical distribution of 12 rpl32-trnL chlorotypes in the 21 C. taliensis populations. The Lancang River is indicated in blue, while red circle showes the range of the species.

The aligned nuclear PAL gene fragments of 627 bp were obtained from the 137 detected individuals of C. taliensis. With two singletons and without indels, 18 polymorphic sites were identified from 274 nrDNA sequences (Table 4). Of them, 13 polymorphic sites were synonymous, while the other five polymorphic sites were replacement changes. Among a total of 17 distinct nrDNA haplotypes found in the species, five haplotypes were common in the whole set of samples (Table 5 and Figure 2). The most frequent haplotype was H4 (observed 75 times, 27.4%), while H2 (observed 56 times, 20.4%), H6 (observed 44 times, 16.1%), and H1 (observed 34 times, 12.4%) were present in a total of 14, 18, 11 and 13 populations, respectively. In addition, Haplotype H3, which had only one mutational step from H1 and H6, was observed 20 times (7.3%) and appeared in a total of ten populations. All other haplotypes were observed 10 times or fewer (≤ 3.6%) and only present in fewer than two populations.

Table 4 Seventeen haplotypes of C. taliensis identified in nrDNA PAL sequences
Table 5 PAL haplotype distribution and measures of haplotype diversity in C. taliensis populations
Figure 2
figure 2

The geographical distribution of 17 PAL haplotypes in the 21 C. taliensis populations. The Lancang River is indicated in blue, while red circle showes the range of the species.

To investigate whether natural selection on the PAL may affect the inference of population structure in C. taliensis, neutrality test was performed by analyzing the entire dataset. Neither Tajima's D (D = −0.257, P > 0.1) nor Fu and Li's D* (D* = 0.52565, P > 0.1) rejected the null hypothesis of neutral evolution. Furthermore, we found that the minimum number of recombination events, Rm, was zero at PAL. Since PAL provided sufficient variation without the recombination and neutrally evolves, patterns of haplotype variation at this locus may reliably reflect the population history of C. taliensis.

Population genetic structure

Levels of haplotype and nucleotide diversity were investigated at both the nuclear PAL and chloroplast rpl32-trnL across all the 21 natural populations of C. taliensis. On the whole, levels of total haplotype diversity and overall nucleotide diversity detected at the locus rpl32-trnL (h = 0.841; π = 0.00314) (Table 3) were almost as high as at the locus PAL (h = 0.836; π = 0.00417) (Table 5). In this study, we failed to detect sequence variation within populations except for the CNB population at the locus rpl32-trnL (Table 3). However, it is noticeable that genetic diversity at the locus PAL varied largely from one population to another, with haplotype diversity ranging from 0.439 to 0.867, and nucleotide diversity varying from 0.0007 to 0.0047 (Table 5). Among the studied populations, the XM population exhibited the most abundant genetic diversity (h = 0.86667; π = 0.00471), while the FQ population possessed the lowest levels of genetic variability (h = 0.43956; π = 0.0007).

To further investigate population genetic structure of C. taliensis, genetic differentiation was examined by detecting sequence variation at both the nuclear PAL and chloroplast rpl32-trnL across the 21 natural populations. Chlorotype variation revealed that population differentiation was fairly high (GST = 0.988), which was almost as high as the ordered alleles (NST = 0.989). A permutation test showed that the difference between NST and GST was not significant (U = 0.07, P > 0.05). Nevertheless, we found a significantly larger NST of 0.301 than GST of 0.222 detected at the locus PAL (U = 3.34, P < 0.01). Analysis of molecular variance (AMOVA) further showed that the majority of chlorotype variation (98.75%, P < 0.001) was found among populations, and only a small amount (1.25%) was partitioned within populations (Table 6A). A global F ST value of 0.9875 also indicated fairly high differentiation among the sampled populations at the locus rpl32-trnL. However, AMOVA exhibited contrastingly different pattern of genetic differentiation among and within populations at the locus PAL. Although nucleotide diversity (77.49%) was mainly attributable to the variation within populations, significant proportion of diversity (22.51%, P < 0.001) was partitioned among populations (Table 6B). F ST analysis (F ST  = 0.225, P < 0.001) also indicate that considerable differentiation existed significantly among the sampled populations.

