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. 2022 Feb 2;2022:8319396. doi: 10.1155/2022/8319396

Artificial Selection Drives SNPs of Olfactory Receptor Genes into Different Working Traits in Labrador Retrievers

Min Yang 1, Han-Xin Zhang 2, Guang-Jun Geng 3, Fu-Jin Wang 4, Cheng-Wu Liu 1, Jian-Li Liu 5,
PMCID: PMC8828343  PMID: 35185392

Abstract

Labs as guide dogs or sniffer dogs in usage have been introduced into China for more than 20 years. These two types of working dogs own blunt or acute olfactory senses, which have been obtained by artificial selection in relatively closed populations. In order to attain stable olfactory attributes and meet use-oriented demands, Chinese breeders keep doing the same artificial selection. Though olfactory behavior is canine genetic behavior, genotypes of OR genes formed by breeding schemes are largely unknown. Here, we characterized 26 SNPs, 2 deletions, and 2 insertions of 7 OR genes between sniffer dogs and guide dogs in order to find out the candidate alleles associated with working specific traits. The results showed that there were candidate functional SNP alleles in one locus that had statistically severely significant differences between the two subpopulations. Furthermore, the levels of polymorphism were not high in all loci and linkage disequilibrium only happened within one OR gene. Hardy–Weinberg equilibrium (HWE) tests showed that there was a higher ratio not in HWE and lower FST within the two working dog populations. We conclude that artificial selection in working capacities has acted on SNP alleles of OR genes in a dog breed and driven the evolution in compliance with people's intentions though the changes are limited in decades of strategic breeding.

1. Background

Artificial selection has been largely responsible for breed-specific and strain-specific traits of modern dogs [1]. Compared with early domestication of a dog breed driven by natural factors such as dietary conditions and geographical environments, the recent subpopulation differentiations are more dramatically caused by artificial goal-directed breeding practices, especially during the last two centuries [2]. Strain-dependent differences of dogs are mainly presented in body size, coat color, and work capacity [3, 4]. Labrador Retriever (Lab) is a traditional waterdog in Newfoundland. During the latter half of the nineteenth century, British breeders had refined and standardized Labs that had become a popular breed because they were famously friendly and exuberant around the world [57]. Many Labs play an important role such as sniffer dogs or guide dogs in many countries. These two types of work abilities are based on either enhanced olfaction or blunt olfaction. In order to attain stable olfactory attributes and meet use-oriented demands, Labs are bred in relatively closed populations by strict selection [8, 9].

The offsprings of pure breed Labs as guide dogs or sniffer dogs abroad were purchased from Japan by guide dogs training organizations and from Germany by police departments into China two decades ago. The same as foreign ones did, Chinese working dog organizations continued to breed Labs following the principle of closed-flock reproduction and occasionally adopted some excellent bloodlines of Labs from amateurs in the civilian clubs into Lab working dogs populations. Based on Labs' health, a temperament test of scent interest and a search test divide Labs into candidates of guide dogs with no scent interest or sniffer dogs displaying great scent interest and eager searching during early training [1012]. Then, behavioral suitability of a working dog is shaped by specialized training [8, 13]. Subsequently, the olfactory detection phenotype of qualified sniffer dogs is that the dog indicates a target odor in the manner in which it was trained while qualified guide dogs could navigate by avoiding obstacles [1416]. As far as disqualified Labs are concerned, their outcome is to be screened out of the subpopulations. Therefore, the offsprings did not degenerate and gradually became more competent for mobility support for the visually impaired/blind or scent detection for law implement. Detailed subgroup analyses are expected to explain the genetic basis for variation in olfactory behavior and to establish protocols for the reproduction of the two Labs' working strains.

