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PLOS ONE logoLink to PLOS ONE
. 2015 Apr 17;10(4):e0121732. doi: 10.1371/journal.pone.0121732

Exploring the Genetic Signature of Body Size in Yucatan Miniature Pig

Hyeongmin Kim 1,, Ki Duk Song 2,, Hyeon Jeong Kim 3, WonCheoul Park 1, Jaemin Kim 4, Taeheon Lee 1, Dong-Hyun Shin 1, Woori Kwak 4, Young-jun Kwon 4, Samsun Sung 3, Sunjin Moon 1, Kyung-Tai Lee 5, Namshin Kim 6, Joon Ki Hong 7, Kyung Yeon Eo 8, Kang Seok Seo 9, Girak Kim 1, Sungmoo Park 1, Cheol-Heui Yun 1, Hyunil Kim 10, Kimyung Choi 10, Jiho Kim 10, Woon Kyu Lee 11, Duk-Kyung Kim 2, Jae-Don Oh 2, Eui-Soo Kim 12, Seoae Cho 3, Hak-Kyo Lee 2,*, Tae-Hun Kim 5,*, Heebal Kim 1,3,*
Editor: Norman Johnson13
PMCID: PMC4401510  PMID: 25885114

Abstract

Since being domesticated about 10,000–12,000 years ago, domestic pigs (Sus scrofa domesticus) have been selected for traits of economic importance, in particular large body size. However, Yucatan miniature pigs have been selected for small body size to withstand high temperature environment and for laboratory use. This renders the Yucatan miniature pig a valuable model for understanding the evolution of body size. We investigate the genetic signature for selection of body size in the Yucatan miniature pig. Phylogenetic distance of Yucatan miniature pig was compared to other large swine breeds (Yorkshire, Landrace, Duroc and wild boar). By estimating the XP-EHH statistic using re-sequencing data derived from 70 pigs, we were able to unravel the signatures of selection of body size. We found that both selections at the level of organism, and at the cellular level have occurred. Selection at the higher levels include feed intake, regulation of body weight and increase in mass while selection at the molecular level includes cell cycle and cell proliferation. Positively selected genes probed by XP-EHH may provide insight into the docile character and innate immunity as well as body size of Yucatan miniature pig.

Introduction

Pigs (Sus scrofa domesticus) were domesticated from Eurasian wild boars approximately 10,000–12000 years ago [1,2]. They have been domesticated in a wide variety of environmental conditions, and are currently found all over the world. Due to their tendency to grow and reproduce quickly, they are most often raised for human consumption and have become one of the main sources of protein for humans. To this end, swine breeds widely used in the livestock industry have been selected for traits of economic importance including average daily weight gain, longissimus muscle area, backfat thickness, and intramuscular fat content [3], and large body size. On average, swine breeds grow to be 4.8 kg at 3~4 weeks, 17.6 kg at 2.1~2.4 months, 53kg at 3.6~4.3 months, and 111kg at 6~8.3 months [4]. Duroc pigs known for its rapid growth rates, grow up to roughly 30kg by 10 weeks, 70kg by 16 weeks and 105kg by 22 weeks [5]. Similarly, Yorkshire pigs grow up to 29 kg by 10 weeks, 52.4 kg by 15 weeks and 82.6 kg by 20 weeks [6]. According to the Korea National Park Service, Korean wild boars are around 200kg when they are fully grown. It was reported that young male wild boar of 1.5 year age and 70 kg, female wild boars of 3~4 year age and 120~150 kg and male wild boars of 3~4 year age and 150~300 kg were observed at the town by local news journals in Korea.

Yucatan miniature pigs (YMP), however, grow slowly and even when fully grown are smaller than other pig breeds. The mean body weight of YMP is 31kg at 8 months and 83 kg at 24 months. (S1 Table). YMP have been bred from a naturally small breed, which was domesticated in the hot and arid Yucatan peninsula. It was imported into the United States in 1960 and since then, has been selected specifically for small body size for laboratory use and called YMP [7]. In 1970s and 1980s, they were studied at Colorado State University and were found to have distinct traits such as gentleness, intelligence, resistance to disease, and relative lack of odor [7,8,9]. For these characteristics, in addition to their size, YMP are used as laboratory animals worldwide.

Changes in the environment can act as a selective pressure and lead to the selection of organisms that are best suited for the new environmental conditions. In the case of domestic animals, selective pressure occurs as a combination of both natural selection (survival and reproductive ability in an enclosure) and artificial selection (intentional breeding by humans) [10]. These selective pressures have cherry-picked animals that have visibly higher fitness and led to the proliferation of these animals in the population. As the mutation that confer this higher fitness increases in frequency within the population, standing genetic variation at or near the mutation are either eliminated or reduced [11]. This process is known as a “selective sweep” and we can expect to find mutations affecting phenotypic traits by investigating regions of the genome with reduced variability or lack of standing variation. By comparing the YMP genome to other large swine breeds, signatures of selection specific to body size may be detected.

The aim of this study is to find genetic signatures of selective sweep in YMP using whole genome sequencing data of YMP, and other large pig breeds (Yorkshire, Landrace and Duroc). Whole genome sequencing data of 60 pigs were analyzed by the population statistic Cross Population Extended Haplotype Homozygosity (XP-EHH) to investigate the genetic characters of YMP, which derived from recent and artificial selection [12,13].

Results

Basic features about re-sequencing data of 70 pigs

In this study, 198,396,895 reads of average read counts were generated (from 148,854,532 reads to 335,518,129 reads) from re-sequencing of 70 pigs, which had 100 bp or 101 bp of planned read length, 406 bp of average distance between the paired reads (from 279 bp to 478 bp) and 44.2 bp of standard deviation of average distance (from 22.5 bp to 87.6 bp). Of total reads, 88 percent of reads were mapped to the reference genome (from 80.95% to 90.79%) (S2 Table). The reads covered 88 percent of genome (from 83.15% to 88.84%), and the sequencing data had average depth of 11.63 (from 4.93 to 15.08) nucleotides for the sequenced region and 10.26 (from 4.25 to 13.39) nucleotides for the whole genome region (S3 Table). For each swine sample, 6,625,510 SNPs were called averagely, and 29,368,693 SNPs were called in total (S2 and S4 Tables). SNP density of 106-bp non-overlapping window for each swine breed is shown in S1 Fig.