Table 6 AMOVA analysis of the 21 C. taliensis populations by using rpl32-trnL (A) and PAL (B) sequences

In addition, a significant correlation was detected between genetic and geographical distances (r = 0.234, P < 0.001) at the locus PAL, indicative of the isolation by distance between populations. Nevertheless, there was no significant correlation between genetic and geographical distances (r = −0.1134, P = 0.966) for the locus rpl32-trnL.

Nested clade phylogeographic analysis

A nested cladogram of chlorotypes was constructed through a TCS network by linking the haplotypes in a hierarchical manner (Figure 3). Seven one-step and three two-step clades were revealed with five clades that were significant under NCPA. In this study, we detected allopatric fragmentation in Clades 1–1 and 2–3. Clade 1–1 included chlorotypes C3, C10 and C11 sampled from the westernmost range of the species, while Clade 2–3 consisted of chlorotypes C2 and C12 distributed in eastern populations of the species. Clade 1–4 showed a restricted gene flow but with some extent of long-distance dispersal, and they distributed in the Lancang River region (Chlorotype C1), western (chlorotypes C5, C6 and C8) and eastern range (Chlorotype C4), respectively. As for Clade 2–2, we detected restricted gene flow/dispersal but with some extent of long-distance dispersal over intermediate areas not occupied by the species or past gene flow/dispersal followed by the extinction of intermediate populations. From the entire cladogram, it was inferred that they might have arisen via long-distance colonization and/or past fragmentation in (Additional file 1: Table S1).

Figure 3
figure 3

Nested cladogram of 12 chlorotypes across the 21 C. taliensis populations. Circles in colors denote different haplotypes, and the size of each circle is proportional to that haplotype frequency across populations. Each branch between the haplotypes represents a mutational step. The dotted lines indicate independent mutation events converging on a shared haplotype. The squared loops show the nested clades or haplotypes in the network, which were resolved by nested clade phylogeographic analysis (NCPA).

The conversion of statistical parsimony network for nrDNA haplotypes into a hierarchical nested design resulted in five one-step and three two-step clades (Figure 4). In total, NCPA showed that four clades were significant. In Clades 1–1 and 1–5, we detected restricted gene flow/dispersal but with some long-distance dispersal over intermediate areas not occupied by the species, or past gene flow followed by extinction of intermediate populations. Contiguous range expansion could account for the distribution of genetic variation within the Clade 2–3. Meanwhile, restricted gene flow with isolation by distance could be inferred, which might have shaped patterns observed within the total cladogram in (Additional file 2: Table S2).

Figure 4
figure 4

Nested cladogram of 17 nrDNA haplotypes across the 21 C. taliensis populations. Circles in colors denote different haplotypes, and the size of each circle is proportional to that haplotype frequency across populations. Each branch between the haplotypes represents a mutational step. The dotted lines indicate independent mutation events converging on a shared haplotype. The squared loops show the nested clades or haplotypes in the network, which were resolved by nested clade phylogeographic analysis (NCPA).

The net pairwise cpDNA divergence (dA) between three pairs of two-level clades was estimated to be 0.006245 (2–1 vs 2–2), 0.004753 (2–1 vs 2–3) and 0.001488 (2–1 vs 2–3), respectively. Assuming 1.0-3.0 × 10-9 s/s/y for synonymous cpDNA in seed plants [24], clade 2–1 and 2–2 might diverge approximately 1.04-3.12 MYA, the time of divergence between clade 2–1 and 2–3 could be dated to 0.79-2.38 MYA, and the divergence time between clade 2–2 and 2–3 was estimated to be 0.24-0.74 MYA.