Olfactory capacity and sensitivity are related to canine olfactory receptor gene polymorphism in dog breeds and individuals [9, 13]. Selections of different forms have acted on OR genes in dogs since domestication. The genetic diversity of 109 OR genes in six breeds including Labs was studied, which were representative of a large number of families, subfamilies, and clusters [17]. Through OR genes sequencing data analysis, the SNPs were identified and its Minor Allele Frequency (MAF) values testified that the 8 SNPs in 7 OR genes were private and restricted to only Labs. Because most of private SNPs arose following dog-breed formation under the selection from breeding practices and SNP alleles might present a pair of phenotypes' pros and cons in olfactory cognition, 30 SNPs including 7 private SNPs and 23 representative SNPs in the same OR genes might be studied to find out how the artificial selection drives them into phenotypic differentiation of olfactory behavior in Labs. Identifying the distributions of SNP alleles between the two subgroups might provide insights into genetic variation that might explain specific working traits and then efficiently obtain a desired phenotype [18].

2. Materials and Methods

2.1. Ethical Statement

This study was carried out in Police-Dog Technology Department, Criminal Investigation Police University of China. The protocol for the animal experiment was reviewed and approved by the Ethics Committee of Police-Dog Technology Department (JQJS2019-0001), and all applicable institutional and governmental regulations concerning the ethical use of animals were followed.

2.2. Animals and Blood Sample Collection

The trial included two subpopulations, 49 guide dogs (males, n = 36; females, n = 13) and 43 sniffer dogs (males, n = 31; females, n = 12) of Labs, whose ages ranged from 2 to 4 years old. The Labs were reproduced by China Guide Dog Training Center and Police-Dog Technology Department, Criminal Investigation Police University of China. According to the certificates of the dogs' pedigree, the two groups sampled were unrelated. All the dogs treated in a humane manner passed the qualification assessments of working dogs and had been competent for the tasks assigned. Blood samples were obtained from each dog, and then Universal Genomic DNA Extraction Kit (Takara, China) was used to extract DNAs.

2.3. SNP and Primer Design

30 SNP loci lying in exonic regions of 7 OR genes were analyzed and are shown in Table 1. Asterisks marked out the breed-specific SNPs [17]. No asterisks meant that the SNPs could be found in other dog breeds besides Labs. Because non-breed-specific SNPs in the 7 OR genes led to amino-acid substitutions, frameshift variants, protein altering variants, and splicing donor variants, they were studied too. Pairs of specific primers for fraction amplification of 7 OR genes were designed using the Primer-BLAST and Primer Premier 5 program. The primer sequences, fragment sizes, and annealing temperatures (Tm) above mentioned are shown in Table S1.

Table 1.

Characteristics of the analyzed SNPs.

SNP Amino acid variant Domain MAF
OR0006:c.524 G > T p.R175L EC2 <0.01
OR0007:c.331T>C p.F111L TM3 0.50
OR0007:c.430 G > A p.G144S IC2 0.50
OR0007:c.508 G > A p.V170M TM4 0.01
OR0007:c.691 G > C p.V231L TM5 0.38
OR0007:c.730 T >C p.W244R TM6 0.39
OR0007:c.793 G > C p.V265L TM6 0.41
OR0007:c.829 C >T p.P277S EC3 0.40
OR0007:c.830 C >T p.P277L EC3 0.40
OR16C11:c.294 G > A p.Q98Q TM2 0.03
OR16C11:c.368 C >A p.A123D EC1 0.12
OR16C11:c.391 A >G p.T131A EC1 0.01
OR16C11:c.632del I212Y Ter2 TM4
DOPRX09:c.479 G > A p.S160N EC2 0.49
DOPRX09:c.481 T >G p.S161A EC2 0.49
DOPRX09:c.486 T >G p.F162L TM5 0.49
DOPRX09:c.889 G > A p.V263I C 0.03
OR08G02:c.756 G > T p.G252G N/A
OR7215:c.251 C >T P.84L TM2 0.36
OR7215:c.272ins- > TCTTCC p.C91FFR EC1
OR7215:c.273ins-> CTTC/CTTCCA p.C91CFX91CFH EC1 0.25
OR7215:c.286 G > A p.G96S EC1 0.02
OR7215:c.299 A >G p.Y100C TM3 0.21
OR7215:c.339 G > A p.M113I TM3 0.14
OR7215:c.398delTGCGCTA > - TM4 0.11
OR7215:c.413 G > A R138H TM4 0.04
OR7215:c.578 A >T N193I TM5
OR04B06:c.215 T >G L72 R TM2
OR04B06:c.394 A >G A132 T TM4
OR04B06:c.411 A >T F137 L TM4
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Asterisks marked out the breed-specific SNPs. No asterisks meant that the SNPs could be found in other dog breeds besides Labs. MAF: minor allele frequency.