Nucleotide diversity of 107-bp non-overlapping window was calculated, and π value and its cumulative average for each swine breed are shown in Fig 1A and 1B. Fig 1C shows pairwise π values between YMP and other swine breeds from Fig 1A. YMP had the lowest nucleotide diversity and Wild boar had the highest nucleotide diversity among 5 swine breeds.

Fig 1. Nucleotide diversity (A and C) and cumulative average of nucleotide diversity (B) for each swine breed.

Fig 1

Nucleotide diversity of 107-bp non-overlapping window is shown. Each pig breed is marked by a colored line; orange for wild boar, blue for Landrace, green for Yorkshire, purple for Yucatan miniature pig and yellow for Duroc.

Phylogenetic tree, population admixture and principal component analyses

To assess the phylogenetic relationship among the pig breeds, we constructed an unrooted phylogenetic tree of 70 pigs based on pairwise identity-by-state (IBS) distance from the information of all autosomal SNPs. All individuals were grouped into five separate pig breeds as expected (Fig 2). Wild boars had the greatest genetic distance from the other breeds, followed by YMP with the next largest distance from Yorkshires, Landraces, and Durocs. Yorkshires and Landraces were genetically closer to each other than any other two breeds.

Fig 2. Unrooted phylogenetic tree of 70 pigs based on pairwise identity-by-state (IBS) distance from the entire autosomal SNPs.

Fig 2

Each pig breed is marked by a colored circle; orange for wild boar, blue for Landrace, green for Yorkshire, purple for Yucatan miniature pig and yellow for Duroc. Scale bar indicate distance measure between each individual (1-IBS).

The estimated population admixture in the 70 analyzed pigs is shown in S2 Fig. We found that the five pig breeds were clearly distinguished when we assumed that the number of population (K) is 6. However, Yorkshire and Landrace shared components with each other.

Similar to the result of the unrooted phylogenetic tree, principal component analysis (PCA) scatter diagram showed clear division among the breeds with a similar pattern of distances between the groups (S3A and S4 Figs). Furthermore, Yorkshires and Landraces were not clearly distinguished in the PCA analyses whether it was conduct with all swine breeds or separately with the two breeds (S3B Fig).

Signature detected by XP-EHH

The signatures of selection were identified based on a population comparison by the Cross Population Extended Haplotype Homozygosity (XP-EHH) test, which was devised to detect ongoing or nearly fixed selective sweeps by comparing haplotypes from two populations [14,15]. To get XP-EHH values, Extended Haplotype Homozygosity (EHH) and the log-ratio integrated EHH (iHH) were calculated using haplotype information of autosomal SNPs identified in the study. XP-EHH tests were performed in pairwise comparison between YMP and each of the large pig breed (Duroc, Landrace and Yorkshire). XP-EHH values are directional: extreme positive values imply selection in YMP while negative values suggest selection in other breed used in comparison. The distribution plot of raw XP-EHH values between YMP and other swine breeds is shown in S5 Fig. XP-EHH values have normal distribution.

For each comparison, we split the autosome into non-overlapping segments of 50 kb and the highest XP-EHH value was used as summary statistic for each window. Then the segments were grouped into 4 clusters according to their number of SNPs to take SNP frequency into account. For each cluster, empirical p-values of < 0.01 were used as cut off values to select significant regions in YMP. Under the assumption that the genes located within boundary of these regions are also outlier loci (genes), we selected genes associated with outlier loci (regions).

By XP-EHH test, we identified a total of 390 outlier regions and 429 associated genes in YMP from three comparative analyses: 164 regions (184 genes), 137 regions (146 genes), and 181 regions (196 genes) when compared to Duroc, Landrace, and Yorkshire, respectively (S7 Fig). There were 14 regions and 14 genes, which were detected by all three XP-EHH analyses. XP-EHH values, p-values and associated genes of outlier loci (regions) are shown in S5 Table.

For outlier loci (genes) in each comparison, we performed Gene Ontolgy (GO) term enrichment analyses with EASE < 0.05 to investigate their representation of functional groups (Fig 3). There were 45 enriched GO terms in all three comparisons. To reduce GO term list to the most relevant terms, we picked up representative GO terms based on the list of genes involved in. Representative GO terms associated with genes located in outlier loci (regions) detected by XP-EHH are shown in Table 1. The outlier loci (genes) between YMP and Duroc were mainly associated with detection of fungus, sensory perception of smell, ion transport, protein amino acid phosphorylation, cell proliferation, microtubule-based process and cell cycle in GO term. The outlier genes detected between YMP and Landrace were mainly associated with neuron fate commitment, response to organic substance, transcytosis, sensory perception of smell, regulation of cyclase activity and neurological system process. The outlier genes detected between YMP and Yorkshire were mainly associated with glutamate signaling pathway, vesicle-mediated transport, regulation of cell migration and learning. Nucleotide diversity plot of 14 genes in the intersection of all three XP-EHH analyses and 5 genes of interest which are known for their relation to growth is shown in S8 Fig.

Fig 3. Hierarchical clustering of biological process GO terms associated with genes located in outlier loci (regions) detected by XP-EHH method in comparisons between Yucatan miniature pig and Duroc (A), Landrace (B) and Yorkshire (C).

Fig 3

The gene list of each GO term clustered using DAVID was compared to calculate the distance between the GO terms. For a distance value of > 0.4~0.5, GO terms were re-clustered, and GO term groups are shown in boxes. The representative GO terms manually selected are shown in red. The numbers of genes in the GO terms are in brackets with the corresponding p-values.

Table 1. Representative biological process GO terms associated with genes located in outlier loci (regions) detected by XP-EHH method.