Discussion

Genetic diversity and population structure

Of the 34 regions surveyed in the chloroplast genomes, rpl32-trnL intergenic spacer was previously proven to be suitable for the population-level phylogenetic studies [17], and thus has been successfully applied in phylogeography analyses of plants [18, 19]. In comparison to mean estimate of cpDNA diversity (h T  = 0.67) detected by various cpDNA markers in 170 plant species [4], our study showed that C. taliensis possessed an abundant variation in the chloroplast rpl32-trnL intergenic with cpDNA diversity (h) of 0.841. In addition, levels of total haplotype diversity and overall nucleotide diversity within natural populations of C. taliensis at rpl32-trnL (h = 0.841; π = 0.00314) (Table 3) were higher than the three cultivated populations of C. taliensis (h =0.610, π = 0.00225), indicating the reduction of genetic diversity during the domestication [25]. However, nucleotide diversity within C. taliensis in this study appears as high as that of nine cultivated populations of C. sinensis var. assamica from Yunnan, China (h =0.728, π = 0.00469) [25].

By using rpl32-trnL intergenic spacer and PAL gene fragment as markers, we estimated genetic structure of C. taliensis populations across its distribution range in China. cpDNA data suggest that the differentiation among the C. taliensis populations was rather high (GST = 0.988; NST = 0.989), placing it among the surveyed plant species with the highest cpDNA differentiation [4]. Partitioning of genetic variability showed that, on average, merely 1.25% of cpDNA variation was distributed within C. taliensis populations and up to 98.75% among populations (Table 6A). In comparison with the above-described cpDNA data, it is of interest to uncover that nrDNA PAL data showed a contrastingly different genetic structure of C. taliensis populations. Genetic differentiation (GST = 0.222, NST = 0.301) shows that, on average, up to 69.9-77.8% of nrDNA variation was partitioned within C. taliensis populations and merely 22.2-30.1% among populations. The estimates were slightly higher than the mean value of Gst of 0.184 for the other 77 angiosperms species [4]. In this study, we found that NST was significantly higher than GST, suggesting that pairs of different nrDNA haplotypes from the same population have more similar sequence than pairs of different haplotypes from markedly different populations. AMOVA analysis further revealed that the majority of PAL nucleotide diversity (77.49%, P < 0.001) was significantly attributable to the variation within populations (Table 6B). The lack of genetic differentiation in the nuclear genes probably results from ancestral polymorphisms maintained by a larger effective population size, or high dispersal possibilities of nuclear genes [5]. As for the wild tea tree of C. taliensis, it is likely that smaller effective population size of organelle DNA than nuclear DNA results in strong genetic drift and high levels of population differentiation [4, 5]. Because of the nature of cpDNA maternal inheritance in angiosperms, seed dispersal often plays an important role in shaping population genetic structure of maternally inherited cpDNA. C. taliensis usually generates heavy nut fruit with short-distance seed dispersal, and thus, rather limited abilities of seed dispersal among populations might lead to the observation of high cpDNA population subdivision.