2.4. PCR and Sequencing

Polymerase chain reaction (PCR) was conducted using a Veriti thermal cycler (ABI, USA) in a total volume of 50 μL that included 2 μL 100 ng of genomic DNA, 25 μL Premix Taq (Takara, China), and 1 μM (final conc.) of each specific primer and water up to 50 μL. PCR products were loaded onto a 2% agarose gel stained with GeneFinder (Biov, China) and DNAs were extracted from the gel. The purified products of PCR were cloned into pMD18-T vector (Takara, China) and positive clones specific for each of the seven amplicons were sequenced in both directions. Nucleotide BLAST of the sequences was done. Then the purified products of PCR were massively directly sequenced by the forward or reverse primers.

Sequencing PCR reaction was performed in a 10 μl reaction system that consisted of Premix 4 μL, the purified PCR products 0.5 μL, primer 1 μL (1 μM), and 4.5 μL ddH2O, starting with 30 cycles of denaturation at 96°C for 20 secs, annealing at 55°C for 20 secs, and extension at 60°C for 4 mins, followed by an extra stop reaction initiated by adding 0.5 μL of glycogen, 1 μL of 3M sodium acetate (pH5.2), and 1 μL of 100 mM Na2-EDTA (pH8.0) per reaction. 40 μL of sample loading solution was added into DNA precipitates with ethanol in individual tubes to resuspend the samples. The capillary electrophoresis was analyzed on Beckman GeXP Genetic Analysis System according to Genome-Lab Dye Terminator Cycle Sequencing with Quick Start Kit (Beckman, USA).

2.5. Statistical Analysis

Allele frequency, Genotype frequency, observed heterozygosity (Ho), and polymorphism information content (PIC) were calculated by PowerStats software v1.2 [19]. Expected heterozygosity (He) was counted by CERVUS 3.0.3 [20] software. The F-value of an inbreeding coefficient was derived by [1- (Ho/He)] by EXCEL software too [21]. Hardy–Weinberg equilibrium (HWE) tests were performed by ARLEQUIN software v3.5 [22]. Linkage disequilibrium analyses (correlation coefficient, r2) and the chi-square test about alleles on single locus in a pairwise study were analyzed by SHEsis online tool. A logistic regression analysis of alleles and genotypes was performed on IBM SPSS Statistics 25 software. Fst values were calculated by GenAlEx 6.5 software [23]. The tools including Protein Variation Effect Analyzer (PROVEAN) http://provean.jcvi.org/index.php [24], Align-Grantham variation and Grantham deviation (Align GVGD) http://agvgd.hci.utah.edu/ [25], and Sorting Intolerant from Tolerant (SIFT) https://sift.bii.astar.edu.sg/ [26] were used to predict the effect of nonsynonymous SNPs in the encoded proteins.