Comparison Biological process GO term (No. of genes)
YMP vs Duroc detection of fungus (2)
sensory perception of smell (10)
ion transport (13)
protein amino acid phosphorylation (12)
cell proliferation (9)
microtubule-based process (7)
cell cycle (16)
YMP vs Landrace neuron fate commitment (3)
response to organic substance (11)
transcytosis (2)
sensory perception of smell (8)
regulation of cyclase activity (5)
neurological system process (17)
YMP vs Yorkshire glutamate signaling pathway (3)
vesicle-mediated transport (13)
regulation of cell migration (7)
learning (4)

Discussion

Phylogenetic tree, population admixture and principal component analyses

Before investigating selection signatures, we first assessed the phylogeny of the pig breeds to evaluate the phylogenetic position of YMP within the species (Fig 2). An unrooted phylogenetic tree of 70 pigs identified clear division among the five pig breeds, as expected. Phylogenetically, YMP was distant from the wild boar group while being relatively close to Landrace, Yorkshire and Duroc groups. Wild boar had the greatest distance from the other breed groups. The distance between groups was concordant with previously reported phylogenetic trees, which were constructed by using neighbor-joining clustering and the unweighted pair group method with the arithmetic mean from microsatellite markers [16].

The distance pattern between the swine breeds was also identified by PCA (S3 and S4 Figs). However, Yorkshire and Landrace were not clearly distinguishable in either the PCA conducted with the five breeds or in a separate PCA of Yorkshire and Landrace, indicating the possibility of shared genetic components between the two breeds (S2 Fig). In the PCA of the two breeds, multiple eigenvectors accounted for similar proportion (5%) of the total variance in the genetic relationship matrix, limiting the power to stratify the two pig breed populations. This indicates that stratification using IBS is more sensitive than multiple eigenvectors.

Signature detected by XP-EHH

For investigating recent selective sweep, we calculated XP-EHH values for YMP and other large swine breeds. XP-EHH tests were performed in pairwise comparison between YMP and each of the large pig breed that shows body size difference clearly (Duroc, Landrace and Yorkshire). XP-EHH statistic estimates haplotype differences between two populations and detects selective sweeps at or near fixation in one or the other population [13]. Thus, we expected being able to unravel the signatures of selection of body size in YMP.

The genes identified as being positively selected for in YMP are shown in S5 Table and the biological process GO terms associated these genes are shown in Fig 3. Representative GO terms from Fig 3 are shown in Table 1. According to GO term enrichment test results, the genes related to ‘cell proliferation’, ‘microtubule-based process’ and ‘cell cycle’ in comparison between YMP and Duroc (Fig 3A) could be involved in the growth and body size of YMP. Their function in regulation of cell cycle, cell division and cell proliferation are expected to affect the growth of YMP at the cellular level. The genes related to ‘response to organic substance’ and ‘transcytosis’ in comparison between YMP and Landrace (Fig 3B), and ‘vesicle-mediated transport’ and ‘regulation of cell migration’ in comparison between YMP and Yorkshire (Fig 3C) also could be involved in the growth and body size of YMP. Their roles involved in the process of change of cellular activity caused by stimulus of carbon containing molecule, transporting molecule across cell membrane and cellular component movement are important. They represent metabolism and increase or decrease of cellular component, and they are closely related to the regulation of cell cycle and cell proliferation, which could affect the growth of YMP at the cellular level.

We identified outlier loci (gene) TGFB2 in comparison between YMP and Landrace, and between YMP and Yorkshire. The TGFB2 gene (transforming growth factor, beta 2) encodes a member of the transforming growth factor beta (TGFB) family of cytokines, which has multiple functions, such as regulation of proliferation, differentiation, adhesion and migration [17]. TGF-betas are known to have critical roles in growth regulation and development, and have been studied extensively [18].

In Table 1 and Fig 3, the GO term, ‘sensory perception of smell’ was also enriched, suggesting a possible link between the senses and body size. Pigs are incredibly sensitive to smell, and adding garlic to feed as sweetener or modifying cereal inclusion rate has been shown to affect the palatability of meals which results in differences in the growth and meat producing performance [19,20].

The GO term ‘growth’ is defined as the increase in size or mass of an entire organism, a part of an organism or a cell. Therefore, genes detected by XP-EHH method and identified as being involved in growth term were thought to be related to the body size of YMP at the cellular level or at the level of organism. In all comparisons, we found 4 genes detected by XP-EHH and related to the ‘growth’ term, which are APP, ACVR2B, PLEKHA1 and CD 38 genes. APP (Amyloid Beta (A4) Precursor) gene encodes specific kind of cell surface receptor and transmembrane precursor protein, which are amyloid beta proteins and it is known as being genetically linked to familial Alzheimer’s disease. It was reported that APP knockout mice weighed 15%-20% less than wild-type mice [21]. ACVR2B (Activin Receptor Type-2B; Act RIIB) gene is a myostatin-related gene involved in the regulation and signaling of myostatin [22]. Transgenic mice expressing dominant-negative form of Act RIIB had increased muscle mass up to 125% more than those of control mice. Also, there was a study that haplotype structure at Act RIIB could explain the interindividual variation in skeletal muscle mass and strength in human [23]. PLEKHA1 (Pleckstrin Homology Domain Containing, Family A (Phosphoinositide Binding Specific) Member 1) gene, also known as TAPP1, encodes a pleckstrin homology domain-containing adapter protein, which is localized to the plasma membrane of cell. This encoded protein has been studied for its role in regulating downstream of growth factor stimulation [24]. CD38 gene is a multifunctional ectoenzyme widely expressed in cells and tissues. It was shown to be involved in regulating a wide variety of signaling pathways, such as those that regulate metabolism [25]. In the study of Barbosa et al. [26], CD38 knockout mice had a higher metabolic rate compared to wild-type mice, and were protected against high-fat diet-induced obesity. The role of CD38 was demonstrated as a regulator of body weight.

These genes involved in the biological process GO terms are not master gene such as IGF1, BMP2 or GH1 that directly affect body size as previously reported in mouse [27], dog [28], goat [29], pig [30] and human [31]. However, the genes identified in the study as having signatures of selection detected by XP-EHH method are related to the growth and body size. Thus, we found that genetic changes from the cellular level to the organismal level occurred in the evolutionary history of Yucatan Miniature Pig. However we could also find that the genes identified as being positively selected for in YMP are involved in neurological system and innate immunity.