Demographic history of C. Taliensis

NCPA in this study indicates that restricted gene flow and effects of the past fragmentation appear to be of significance in together shaping the observed patterns of chlorotype variation in C. taliensis. Allopatric fragmentation was apparently detected in clades 1–1 and 2–3 of the chlorotype network. The most likely explanation is that the species has recently suffered the degradation and fragmentation of natural habitats in consequence of recent human overexploitation to subtropical forests. Our field surveys particularly found that, driven by market incentives, a number of natural populations of C. taliensis have been seriously destroyed and thus become endangered in small effective population sizes caused by over-picking of organic leaves from natural populations of C. taliensis (Gao and Liu, unpublished data). Moreover, the range of C. taliensis in China covers western region of Yungui Plateau, which is adjacent to the southeast of Qinghai-Tibetan Plateau with an average elevation of approximately 4,500 m above sea level, the largest and highest plateau in the world [26]. The extremely complex topography and climates were formed during the uplift of the Plateau especially in the southeastern region of Qinghai-Tibetan and Yungui plateaus. As a result, significant increase in geological and ecological diversity has largely enhanced rapid divergence and speciation in small and isolated populations [27]. In addition to the recently fragmented habitats as a result of human destruction, the estimated range of separation times of 0.24-3.12 MYA among clades in this study post-dates the most recent uplift the Tibetan Plateau around 3.4 MYA [28, 29]. The species may have experienced habitat fragmentation possibly as a result of the uplift of Qinghai-Tibetan Plateau and subsequent larger-scale drainage. The past fragmentation may have resulted in the observed chlorotype structure of C. taliensis, although there is a lack of direct evidence to strongly support such an association of geographical patterns with the unspecified historical events. NCPA also detected the restricted gene flow in Clade 1–4 which included individuals from a total of eleven populations. It is true that the C. taliensis plants often produce heavy nut fruits with short-distance seed dispersal and thus the gene flow is fairly restricted among populations. The seriously fragmented habitats together with their endangered status indeed have largely accelerated the restricted gene flow among the small surviving natural populations detected in the species. However, one important characteristics of chlorotypes distribution was that Chlorotype C1 was found in the seven populations resided in the Lancang River region without exception. Such a geographical distribution of Chlorotype C1 suggests that the Lancang River might have provided northwards or southwards natural corridors for the long-distance dispersal of C. taliensis in China.

Hybridization is expected to have served as a possible driver of the observed patterns of chlorotypes. Geographic distribution of C. taliensis mostly covers the extensively growing range of C. sinensis. As previously documented in Baiying Mountains, Yunnan Province, hybrid zone which consists of a number of populations, called as “Er’Ga’Zi Tea”, was found to have formed between these two species (Chong-ren Yang, personal communications). However, the extent and effects of hybridization which might affect levels genetic variation and patterns of geographic population structure of C. taliensis remains largely unsettled and stays to be further studied.

It is our discovery that populations with geographical proximity did not share closely related geographical chlorotypes. For example, although TCB and TCD populations were geographically close with only 10 km distance apart, they were fixed for the distinct chlorotypes of C5 and C6, respectively. Such a pattern of cpDNA variation may come from incomplete lineage sorting of polymorphisms. As a kind of stochastic process randomly allocating ancestral polymorphisms into different populations or species, lineage sorting has been proven to be a major factor for the lack of associations between genealogical relationships of haplotypes and their geographical distributions [2]. Another possible explanation is that the past and recent habitat fragmentation of ancestral populations has led to the observed patterns of chlorotype structure in the species.

Isolation by distance can be tested through both the correlation of genetic and geographical distances and the nested clade phylogeographic analysis [30]. In this study, Mantel tests exhibited a significant correlation between genetic and geographical distances of PAL haplotypes, supporting the isolation by distance model across the study populations in C. taliensis. Moreover, the total cladogram of PAL haplotype network also showed the evidence of restricted gene flow with isolation by distance. Overall, both the correlation of genetic and geographical distances and NCPA together demonstrated that the population genetic structure of the species fitted the model of isolation by distance. Nevertheless, Mantel’s tests failed to detect significant correlations between genealogical relationships of chlorotypes and geographical distances. The discrepancy between the nrDNA PAL and cpDNA phylogeography of C. taliensis could result from different transmission mechanisms of nuclear and organelle genes, and/or their different tempos of lineage sorting through drift [5].

Implications for the germplasm conservation

As the most popular non-alcoholic beverage throughout the world, a large number of tea germplasms have been collected and ex situ preserved in China, Japan, India and Kenya [31]. Unlike cultivated tea varieties, their wild relatives have cold tolerance and are resistant to common diseases infecting cultivated tea tree, and thus they constitute valuable gene resources for local and international tea tree improvement programs in the future. Although efforts have been made to preserve cultivated tea germplasms, it is vital that more attention to be paid to the conservation of their wild relatives has been largely neglected so far. Knowledge of genetic variation between and within populations of rare and endangered species is extremely useful for making appropriate management strategies directed towards their conservation [32]. Of these wild species, C. taliensis is one of the most important wild relatives of the cultivated tea and is subject to increasing threats as a result of the overexploitation and deforestation. The uncovered genetic profile presented here not only helps to gain important insights into genetic structure of C. taliensis populations, but also has critical implications for taking appropriate strategies of the conservation and germplasm management.