3. Results

Allele frequencies and genotype frequencies of 30 SNP loci are given in Table 2, which ranged from 0 to 1. Overall, the most of the SNP loci had a major allele whose frequencies were beyond 0.8 except for six loci in guide dogs, seven loci in sniffer dogs, and seven loci in the collective. Furthermore, a unique homozygous genotype was presented in 12 SNP loci, while the only heterozygous genotype was found in 2 SNP loci within all Labs. So, the 14 SNP loci were excluded in the chi-square test for differences of alleles on a single SNP locus in a pairwise study. Among the 12 homozygous loci, the deletions of the loci OR16C11:c.633del and OR7215:c.398del that could result in no expression of gene OR16C11 and a splice donor variant of gene OR7215 did not happen and the insertion of OR7215:c.272ins producing a protein altering variant did not happen either. Noticeably the insertion of OR7215:c.273insCTTCCA producing a frameshift variant occurred to all Labs. Regarding the remaining 16 loci, there were differences either in genotypes or in genotype frequencies between sniffer dogs and guide dogs. All three genotypes were found in the two loci OR0007:c.691 G > C and OR0007:c.830 C >T only in guide dogs while sniffer dogs presented GG or GC genotype in the locus OR0007:c.691 G > C and were all homozygotes with TT genotype in the locus OR0007:c.830 C >T. Consequently, the alleles in seven SNP loci showed significant differences (P < 0.05), and highly significant differences (P < 0.001) were shown in the four SNP loci of which the three SNP loci were breed-specific between the two working groups given in Table 3. On the basis of differences of the SNP alleles between sniffer dogs and guide dogs, a binary logistic regression analysis was carried out, and it found that the alleles and genotypes in five SNP loci could affect types of working dogs (P < 0.05) given in Table 4.

Table 2.

Allele frequency and genotype frequency of 30 SNP loci.