Outlier loci (genes) (PARK2, APP, CTNND2 and DRD5) were enriched for the GO term ‘learning’ in comparison between YMP and Yorkshire (Table 1 and Fig 3). In GO term, ‘learning’ means any process in an organism in which a relatively long-lasting adaptive behavioral change occurs as the result of experience. These involved genes are also related to the GO term ‘behavior’, which is defined as the specific actions or reactions of an organism in response to external or internal stimuli. In comparison between YMP and Landrace, the GO term ‘neurological system process’ was enriched, and GRM5 (Glutamate Receptor, Metabotropic 5) gene was detected by all three XP-EHH analyses, which is one of the major genes of neurotransmission in central nervous system. This may affect intelligence or behavioral response to stimuli of YMP. Selection signatures in ‘learning’ and ‘neurological system process’, these indicate that the docile character of YMP might have evolved in the history of domestication.

Among 14 genes in the intersection of all three XP-EHH analyses, 5 genes were identified as being involved in innate immunity, which are ITLN2, CLEC7A, OLR1, GABARAPL1 and SH3BP2 (Table 2). ITLN2 (Intelectin 2) gene has no known function yet. However, it has an important paralog ITLN1, which may play a role in the defense system recognizing bacterial cell wall [32], and ITLN2 may play a role in the defense system by its sequence similarity. CLEC7A (C-Type Lectin Domain Family 7, Member A) gene encodes a member of C-type lectin/C-type lectin-like domain superfamily. It functions as a receptor that recognizes cell wall components of pathogenic bacteria and fungi, and many immune cells such as natural killer cells, macrophages and dendritic cells have this type of receptor and play important roles in the innate immune response [33]. OLR1 (Oxidized Low Density Lipoprotein (Lectin-Like) Receptor 1) gene, also known as LOX1 (lectin-type oxidized LDL receptor 1), also encodes a low density lipoprotein receptor that belongs to the C-type lectin superfamily, and it is thought to be involved in inflammatory response and antigen cross-presentation [34,35]. GABARAPL1 (GABA(A) Receptor-Associated Protein Like 1) gene is involved in formation of autophagosomal vacuoles [36] and SH3BP2 (SH3-Domain Binding Protein 2) gene has important function in regulating T-cell activation, natural killer cell activation and mast cell activation [37]. The result that these important immune related genes were found by all three XP-EHH analyses, indicates that innate immunity of YMP might have been changed in the evolutionary history.

Table 2. Outlier regions detected by all three XP-EHH tests between Yucatan miniature pig and each of large swine breed (Duroc, Landrace and Yorkshire) and associated genes.

Chromosome Position start Position end Number of SNPs XPEHH between YMP and Duroc p-value of XPEHH between YMP and Duroc XPEHH between YMP and Landrace p-value of XPEHH between YMP and Landrace XPEHH between YMP and Yorkshire p-value of XPEHH between YMP and Yorkshire Associated gene
4 97600000 97650000 790 3.73274 0.0039032 3.84921 0.0090749 4.28436 0.0050742 ITLN2
5 32200000 32250000 885 4.13872 0.0009758 3.85147 0.0086846 5.0409 0.0002927 TBC1D30
5 64550000 64600000 936 4.11254 0.0010734 4.53552 0.0013661 4.8002 0.0005855 CLEC7A,OLR1
5 64600000 64650000 148 2.56887 0.0082842 3.80914 0.0015907 3.19335 0.0081511 GABARAPL1
8 1150000 1200000 763 3.60337 0.0054645 4.26101 0.003025 4.39272 0.0031226 SH3BP2
8 5900000 5950000 754 3.61304 0.0053669 4.2187 0.0034153 4.05338 0.0083919 ZNF518B
9 24500000 24550000 985 4.05559 0.0014637 5.08135 9.76E-05 4.6132 0.0012685 GRM5
10 9850000 9900000 656 3.20103 0.0049394 3.94388 0.0036257 4.1702 0.0020004 SPATA17
10 9900000 9950000 1348 3.60608 0.0085831 4.67026 0.0037824 4.89801 0.002764 SPATA17
12 62550000 62600000 96 2.71247 0.0054344 3.80487 0.0016569 4.05116 0.0010603 ALDH3A2
13 20250000 20300000 793 3.82096 0.0029274 4.68363 0.0004879 4.2517 0.0056596 CMTM6
15 14900000 14950000 912 3.46727 0.0073185 3.95373 0.0066354 4.29819 0.0046838 U6
15 50000000 50050000 303 2.80518 0.004374 3.72619 0.0021209 3.55649 0.0035785 7SK
17 9650000 9700000 236 2.65267 0.0063623 4.60263 0.0001326 4.70793 0.0002651 HGSNAT

Thus, we could find the selection signatures involved in growth, body size, docile character and innate immunity of YMP using XP-EHH. Therefore, we suggest that the evolution in body size of YMP at the level of organ and organism, including feed intake, regulation of body weight and increase in mass of entire organism, and at the cellular level, including cell cycle and cell proliferation occurred during domestication process started about 10,000 years ago. We also suggest that the evolution related to docile character and innate immunity of YMP occurred simultaneously.

Materials and Methods

Sample preparation and whole genome re-sequencing

For the pigs experiment, the study protocol and standard operating procedures were reviewed and approved by the National Institute of Animal Science's Institutional Animal Care and Use Committee, Suwon, South Korea (approval No. 2009–077, C-grade, experiment for Landrace, Yorkshire and wild boar) and Seoul National University Institutional Animal Care and Use Committee, Seoul, South Korea (approval No. SNU-130527-8, experiment for Yucatan miniature pig,).

We used next generation sequencing data of 15 Yorkshires, 13 Landraces, 10 wild boars, 20 Durocs and 12 Yucatan miniature pigs to total 70 individuals.

For the different pig breeds, either blood or muscle samples were obtained for DNA extraction. Blood samples were collected from Landraces (seven male, six female) and Large Whites (seven male, eight female) from the National Institute of Animal Science, Korea. Blood (10 ml) was drawn from the carotid artery and was treated with heparin to prevent clotting. Muscle samples were collected from three male and seven female wild boars from the Southern part of Korea. For these samples, 3 μg of genomic DNA was randomly sheared using the Covaris System to generate ~300-bp inserts. The fragmented DNA was end-repaired using T4 DNA and Klenow polymerases, and Illumina paired-end adaptor oligonucleotides were ligated to the sticky ends. We analyzed the ligation mixture by electrophoresis on an agarose gel, and then purified the fragments. The purified DNA library was sequenced using the HiSeq2000 (Illumina, Inc). Clusters of PCR colonies were then sequenced on the HiSeq2000 platform using the manufacturer-recommended protocols.

