Sampling

Tissue samples for this study were collected from 2012 to 2014 in the range of S. alpinus. Tissue samples were stored in 96 % ethanol until DNA extraction. The samples comprised 71 individuals from 18 localities, which covers the majority of S. alpinus distribution (Fig. 1). Elaborated material includes Sudetic Mts. (Krkonoše Mts. and Jizerské hory Mts.), the Carpathians, eastern Alps, the Dinaric Mts. (Mt. Snežnik, Šator Mts., Bjelašnica Mts., Zelengora Mts. and Komovi Mts.) and two isolated small ranges: Žd'árské vrchy Mts. situated between Sudetic Mts. and Šumava Mts., and Rhön Mts. in SE Germany (Fig. 1).

Fig. 1.

Extant range of the Alpine shrew (modified from  www.iucnredlist.org) depicted by violet with sampling localities shown by dots.

DNA extraction and sequencing

Genomic DNA was extracted from tissue samples using the commercial DNeasy® Blood and Tissue Kit (Qiagen, Hilden, Germany) according to the manufacturer's instructions. For PCR amplification of the left domain of mitochondrial control region (Fumagalli et al. 1996), primers L15926 (5′TCAAAGCTTACACCAGTCTTGTAAACC3′) from Kocher et al. (1989) and H16498 (5′CCTGAAGTAAGAACCAGATG3′) from Southern et al. (1988) were used. The 25 µl PCR reaction mixtures contained 1× Taq buffer, 2.5 mM MgCl₂, 200 µM dNTPs, 0.5 µM primers, 1 U Taq polymerase (Promega, Madison, WI, U.S.A.) and approximately 50–100 ng of genomic DNA. The temperature profile for 35 cycles of PCR amplification was 3 min at 95 °C (initial denaturation step), 1 min at 95 °C, 1 min at 55 °C (annealing temperature), 1 min at 72 °C, followed by a final extension step of 4 min at 72 °C. The reaction was purified using the QIAquick® PCR Purification Kit (Qiagen) or excised from agarose gel and purified with the QIAquick® Gel Extraction Kit (Qiagen). The purified products were sequenced with forward and reverse primers on the 3130 Genetic Analyzer by Applied Biosystems® using the BigDye® Terminator v3.1 Cycle Sequencing Kit (Applied Biosystems®, Waltham, MA, U.S.A.).

Table 1.

Details of sampling localities and number of sampled individuals.

Data analysis

Amplification and sequencing reactions of mitochondrial control region were successful in 71 individuals of the Alpine shrew. Sequences were compiled in the software Geneious®, version 6.1.8. ( http://www.geneious.com, Kearse et al. 2012). An alignment of the sequences was performed using the online program MAFFT, version 7 (Katoh & Standley 2013), which automatically selects an appropriate algorithm according to the data size (Katoh et al. 2002). From the dataset of 71 samples, 20 samples were excluded due to the poor-quality signal of the PCR product or due to the presence of nuclear copies of the mtDNA (numts) in the targeted DNA fragment. Numts were distinguished from the mtDNA sequences as they formed a clade distant from the rest of the sequences (p-distance ranged from 0.094 to 0.109). The numts also contained indels and lacked geographic variation among localities.

High degree of sequence conservation in d-loop-like nuclear copies, contrasting with rapid mutation rate in mitochondrial d-loop, was ascertained also in other studies (Zhang et al. 2006). Consequently, 51 sequences were used for further phylogeographic analyses as final dataset. Three regions with low consensus values resulting from a large amount of missing data or high degree of sequence polymorphisms consisting of indels were excluded to avoid incorrect identification of homologies. Two regions with low consensus values (56 bp at the 5′ end and 106 bp at the 3′) were excluded because of a large number of missing sequences. One section of 316 bp from the R1 variable region (Fumagalli et al. 1996) was excluded due to occurrence of indels (e.g. Warnow 2012). Alignment (both unedited and edited versions) is accessible at TreeBASE ( http://purl.org/phylo/treebase/phylows/study/TB2:S18503). Locality descriptions and sample sizes are given in Table 1. Sequences were collapsed to haplotypes in DnaSp version 5.10.1 (Librado & Rozas 2009) and the haplotypes were submitted to GenBank (accession numbers: KT725725–KT725775).

Relationships among mitochondrial haplotypes were visualized using a median-joining network implemented in the software NETWORK, version 4.613 (Bandelt et al. 1999). Nucleotide polymorphism and haplotype diversity was calculated in the program DnaSP, version 5.10.1 (Librado & Rozas 2009). Best model of nucleotide evolution of ingroup was evaluated in JModelTest 2.1.7 (Darriba et al. 2012). Bayesian inference analysis implemented in the program MrBayes (Ronquist et al. 2012) was used to reconstruct phylogenetic relationships among haplotypes. Analysis consisted of two runs with four chains (one cold and three heated) and was run for 20000000 generations of Markov Chain Monte Carlo (MCMC) simulations sampled every 100 generations. Bum-in period was set to 25 %. Convergence of the two runs was verified in AWTY (Wilgenbusch et al. 2004). Runs were checked for stationarity and convergence by the cumulative plots that show posterior probabilities of splits at selected increments over an MCMC run, and by the bivariate plot of the split frequencies. Resulting Bayesian tree was edited in program FigTree v1.4.2. ( http://tree.bio.ed.ac.uk/software/figtree/).