Loci Guide dog Sniffer Collective
Allele frequency Genotype frequency Allele frequency Genotype frequency Allele frequency Genotype frequency
OR0006:c.524 G > T G/0.980 T/0.020 GG/0.959 GT/0.041 G/0.942 T/0.058 GG/0.884 GT/0.116 G/0.962 T/0.038 GG/0.924 GT/0.076
OR0007:c.331 T >C T/0.878 C/0.122 TT/0.755 TC/0.245 T/0.709 C/0.291 TT/0.419 TC/0.581 T/0.799 C/0.201 TT/0.598 TC/0.402
OR0007:c.430 G > A A/0.796 G/0.204 AA/0.592 GA/0.408 A/0.942 G/0.058 AA/0.884 GA/0.116 A/0.864 G/0.136 AA/0.728 GA/0.272
OR0007:c.508 G > A G/1 GG/1 G/0.907 A/0.093 GG/0.814 GA/0.186 G/0.957 A/0.043 GG/0.913 GA/0.087
OR0007:c.691 G > C G/0.663 C/0.337 GG/0.408 GC/0.510 CC/0.082 G/0.628 C/0.372 GG/0.256 GC/0.744 G/0.647 C/0.353 GG/0.337 GC/0.620 CC/0.043
OR0007:c.730 T >C C/0.878 T/0.122 CC/0.755 CT/0.245 C/1 CC/1 C/0.935 T/0.065 CC/0.870 CT/0.130
OR0007:c.793 G > C C/0.837 G/0.163 CC/0.673 CG/0.327 C/0.942 G/0.058 CC/0.884 CG/0.116 C/0.886 G/0.114 CC/0.772 CG/0.228
OR0007:c.829 C >T C/0.541 T/0.459 CC/0.082 TC/0.918 C/0.5 T/0.5 TC/1 C/0.522 T/0.478 CC/0.043 TC/0.957
OR0007:c.830 C >T C/0.837 T/0.163 TT/0.755 TC/0.163 CC/0.082 T/1 TT/1 C/0.087 T/0.913 TT/0.870 TC/0.087 CC/0.043
OR16C11:c.294 G > A G/0.929 A/0.071 GG/0.857 GA/0.143 G/0.884 A/0.116 GG/0.767 GA/0.233 G/0.908 A/0.092 GG/0.815 GA/0.185
OR16C11:c.368 C >A C/1 CC/1 C/0.953 A/0.047 CC/0.907 CA/0.093 C/0.978 A/0.022 CC/0.957 CA/0.043
OR16C11:c.391 A >G A/0.969 G/0.031 AA/0.939 GA/0.061 A/1 AA/1 A/0.984 G/0.016 AA/0.967 GA/0.033
OR16C11:c.632del NONE NONE NONE NONE
DOPRX09:c.479 G > A G/0.5 A/0.5 GA/1 G/0.5 A/0.5 GA/1 G/0.5 A/0.5 GA/1
DOPRX09:c.481 T >G T/0.5 G/0.5 TG/1 T/0.5 G/0.5 TG/1 T/0.5 G/0.5 TG/1
DOPRX09:c.486 T > G G/0.541 T/0.459 GG/0.082 GT/0.918 G/0.698 T/0.302 GG/0.395 GT/0.605 G/0.614 T/0.386 GG/0.228 GT/0.772
DOPRX09:c.889 G > A G/0.102 A/0.898 GG/0.796 GA/0.204 G/1 GG/1 G/0.946 A/0.054 GG/0.891 GA/0.109
OR08G02:c.756 G > T G/1 GG/1 G/1 GG/1 G/1 GG/1
OR7215:c.251 C >T C/0.163 T/0.837 CC/0.163 TT/0.837 C/0.605 T/0.395 CC/0.605 TT/0.395 T/0.370 T/0.630 CC/0.370 TT/0.630
OR7215:c.272ins None None None
OR7215:c.273ins CTTCCA/1 CTTCCA/1 CTTCCA/1 CTTCCA/1 CTTCCA/1 CTTCCA/1
OR7215:c.286 G > A G/1 GG/1 G/1 GG/1 G/1 GG/1
OR7215:c.299 A >G G/1 GG/1 G/1 GG/1 G/1 GG/1
OR7215:c.339 G > A G/1 GG/1 G/1 GG/1 G/1 GG/1
OR7215:c.398del None None None
OR7215:c.413 G > A G/1 GG/1 G/1 GG/1 G/1 GG/1
OR7215:c.578 A >T A/1 AA/1 A/0.838 T/0.162 AA/0.838 TT/0.162 A/0.924 T/0.076 AA/0.924 T T/0.076
OR04B06:c.215 T >G T/1 TT/1 T/1 TT/1 T/1 TT/1
OR04B06:c.394 A >G G/1 GG/1 G/1 GG/1 G/1 GG/1
OR04B06:c.411 A >T T/1 TT/1 T/1 TT/1 T/1 TT/1
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Asterisks marked out the breed-specific SNPs. No asterisks meant that the SNPs could be found in other dog breeds besides Labs.

Table 3.

Differences of SNP alleles between sniffer dogs and guide dogs.

Loci P value
OR0006:c.524 G > T 0.182
OR0007:c.331 T >C 0.005
OR0007:c.430 G > A 0.004
OR0007:c.508 G > A 0.002
OR0007:c.691 G > C 0.617
OR0007:c.730 T > C 0.001
OR0007:c.793 G > C 0.025
OR0007:c.829 C > T 0.580
OR0007:c.830 C > T 8.88e − 005
OR16C11:c.294 G > A 0.295
OR16C11:c.368 C > A 0.031
OR16C11:c.391 A > G 0.183
DOPRX09:c.486 T > G 0.029
DOPRX09:c.889 G > A 0.002
OR7215:c.251 C > T 6.25e − 010
OR7215:c.578 A > T 3.28e − 005
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Asterisks marked out the breed-specific SNPs. No asterisks meant that the SNPs could be found in other dog breeds besides Labs.

Table 4.

Logistic regression analysis of alleles and genotypes between sniffer dogs and guide dogs.