Muscle samples from twenty male Durocs raised at a pig breeding company (Suncheon, Korea) were collected from a local slaughter house and YMP blood samples were collected from twelve females at a local laboratory pig distributor (Optipharm, Inc). Genomic DNA was extracted and a quality check was carried out using fluorescence-based quantification on an agarose gel, a standard electrophoresis on a 0.6% agarose gel and, via a pulsed-field gel, using 200 ng of DNA. Manufacturers’ instructions were followed to create a paired library of 500-bp fragments. This consisted of the following: purified genomic DNA fragments of less than 800 bp, fragments with blunt ends, fragments with 5′ phosphorylated ends, fragments with a 3′- dA overhang, some with adaptor-modified ends, purified ligation product, and a genomic DNA library. Following this, we generated sequence data using HiSeq2000.

Using the Burrows-Wheeler Aligner [38] with default settings, pair-end sequence reads were mapped to the reference pig genome (Sscrofa10.2). We used open-source software packages: Picard Tools, SAMtools [39], and the Genome analysis toolkit [40] for downstream processing and variant calling. Substitution calls were made with GATK UnifiedGenotyper [41] and all calls with a Phred-scaled quality of less than 20 were filtered out. For each chromosome, we simultaneously inferred the phased haplotype and imputed the missing alleles for the entire set of pig populations using BEAGLE [42]. Nucleotide diversity of 107-bp non-overlapping window for each swine breed was calculated using PLINK [43].

Estimation of phylogenetic tree and admixture in porcine population, and principal component analysis

Using GATK BeagleOutputToVCF [41], BEAGLE output files of each chromosome were converted to Variant Call Format (VCF) files. Then, the VCF files of autosome were converted to PLINK [43] input files using VCFtools [44]. From the information of all autosomal SNPs, population stratification was estimated using PLINK, which uses complete linkage agglomerative clustering based on pairwise identity-by-state (IBS) distance. In terms of IBS, there are three states between two individuals: 0, 1, or 2 shared alleles at a given locus. Symmetric matrix of IBS for all pairs of individuals was made, and these values ranged from 0 to 1, in which twin pairs had a value of 1. A distance matrix (1-IBS) for all pair of individuals was used to estimate a phylogenetic tree by neighbor-joining method [45]. Figures of the neighbor-joining trees were drawn using FigTree [46] (version 1.40).

Population admixture was investigated using STRUCTURE [47] (version 2.3.4), which carries out a model-based clustering method using genotype data. Due to limited computational power, we selected one out of every fifty SNPs to construct the STRUCTURE input file, and the population structure was estimated based on an admixture model.

Using the information of all autosomal SNPs, genetic relationship matrix (GRM) between pairs of individuals was estimated and principal component analysis (PCA) was performed by GCTA [48]. GCTA calculates eigenvectors, which are equivalent to those of EIGENSTRAT [49].

Estimation of XP-EHH value and outlier loci detection

To detect selective sweep, Cross Population Extended Haplotype Homozygosity (XP-EHH) was calculated using the software xpehh [14] (http://hgdp.uchicago.edu/Software/).

For pairwise comparison of the Yucatan miniature pig and other large swine breed populations (Duroc, Landrace and Yorkshire), we used haplotype information of SNPs from the entire autosome to calculate Extended Haplotype Homozygosity (EHH) and the log-ratio integrated EHH (iHH). The distribution plot of raw XP-EHH values between YMP and other breeds is shown in S5 Fig. Then we split the autosome into non-overlapping segments of 50 kb and picked up the highest XP-EHH value as summary statistic for each window. The reason why we applied a maximum for XP-EHH to detect selection signature in YMP is that the XP-EHH values are directional: positive values imply selection in YMP while negative values suggest selection in other swine populations. To avoid bias towards windows have high SNP frequency in selecting significant windows, we grouped segments into 4 clusters according to their number of SNPs in increments of 350 SNPs (0 < cluster 1 < 350, 349 < cluster 2 < 700, 699 < cluster 3 < 1050 and 1049 < cluster 4). The number of SNPs in each window is shown in S6 Fig. Within each cluster, for each window i, the fraction of windows with a value of the statistic greater than that in i is defined as the empirical p-value, following the method previously reported [13,50,51]. We then chose the regions with empirical p-value < 0.01, which were considered to have strong signals in YMP. Genes related to these regions were determined by identifying genes located within boundary of regions.

In this study, empirical p-values were used as there are uncertainties in the demographic parameters making the use of p-values based on demographic models unreliable. A low empirical p-value for a locus implies that the locus is an outlier in comparison to the rest of the sampled loci in the genome. It has been reported that the use of empirical p-values has a tendency to under-represent the truly selected loci, especially when it comes to selection on standing variation and recessive loci [52].

Gene ontology terms enrichment tests

The porcine Ensembl gene annotation (Ensembl Genes 78) and associated gene symbols were used for functional clustering and enrichment analyses using the Database for Annotation, Visualization and Integrated Discovery (DAVID) [53]. The representation of functional groups in Yucatan miniature pig relative to the whole genome was investigated using the Expression Analysis Systematic Explorer (EASE) tool [54] within DAVID. EASE is a modified Fisher’s exact test used to measure enrichment of gene ontology (GO) terms [55].

GO term enrichment tests were performed using EASE with a cut-off value of <0.05 for the outlier loci (genes) associated with XP-EHH.

Ethics Statement

For the pigs experiment, the study protocol and standard operating procedures were reviewed and approved by the National Institute of Animal Science's Institutional Animal Care and Use Committee, Suwon, South Korea (approval No. 2009–077, C-grade, experiment for Landrace, Yorkshire and wild boar) and Seoul National University Institutional Animal Care and Use Committee, Seoul, South Korea (approval No. SNU-130527-8, experiment for Yucatan miniature pig,).

Supporting Information

S1 Fig. SNP density plot of 70 pigs.

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S2 Fig. Proportion of membership of 70 pigs into each of the five different breeds showing population admixture.