Comprehensive understanding of regional genetic structure of C. taliensis in this study is required to design an appropriate conservation scheme. In view of abundant genetic diversity resided within C. taliensis populations, an appropriate strategy for both germplasm sampling and developing in situ conservation of those populations with a higher variation on behalf of different geographical regions is needed. In order to capture the considerable genetic variation harbored among populations, ex situ germplasm collection should have sufficient sample size from each population. Since at least 22% genetic diversity of PAL nucleotide diversity distributed among populations, germplasm collections should be sampled from extensive geographic origins. The observation that the majority of PAL variation was distributed within populations of this species is instructive for adopting a plan of involving fewer populations but more individuals within populations. Apparently, the populations with abundant haplotype diversity, such as XM, YJ, GM, YD, ZY, CY, and NE (Table 5), may be more attractive for both in situ conservation and ex situ germplasm collections. The populations with the unique PAL haplotypes, such as CNB, JC, TCH, XM, YD and YJ, should be given conservation priority (Table 5). The observed chlorotype structure showed an allopatric fragmentation in C. taliensis such as between Clades 1–1 and 2–3. Notably, three chlorotypes (C3, C11 and C10) distributed in the westernmost range of C. taliensis, while other two (C2 and C12) was found in eastern populations of the species (Figure 3), further implying that both germplasm sampling and setting in situ conservation localities should take different geographical origins and the observed chlorotype structure into consideration.

Considering that the most remnant populations of C. taliensis are turning into smaller as a result of human destruction, however, it is quite possible that the process of habitat fragmentation will lead to a loss of genetic diversity by dramatically increasing mating opportunities between relatives within small populations. The C. taliensis populations may have suffered habitat fragmentation due to either the uplift of Tibetan Plateau or recent deforestation, and thus brought about the observed chlorotype structure in C. taliensis. However, NCPA suggest that restricted gene flow/seed dispersal may have resulted in smaller effective population sizes of the outcrossing plant species due to the recently fragmented habitats and long-distance colonization. Consequently, conservation and restoration genetics should concentrate on the maintenance of historically significant processes such as strong gene flow/seed dispersal as well as large effective population size in the species.

Conclusions

Our phylogeographic study has revealed abundant genetic diversity and moderate genetic differentiation of natural populations of C. taliensis from the whole range of China. The data are indicative of taking effective conservation actions of these precious tea tree germplasm. However, it should be noted that samples from the entire range of the species are not represented in the present study. Therefore, a full picture of population genetic structure for the species as well as further understanding of evolutionary history and forces could be better outlined if extensive studies are completed in the seeing future. In addition, further detailed studies on reproductive biology should also help to explain the observed population structure of the wild tea tree species. Undoubtedly, such efforts will be critical for taking effective conservation of precious genetic resources of wild C. taliensis. Last of all, conservation consideration should be set to habitat management because human destruction of the species’ habitats has led to the species’ endangerment. Recent human destruction of wild C. taliensis populations driven by economic incentives plus the overexploitation and deforestation in subtropical regions have together led to the degradation and fragmentation of habitats suitable for natural populations of these species. Thus, the genetic diversity of remaining populations of the species has to be dynamically maintained in changeable environments, and long-term habitat protection is the most important to prevent genetic variation from further loss and a reduction of effective population size. Without a shred of doubt, successful conservation will largely rely on the scale of protection range of natural habitats and indeed the amount of positive participation by governments and local communities.

Methods

Material sampling and DNA extraction

In this study, a total of 185 individual plants from 21 wild populations of C. taliensis were sampled, representing almost the entire range of the species in China (Table 1; Figures 1 and 2). For each population, young, healthy leaves were collected from seven to thirty individual trees, depending on population size. To ensure adequate population coverage, random samples were taken from trees at an interval of about 3–100 m across the whole studied population. Voucher specimens were collected and deposited in the Herbarium of Kunming Institute of Botany, Chinese Academy of Sciences (KUN). Leaves were individually harvested in the field and silica-dried for subsequent DNA extractions. Genomic DNA was then isolated from liquid-nitrogen ground leaf tissues according to a CTAB method described by Doyle and Doyle [33].