Landscape genetic method implemented in R (R Core Team 2015) package Geneland (Guillot et al. 2008) was used to assess the spatial distribution of genetic variability of haplotypes in the dataset. Initially, the analysis was performed five times with 100000 MCMC iterations, a thinning of 100, number of populations (K) varying from K = 1 to K = 10, and with an uncorrelated allele frequency model. Finally, the analysis was re-run for the best K with 1000000 iterations, a burn-in of 100 iterations and a thinning of 1000, other parameters had identical settings. Geneland recognized four groups in our data and these groups were treated separately for calculations of the summary statistics of genetic variability which were computed in DnaSP version 5.10.1 (Librado & Rozas 2009).

The occurrence of isolation by distance (IBD) was tested by calculating correlation between matrices of p-distances and matrices of geographic distances among localities. Matrix of p-distances between sequences was calculated in MEGA 5 (Tamura et al. 2011) and matrices of geographic distances among individuals were estimated in Geographic distance matrix generator 1.2.3. (Ersts 2011). Regression line was calculated using the RMA method (Reduced Major Axis). The significance of the correlation was tested with a Mantel test on Isolation by distance web service V3.23 (Jensen et al. 2005). IBD was tested by plotting the parameter p-distance against the logarithm of geographic distance.

The Bayesian skyline plot (BSP) which was implemented in the software Beast v1.8.2. (Drummond et al. 2012) was used to reveal past changes in population size for the entire dataset as well as for each group obtained in landscape genetic analysis separately. The HKY + G model was selected in jModelTest 2.1.7 (Darriba et al. 2012). Analysis of BSP was conducted with 30000000 iterations of the MCMC simulations three times, strict molecular clock with mutation rate of 1, genealogy and parameters of the model were stored every 1000 iterations and burn-in was set to 10000000 iterations. The convergence of chains was assessed in the program Tracer v1.6.0. (Rambaut et al. 2014). We also estimated changes in population size in the past using the mismatch distribution test implemented in DnaSP. Mismatch distribution test compares the observed frequencies of pairwise differences among sequences with the frequencies expected under demographic models. Statistical evaluation of mismatch analysis was conducted in program Arlequin 3.5.2 (Excoffier et al. 2005).

To further assess whether the species experience past population growth we used summary statistics of genetic variability of sequences, including neutrality tests (Fu and Li's F^*, Fu and Li's D^*, Fu's F's and Tajima's D), computed in DnaSP and Arlequin.

Fig. 2.

Bayesian tree based on 41 haplotypes of Sorex alpinus. Colours correspond to the results of the tesselation map from Geneland (Fig. 4). Numbers at nodes indicate posterior probabilities. Sample codes correspond to those in Table 1.

Fig. 3.

The median-joining network of 41 haplotypes of Sorex alpinus. The size of the circle is proportional to the frequency of the haplotype in the dataset, colour codes represent the geographic origin. Small red dots represent hypothetical haplotypes not found in our sample. Haplotypes from isolated populations at Žd'árské vrchy (CZ-KR) and Rhön Mts. (DE-RH1, DE-RH2), and the CZ-OD5 haplotype (shared by four individuals) are labeled. Numbers at branches represent numbers of mutational steps (displayed for n > 1).

Fig. 4.

Tesselation map illustrating spatial distribution of genetic variability for K = 4, inferred by software Geneland. Black dots represent sample sites. The first (white) group comprises populations from the north-western part of the species range (Sudetic Mts.). Second group (green) comprises populations occurring in the southwestern part of the area (Eastern Alps and Northern Dinarids). The third group (yellow) consists of populations from the southern Dinarids. Fourth group (orange) contains populations from the east part of the species range (the Carpathians).

Large population in lower altitudes during glacial period

In this study, we provide information about phylogeographic structure of the Alpine shrew, which occurs in the “Alpine archipelago” without long distance disjunctions (Schmitt 2009). We found low differentiation in mitochondrial DNA with evolution of site-specific haplogroups. This pattern contrasts with other soricid species associated with high mountain systems, where deeply divergent genetic lineages were ascertained in habitat islands. For example, allopatric differentiation likely occurred among clades of Sorex bedfordiae species complex, inhabiting high mountain systems in southeastern part of Tibetan Plateau (Chen et al. 2015). Allopatric differentiation of this species is connected with sky island pattern, facilitated by isolation of particular mountain ridges by large river valleys. In contrast, shallow phylogeny of S. alpinus with lack of deep endemic branches implies relatively rapid and recent differentiation from an ancestral population. Similar patterns were determined in several clades of other soricids preferring intermediate elevations as in Sorex monticolus species complex inhabiting the Rocky Mountains and adjacent regions in western North America (Demboski & Cook 2001, Himes & Kenagy 2010) or Sorex cinereus in the Appalachians in eastern North America (Sipe & Browne 2004).