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S3 Fig. PCA scatter diagram showing the relative position of the five pig breeds (A) and the two closely related Yorkshire and Landrace breeds (B), defined by eigenvectors based on genetic relationship matrix from all autosomal SNPs.

Eigenvector 1 and 2 accounted for 19 and 6% (A) and 5 and 5% (B) of the total variance in the genetic relationship matrix, respectively.

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S4 Fig. 3-dimensional PCA scatter diagram showing the relative position of the five pig breeds defined by eigenvectors based on genetic relationship matrix from all autosomal SNPs.

Eigenvector 1, 2 and 3 accounted for 19, 6 and 5.5% of the total variance in the genetic relationship matrix, respectively.

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S5 Fig. Histogram showing raw XP-EHH score and frequency between Yucatan miniature pig and other swine breeds: Duroc (A), Landrace (B) and Yorkshire (C).

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S6 Fig. Histogram showing the number of SNPs in non-overlapping 50kb window and frequency.

(TIFF)

S7 Fig. Venn diagram showing the number of outlier loci (region) detected by XP-EHH in each comparison between Yucatan miniature pig and other breeds (Duroc, Landrace and Yorkshire).

(TIFF)

S8 Fig. Nucleotide diversity plot of 19 genes detected by XP-EHH.

The nucleotide diversity was estimated for each 5-kb window. Each solid vertical line represents boundary of gene, and each dotted line represents boundary of region detected by XP-EHH. Each pig breed is marked by a colored line; blue for Landrace, green for Yorkshire, purple for Yucatan miniature pig and yellow for Duroc.

(TIFF)

S1 Table. Body weight of Yucatan miniature pig.

(DOCX)

S2 Table. Mapping rate and the number of filtered SNPs of resequencing data of 70 pigs.

(XLSX)

S3 Table. Genome coverage and depth of resequencing data of 70 pigs.

(XLSX)

S4 Table. Number of SNPs in 70 pigs.

(XLSX)

S5 Table. Outlier regions detected by XP-EHH test between Yucatan miniature pig and each of large swine breeed (Duroc, Landrace and Yorkshire).

(XLSX)

Acknowledgments

The DNA re-sequencing data of all 70 pigs from this study have been submitted to the NCBI Sequence Read Archive (SRA) database under accession number SRP047260.

Data Availability

The DNA re-sequencing data of all 70 pigs from this study have been submitted to the NCBI Sequence Read Archive (SRA) database under accession number SRP047260.

Funding Statement

This work was supported by a grant from the Next-Generation BioGreen 21 Program [No. PJ01104401, PJ01110901 and PJ00811602], Rural Development Administration, Republic of Korea. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. Optipharm, Inc provided support in the form of salaries for authors [Hyunil Kim, KC and Jiho Kim], but did not have any additional role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript. The specific roles of these authors are articulated in the ‘author contributions’ section.