PCR amplification and DNA sequencing

The extracted DNA was dissolved in 100 μL TE buffer and then used as the PCR templates. In this study, primer pairs used by Shaw et al. [17] were adopted to amplify the rpl32-trnL noncoding spacer of cpDNA (TRNL: 5' -CTG CTT CCT AAG AGC AGC GT -3', RPL32: 5'-CAG TTC CAA AA A AAC GTA CTT C-3'). In addition, a pair of primers (PAL F: 5'-TGC CAC AAT CAG CCA CAA G-3', PAL R: TGG TTG GTT ACA GGA TTG GC) was designed based on cDNA sequence from C. sinensis due to the unavailability of the entire genomic structure of PAL in C. taliensis.

DNA amplifications were carried out in a T1 thermocycler (Biometra), programmed for an initial 4 mins at 97 °C; followed by 35 cycles of 50 s at 95 °C, 50 s at 52 °C (rpl32-trnL) or 55 °C (PAL), 1 min at 72 °C; and an additional extension for 10 mins at 72 °C. Reactions were performed in 50 μL reaction volumes containing 50 mM KCl, 10 mM Tris–HCl (pH 8.3), 1.5 mM MgCl2, 200 μM of each dNTP, 0.1 μM of each primer, 30–50 ng of template DNA, and 1U Taq polymerase (TaKaRa). Amplification products were run on 0.8% agarose gels and subsequently purified with UNIQ-10 kit (Shanghai Bioengineering). PCR products were sequenced by ABI 3730 at Beijing Genomics Institute (BGI) –Shenzhen.

Although PAL was reported to be a single-copy nuclear gene in C. sinensis, it is possible that lineage-specific duplication occurred in C. taliensis. To exclude the possibility of paralogous loci in C. taliensis, we selected and cloned 15 heterozygous PCR products using pGEM T-easy vectors. For every selected heterozygous PCR product from a single individual, as expected for the amplification of a single locus from a diploid organism, no more than two different alleles were detected. Therefore, it was confirmed that all these haplotypes detected in our data set correspond to the same PAL locus. All sequences reported in this study were deposited in the GenBank database under accession numbers JX161616-JX161644.

Data analyses

Because some of the SNPs used in this study were discovered within close proximity to one another, they could not be treated as independent markers. For each set of linked SNP loci, we employed a Bayesian statistical method implemented in Phase version 2.1.1 [34, 35] to resolve the gametic phase of PAL sequences with multiple heterozygous single nucleotide polymorphisms (SNPs). This program uses allele frequencies and frequencies of known SNP haplotypes in each population to infer the probabilities for each possible haplotype from a group of linked SNPs. A total of five independent runs of 100 iterations each were performed with other parameters as default. The goodness-of-fit values were very similar among different runs, indicating that their run lengths were sufficient in the present study. For each newly ‘phased’ locus, we selected the two haplotypes for each sample that had the highest probability as assessed by PHASE. These haplotypes were then used as multi-allelic genotypes for further analysis. Only those alleles and genotypes resolved with > 95% posterior probabilities were remained for subsequent analyses. Sequences were proofed and aligned by using CLUSTAL _X [36] as implemented in BioEdit [37]. Indels in the cpDNAs were treated as substitutions by following Caicedo and Schaal [2].

Global and population nucleotide diversity (π) [38], haplotype diversity (h), average number of nucleotide differences between the whole sequences (K), and the number of polymorphic sites (S) were calculated using DNASP 4.10 [39]. Tajima's D[40] and Fu & Li's D*[41] neutrality tests were applied to determine whether a locus evolves in a neutral manner. The minimum number of recombination events (RM) was assessed using the algorithm of Hudson and Kaplan [42] in the DNASP 4.10 program.