The climatic conditions of glacial periods included both cooling and desiccation of the environment with respect to the inter-glacial periods. Temperature drop resulted in altitudinal shifts of communities. It is likely that during glacial peaks, species that recently avoid habitats above 2500 m a.s.l. occurred ex situ with respect to the current distributional range, that is, in lower altitudes. Drying of the climate caused reduction of the forested area and spread of semi-open and open habitats. Species that exhibit low dispersal abilities and relatively narrow ecological niches likely respond to the climatic oscillations of the Pleistocene by altitudinal shifts rather than long distance movements. For these species, refugia of the coniferous mountain forest, restricted to the foothills of glaciated high mountain systems (Schmitt & Haubrich 2008), may represent suitable conditions. However, existence of multiple centers of glacial survival often results in evolution of two or more deeply separated lineages, which is not the case of S. alpinus. Therefore, we presume that S. alpinus was fairly continuously distributed during the last glacial period. The phylogeographic pattem of shallow divergences among haplotypes corroborates the hypothesis that the glacial range was more extensive than the current one. This perspective is also supported by demographic characteristics. For example, the BSP shows that the population size culminated before recent. However, the bi-modal mismatch distribution could indicate different demographic scenario in different parts of the range. For example, BSP for the Alps shows population growth in recent past, probably concordant with the current interglacial period. This result corroborates our hypothesis about shift of the species to lower altitudes during glacial period. As the Alps were covered with massive glacier during LGM, the ecological conditions of the region were probably not suitable for the species in this time. Nevertheless, evolution of the semifossorial niche in the Alpine shrew is also consistent with the scenario of a more continuous range during the last glacial period, as this species is capable utilizing different depths in the scree habitats which in turn might have helped stenoecious organisms to survive during glacial periods.

Although the distribution of S. alpinus is relatively continuous, gaps within its range exist between the Alps and the Dinarids and between the Sudetes and the Carpathians, with Danube representing the zoogeographical barrier. In both cases, similar genetic lineages inhabit habitat islands on neighboring mountains. This further supports our conclusion that S. alpinus exhibited continuous population during the latest glacial period which was subsequently fragmented and shifted to higher altitudes (Schmitt 2009).

In addition to the high mountain systems of the Alps and Carpathians, the space of Central Europe contains numerous middle high mountains which still host glacial relict populations (Schmitt 2009), including S. alpinus. It is likely that these mountains and adjacent areas with lower altitudes could play substantial role in Vistulian glacial range of S. alpinus. Similar phylogeographical structure to that observed in S. alpinus was ascertained in many other montane organisms. For example, the distribution of the butterfly Erebia epiphron includes the high mountain systems (Alps, Pyrenees) and many isolated range islands in moderate altitudes, including Krkonoše Mts. and Jeseníky Mts. in Central Europe and this species exhibits striking genetic similarity between Jeseníky and some Alpine lineages (Schmitt et al. 2006). Further sampling in southwestern part of the Alpine shrew range will be necessary, however, to fully resolve this issue. It would also be very interesting to examine museum samples from the Pyrenean region where the Alpine shrew is now probably extinct (Mitchell-Jones et al. 1999).

Range breakup in interglacial period and formation of relict enclaves

Moderate diversification and evolution of shallow site-specific genealogy corroborates the hypothesis that the range of S. alpinus became reduced and fragmented during the latest interglacial period. The process of fragmentation of the species suitable habitat was probably gradual. During the Atlantic period of the current interglacial, humid climate was typical for most of the area of Central Europe and contributed to the formation of the closed woodland. Humid environment and presence of closed woodland represent one of the most important habitat requirements of the Alpine shrew (e.g. Kratochvíl & Grulich 1950, Spitzenberger 1978, 2001). Therefore, we believe that suitable habitats for the Alpine shrew existed also outside the extant range. Anthropogenic deforestation of many regions in lower altitudes in Epiatlantic (Horáček & Ložek 1988) might have further facilitated isolation of suitable habitat patches of many glacial relicts, including the Alpine shrew.

Our landscape genetic analyses supported the four cluster model, corresponding with major European high mountain systems. This model fits well with the classical subspecific division of the species, i.e. alpinus in the Alps, hercynicus in Sudetic Mts. and tatricus in the Carpathians (Spitzenberger 1990); populations from the southern Dinarids still lack a subspecific status. Phylogeographic links between high mountain systems and the hilly regions between them were described in many species (Schmitt 2009). The small isolated enclaves of Alpine shrews in discrete hills (Rhön, Žd'árske vrchy) do not show a genetic signal of rapid evolution of distinct lineages. Consequently, there is no evidence for peripatric model. Nevertheless, analysis of fast evolving nuclear loci (i.e. SNPs or microsatellites) will be necessary to describe in more detail the recent population genetic structure of currently isolated populations.