References

  • 1. Fang X, Mu Y, Huang Z, Li Y, Han L, Zhang Y, et al. (2012) The sequence and analysis of a Chinese pig genome. GigaScience 1: 1–11. 10.1186/2047-217X-1-1 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 2. Larson G, Dobney K, Albarella U, Fang M, Matisoo-Smith E, Robins J, et al. (2005) Worldwide phylogeography of wild boar reveals multiple centers of pig domestication. Science 307: 1618–1621. [DOI] [PubMed] [Google Scholar]
  • 3. Suzuki K, Irie M, Kadowaki H, Shibata T, Kumagai M, Nishida A (2005) Genetic parameter estimates of meat quality traits in Duroc pigs selected for average daily gain, longissimus muscle area, backfat thickness, and intramuscular fat content. Journal of Animal Science 83: 2058–2065. [DOI] [PubMed] [Google Scholar]
  • 4. Haensly WE, Getty R (1968) Age changes in the weight of the adrenal glands of swine from birth to eight years. Journal of Gerontology 23: 53–57. [DOI] [PubMed] [Google Scholar]
  • 5. Suzuki K, Shibata T, Kadowaki H, Abe H, Toyoshima T (2003) Meat quality comparison of Berkshire, Duroc and crossbred pigs sired by Berkshire and Duroc. Meat science 64: 35–42. [DOI] [PubMed] [Google Scholar]
  • 6. Magowan E, E. McCann ME (2009) The effect of sire line breed on the lifetime performance of slaughter generation pigs In: Ireland DoAaRDfN, editor. England: Agri-Food and Biosciences Institute; pp. 1–25. [Google Scholar]
  • 7.(1991)Microlivestock:Little-Known Small Animals with a Promising Economic Future: The National Academies Press. [Google Scholar]
  • 8. Smith DM, Martens GW, Ho CS, Asbury JM (2005) DNA sequence based typing of swine leukocyte antigens in Yucatan miniature pigs. Xenotransplantation 12: 481–488. [DOI] [PubMed] [Google Scholar]
  • 9. Panepinto L, Phillips R (1986) The Yucatan miniature pig: characterization and utilization in biomedical research. Laboratory animal science 36: 344 [PubMed] [Google Scholar]
  • 10. Andersson L (2012) How selective sweeps in domestic animals provide new insight into biological mechanisms. Journal of internal medicine 271: 1–14. 10.1111/j.1365-2796.2011.02450.x [DOI] [PubMed] [Google Scholar]
  • 11. Smith JM, Haigh J (1974) The hitch-hiking effect of a favourable gene. Genetical research 23: 23–35. [PubMed] [Google Scholar]
  • 12. Voight BF, Kudaravalli S, Wen XQ, Pritchard JK (2006) A map of recent positive selection in the human genome. PLoS biology 4: 446–458. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 13. Pickrell JK, Coop G, Novembre J, Kudaravalli S, Li JZ, Absher D, et al. (2009) Signals of recent positive selection in a worldwide sample of human populations. Genome research 19: 826–837. 10.1101/gr.087577.108 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 14. Sabeti PC, Varilly P, Fry B, Lohmueller J, Hostetter E, Cotsapas C, et al. (2007) Genome-wide detection and characterization of positive selection in human populations. Nature 449: 913–918. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 15. Tang K, Thornton KR, Stoneking M (2007) A new approach for using genome scans to detect recent positive selection in the human genome. PLoS biology 5: e171 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 16. Kim T, Kim K, Choi B, Yoon D, Jang G, Lee K, et al. (2005) Genetic structure of pig breeds from Korea and China using microsatellite loci analysis. Journal of Animal Science 83: 2255–2263. [DOI] [PubMed] [Google Scholar]
  • 17. Maglott D, Ostell J, Pruitt KD, Tatusova T (2011) Entrez Gene: gene-centered information at NCBI. Nucleic acids research 39: D52–D57. 10.1093/nar/gkq1237 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 18. Lawrence DA (1996) Transforming growth factor-beta: a general review. European cytokine network 7: 363 [PubMed] [Google Scholar]
  • 19. Horton G, Blethen D, Prasad B (1991) The effect of garlic (Allium sativum) on feed palatability of horses and feed consumption, selected performance and blood parameters in sheep and swine. Canadian Journal of Animal Science 71: 607–610. [Google Scholar]
  • 20. Solà-Oriol D, Roura E, Torrallardona D (2009) Feed preference in pigs: Effect of cereal sources at different inclusion rates. Journal of Animal Science 87: 562–570. 10.2527/jas.2008-0949 [DOI] [PubMed] [Google Scholar]
  • 21. Zheng H, Jiang M, Trumbauer ME, Sirinathsinghji DJ, Hopkins R, Smith DW, et al. (1995) β-Amyloid precursor protein-deficient mice show reactive gliosis and decreased locomotor activity. Cell 81: 525–531. [DOI] [PubMed] [Google Scholar]
  • 22. Lee S-J, McPherron AC (2001) Regulation of myostatin activity and muscle growth. Proceedings of the National Academy of Sciences 98: 9306–9311. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 23. Walsh S, Metter EJ, Ferrucci L, Roth SM (2007) Activin-type II receptor B (ACVR2B) and follistatin haplotype associations with muscle mass and strength in humans. Journal of Applied Physiology 102: 2142–2148. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 24. Hogan A, Yakubchyk Y, Chabot J, Obagi C, Daher E, Maekawa K, et al. (2004) The phosphoinositol 3, 4-bisphosphate-binding protein TAPP1 interacts with syntrophins and regulates actin cytoskeletal organization. Journal of Biological Chemistry 279: 53717–53724. [DOI] [PubMed] [Google Scholar]
  • 25.Galione A, Churchill GC (2000) Cyclic ADP ribose as a calcium-mobilizing messenger. Science Signaling 2000: pe1. [DOI] [PubMed]
  • 26. Barbosa MTP, Soares SM, Novak CM, Sinclair D, Levine JA, Aksoy P, et al. (2007) The enzyme CD38 (a NAD glycohydrolase, EC 3.2. 2.5) is necessary for the development of diet-induced obesity. The FASEB Journal 21: 3629–3639. [DOI] [PubMed] [Google Scholar]
  • 27. Wang J, Zhou J, Powell-Braxton L, Bondy C (1999) Effects of Igf1 gene deletion on postnatal growth patterns. Endocrinology 140: 3391–3394. [DOI] [PubMed] [Google Scholar]
  • 28. Sutter NB, Bustamante CD, Chase K, Gray MM, Zhao K, Zhu L, et al. (2007) A single IGF1 allele is a major determinant of small size in dogs. Science Signaling 316: 112 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 29. Deng C, Ma R, Yue X, Lan X, Chen H, Lei C (2010) Association of IGF-I gene polymorphisms with milk yield and body size in Chinese dairy goats. Genetics and molecular biology 33: 266–270. 10.1590/S1415-47572010005000034 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 30. Fan B, Onteru SK, Du Z-Q, Garrick DJ, Stalder KJ, Rothschild MF (2011) Genome-wide association study identifies loci for body composition and structural soundness traits in pigs. Plos One 6: e14726 10.1371/journal.pone.0014726 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 31. Van Heemst D, Beekman M, Mooijaart SP, Heijmans BT, Brandt BW, Zwaan BJ, et al. (2005) Reduced insulin/IGF1 signalling and human longevity. Aging cell 4: 79–85. [DOI] [PubMed] [Google Scholar]
  • 32. Tsuji S, Uehori J, Matsumoto M, Suzuki Y, Matsuhisa A, Toyoshima K, et al. (2001) Human intelectin is a novel soluble lectin that recognizes galactofuranose in carbohydrate chains of bacterial cell wall. Journal of Biological Chemistry 276: 23456–23463. [DOI] [PubMed] [Google Scholar]
  • 33. Adachi Y, Ishii T, Ikeda Y, Hoshino A, Tamura H, Aketagawa J, et al. (2004) Characterization of β-glucan recognition site on C-type lectin, dectin 1. Infection and immunity 72: 4159–4171. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 34. Hayashida K, Kume N, Minami M, Kita T (2002) Lectin-like oxidized LDL receptor-1 (LOX-1) supports adhesion of mononuclear leukocytes and a monocyte-like cell line THP-1 cells under static and flow conditions. FEBS letters 511: 133–138. [DOI] [PubMed] [Google Scholar]
  • 35. Delneste Y, Magistrelli G, Gauchat J-F, Haeuw J-F, Aubry J-P, Nakamura K, et al. (2002) Involvement of LOX-1 in dendritic cell-mediated antigen cross-presentation. Immunity 17: 353–362. [DOI] [PubMed] [Google Scholar]
  • 36. Despouy G, Perez V, Jouvenot M, Boyer-Guittaut M (2010) GABARAPL1 (GEC1) associates with autophagic vesicles. Autophagy 6: 495–505. 10.4161/auto.6.4.11819 [DOI] [PubMed] [Google Scholar]
  • 37. Miah S, Hatani T, Qu X, Yamamura H, Sada K (2004) Point mutations of 3BP2 identified in human‐inherited disease cherubism result in the loss of function. Genes to Cells 9: 993–1004. [DOI] [PubMed] [Google Scholar]
  • 38. Li H, Durbin R (2010) Fast and accurate long-read alignment with Burrows–Wheeler transform. Bioinformatics 26: 589–595. 10.1093/bioinformatics/btp698 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 39. Li H, Handsaker B, Wysoker A, Fennell T, Ruan J, Homer N, et al. (2009) The sequence alignment/map format and SAMtools. Bioinformatics 25: 2078–2079. 10.1093/bioinformatics/btp352 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 40. McKenna A, Hanna M, Banks E, Sivachenko A, Cibulskis K, Kernytsky A, et al. (2010) The Genome Analysis Toolkit: a MapReduce framework for analyzing next-generation DNA sequencing data. Genome Research 20: 1297–1303. 10.1101/gr.107524.110 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 41. DePristo MA, Banks E, Poplin R, Garimella KV, Maguire JR, Hartl C, et al. (2011) A framework for variation discovery and genotyping using next-generation DNA sequencing data. Nature genetics 43: 491–498. 10.1038/ng.806 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 42. Browning BL, Yu Z (2009) Simultaneous genotype calling and haplotype phasing improves genotype accuracy and reduces false-positive associations for genome-wide association studies. Am J Hum Genet 85: 847–861. 10.1016/j.ajhg.2009.11.004 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 43. Purcell S, Neale B, Todd-Brown K, Thomas L, Ferreira MA, Bender D, et al. (2007) PLINK: a tool set for whole-genome association and population-based linkage analyses. The American Journal of Human Genetics 81: 559–575. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 44. Danecek P, Auton A, Abecasis G, Albers CA, Banks E, DePristo MA, et al. (2011) The variant call format and VCFtools. Bioinformatics 27: 2156–2158. 10.1093/bioinformatics/btr330 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 45. Saitou N, Nei M (1987) The neighbor-joining method: a new method for reconstructing phylogenetic trees. Molecular Biology and Evolution 4: 406–425. [DOI] [PubMed] [Google Scholar]
  • 46.Rambaut A (2012) FigTree.
  • 47. Pritchard JK, Stephens M, Donnelly P (2000) Inference of population structure using multilocus genotype data. Genetics 155: 945–959. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 48. Yang J, Lee SH, Goddard ME, Visscher PM (2011) GCTA: a tool for genome-wide complex trait analysis. American journal of human genetics 88: 76 10.1016/j.ajhg.2010.11.011 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 49. Price AL, Patterson NJ, Plenge RM, Weinblatt ME, Shadick NA, Reich D (2006) Principal components analysis corrects for stratification in genome-wide association studies. Nature genetics 38: 904–909. [DOI] [PubMed] [Google Scholar]
  • 50. Granka JM, Henn BM, Gignoux CR, Kidd JM, Bustamante CD, Feldman MW (2012) Limited evidence for classic selective sweeps in African populations. Genetics 192: 1049–1064. 10.1534/genetics.112.144071 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 51.Lee H-J, Kim J, Lee T, Son JK, Yoon H-B, Baek K-S, et al. (2014) Deciphering the genetic blueprint behind Holstein milk proteins and production. Genome Biology and Evolution: evu102. [DOI] [PMC free article] [PubMed]
  • 52. Teshima KM, Coop G, Przeworski M (2006) How reliable are empirical genomic scans for selective sweeps? Genome research 16: 702–712. [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 53. Dennis G Jr, Sherman BT, Hosack DA, Yang J, Gao W, Lane HC, et al. (2003) DAVID: database for annotation, visualization, and integrated discovery. Genome Biol 4: P3 [PubMed] [Google Scholar]
  • 54. Hosack DA, Dennis G Jr, Sherman BT, Lane HC, Lempicki RA (2003) Identifying biological themes within lists of genes with EASE. Genome Biol 4: R70 [DOI] [PMC free article] [PubMed] [Google Scholar]
  • 55. Alterovitz G, Ramoni MF (2010) Knowledge based bioinformatics: Wiley Online Library. [Google Scholar]