Nested clade phylogeographic analysis (NCPA) was performed by following the approach [43] in the program ANeCA [44]. Significantly parsimonious connections were then constructed by using the program TCS [45], with a 95% parsimony connection limit. On basis of the resulting network, nested clades were further defined following the rules of Templeton et al. [46] and Templeton & Sing [47]. In the study, the program GEODIS [48] was used to test whether there is geographic associations of clades as well as nested clades or not under the null hypothesis, with a 95% confidence level and with 10,000 permutations. If significant values were detected, the inference key of Templeton [49] was used to explain their likely population processes and/or historical events within these clades.

The approximate divergence times between clades defined by nested clade phylogeographic analysis were estimated following Yuan et al. [50], using T = dA/2 μ,where T is the divergence time and μ is the rate of nucleotide substitution [51]. The net pairwise divergence per base pair (dA) was calculated using MEGA4 [52] under the Kimura two-parameter model [53]. In this study, considering that a substitution rate had not yet been estimated for the cpDNA genome of Camellia, 1.0-3.0 × 10-9 substitutions per site per year for synonymous cpDNA sites in seed plants [24], were taken as a rough evolutionary rate for rpl32-trnL intergenic spacers to date their divergence times.

An analysis of molecular variance (AMOVA) [54] was carried out with Arlequin 3.1 [55] to determine the partitioning of variation within and between populations. Two measures of population differentiation GST and NST were compared by using U-statistic implemented by the program HAPLONST [56]. GST values were estimated by haplotype frequencies, while NST was obtained by considering similarities between haplotypes (i.e. the number of mutations between haplotypes). An NST which is significantly larger than a GST, indicates the presence of a phylogeographical structure with closely related haplotypes being detected more frequently in the same area than remotely correlated ones.

The Mantel test implemented in the program Arlequin 3.1 [55] was applied to examine the correlation between the natural logarithm of the geographical distance and Slatkin's measure M M = (1/FST − 1)/2], a measure of the extent of gene flow under an island model at equilibrium [57]. Statistical significance was also tested with 10, 000 permutation tests by using the program Arlequin 3.1.

Abbreviations

AMOVA:

Analysis of molecular variance

NCPA:

Nested clade phylogeographic analysis

PAL:

Phenylalanine ammonia-lyase

SNP:

Single nucleotide polymorphisms.

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Acknowledgments

This work was supported by National Science Foundation of China (U0936603), Key Project of Natural Science Foundation of Yunnan Province (2008CC016), Hundreds Oversea Talents Program of Yunnan Province, Top Talents Program of Yunnan Province (20080A009), Hundred Talents Program of Chinese Academy of Sciences, and Frontier Grant of Kunming Institute of Botany, CAS to Li-zhi GAO. We are grateful for Ya-Yu Fan, Ting-Zhu, Ping-Zhen Xu, and Yong-Sheng Wu for their assistance with experiments.

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Correspondence to Li-zhi Gao.

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Authors’ contributions

YL collected population samples, generated experimental data, performed the whole data analyses, and drafted the earlier versions of the manuscript. SXY and PZJ involved the field sample collection. LZG designed the study, partially analyzed the data, wrote and revised the manuscript. All of the authors have read and approved the final manuscript.

Yang Liu, Shi-xiong Yang contributed equally to this work.

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12862_2011_2107_MOESM1_ESM.doc

Additional file 1: Table S1. Chain of inference from the nested clade analysis of the chlorotype data in C. taliensis using Templeton’s (2004) inference key. (DOC 30 KB)

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Additional file 2: Table S2. Chain of inference from the nested clade analysis of the PAL haplotype data in C. taliensis using Templeton’s (2004) inference key. (DOC 29 KB)

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Liu, Y., Yang, Sx., Ji, Pz. et al. Phylogeography of Camellia taliensis (Theaceae) inferred from chloroplast and nuclear DNA: insights into evolutionary history and conservation. BMC Evol Biol 12, 92 (2012). https://0-doi-org.brum.beds.ac.uk/10.1186/1471-2148-12-92

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