Associated Data

This section collects any data citations, data availability statements, or supplementary materials included in this article.

Supplementary Materials

S1 Fig. SNP density plot of 70 pigs.

(TIFF)

S2 Fig. Proportion of membership of 70 pigs into each of the five different breeds showing population admixture.

(TIFF)

S3 Fig. PCA scatter diagram showing the relative position of the five pig breeds (A) and the two closely related Yorkshire and Landrace breeds (B), defined by eigenvectors based on genetic relationship matrix from all autosomal SNPs.

Eigenvector 1 and 2 accounted for 19 and 6% (A) and 5 and 5% (B) of the total variance in the genetic relationship matrix, respectively.

(TIFF)

S4 Fig. 3-dimensional PCA scatter diagram showing the relative position of the five pig breeds defined by eigenvectors based on genetic relationship matrix from all autosomal SNPs.

Eigenvector 1, 2 and 3 accounted for 19, 6 and 5.5% of the total variance in the genetic relationship matrix, respectively.

(TIFF)

S5 Fig. Histogram showing raw XP-EHH score and frequency between Yucatan miniature pig and other swine breeds: Duroc (A), Landrace (B) and Yorkshire (C).

(TIFF)

S6 Fig. Histogram showing the number of SNPs in non-overlapping 50kb window and frequency.

(TIFF)

S7 Fig. Venn diagram showing the number of outlier loci (region) detected by XP-EHH in each comparison between Yucatan miniature pig and other breeds (Duroc, Landrace and Yorkshire).

(TIFF)

S8 Fig. Nucleotide diversity plot of 19 genes detected by XP-EHH.

The nucleotide diversity was estimated for each 5-kb window. Each solid vertical line represents boundary of gene, and each dotted line represents boundary of region detected by XP-EHH. Each pig breed is marked by a colored line; blue for Landrace, green for Yorkshire, purple for Yucatan miniature pig and yellow for Duroc.

(TIFF)

S1 Table. Body weight of Yucatan miniature pig.

(DOCX)

S2 Table. Mapping rate and the number of filtered SNPs of resequencing data of 70 pigs.

(XLSX)

S3 Table. Genome coverage and depth of resequencing data of 70 pigs.

(XLSX)

S4 Table. Number of SNPs in 70 pigs.

(XLSX)

S5 Table. Outlier regions detected by XP-EHH test between Yucatan miniature pig and each of large swine breeed (Duroc, Landrace and Yorkshire).

(XLSX)

Data Availability Statement

The DNA re-sequencing data of all 70 pigs from this study have been submitted to the NCBI Sequence Read Archive (SRA) database under accession number SRP047260.


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