Loci Allele Genotype
OR (95% CI) P OR (95% CI) P
OR0007:c.331 T >C 3.106(1.453–6.636) 0.003 4.282(1.760–10.422) 0.001
OR0007:c.430 G > A 5.256(1.720–16.068) 0.004 5.241(1.758–15.631) 0.003
OR0007:c.508 G > A 2.030 × 109(0.000-) 0.999 2.262 × 109(0.000-) 0.999
OR0007:c.730 T >C 1.615 × 109(0.000-) 0.999 1.877 × 109(0.000-) 0.999
OR0007:c.793 G > C 8.195(1.827–36.770) 0.006 3.685(1.218–11.150) 0.021
OR0007:c.830 C >T 0.000(0.000-) 0.996 (1) 0.000(0.000-) (1) 0.999
(2) 0.000(0.000-) (2) 0.999
OR16C11:c.368 C >A 1.931 × 109(0.000-) 0.999 2.030 × 109(0.000-) 0.999
DOPRX09:c.486 T >G 1.880(1.023–3.455) 0.042 7.36(2.235–24.213) 0.001
DOPRX09:c.889 G > A 0.000(0.000-) 0.996 0.000(0.000-) 0.999
OR7215:c.251 C >T 7.838(3.938–15.601) 0.000 7.838(2.961–20.748) 0.000
OR7215:c.578 A >T 0.000(0.000-) 0.998 0.000(0.000-) 0.999
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Asterisks marked out the breed-specific SNPs. No asterisks meant that the SNPs could be found in other dog breeds besides Labs.

In this study, except for 12 homozygous monogenotype loci, PIC values of 18 SNPs ranged from 0 to 0.375. Among the 18 SNPs, 10 SNPs belonged to low polymorphism (PIC<0.25) and 5 SNPs belonged to moderate polymorphism (0.25 < PIC<0.5) for all Labs. As far as the other three SNPs, OR0007:c.331 T >C, OR0007:c.430 G > A, and OR7215:c.251 C >T, were concerned, they belonged to either low or moderate polymorphism, which differed between guide dogs and sniffer dogs (seen in Table 5). As could be seen in Table 5, Ho values were within the wide scope of 0 to 1 and He values were not more than 0.5. There were unanimously low Ho values in 12 SNP loci (<0.5) and high Ho values in 4 SNP loci (≥0.5) in the two working groups except that the values varied in the SNP loci of OR0007:c.331 T >C and OR0007:c.829C>T between guide dogs and sniffer dogs.

Table 5.

Genetic polymorphism and HWE analysis of the collective and working dog subpopulations.

Loci Ho He PIC HWE
Guide Sniffer Collective Guide Sniffer Collective Guide Sniffer Collective Guide Sniffer Collective
OR0006:c.524 G > T 0.041 0.116 0.076 0.039 0.109 0.073 0.038 0.103 0.070 0.884 0.686 0.704
OR0007:c.331 T > C 0.245 0.581 0.402 0.214 0.413 0.321 0.191 0.328 0.270 0.329 0.007 0.016
OR0007:c.430 G > A 0.408 0.116 0.272 0.325 0.109 0.235 0.272 0.103 0.207 0.073 0.686 0.132
OR0007:c.508 G > A 0 0.186 0.087 0 0.169 0.082 0 0.154 0.079 0.501 0.663
OR0007:c.691 G > C 0.510 0.744 0.620 0.447 0.467 0.457 0.347 0.358 0.352 0.320 1E − 04 6E − 04
OR0007:c.730 T > C 0.245 0 0.130 0.225 0 0.122 0.191 0 0.114 0.329 0.503
OR0007:c.793 G > C 0.327 0.116 0.228 0.273 0.109 0.202 0.236 0.103 0.182 0.172 0.686 0.217
OR0007:c.829 C > T 0.918 0 0.957 0.497 0 0.499 0.373 0.375 0.375 3E − 09 5E − 11 1E − 18
OR0007:c.830 C > T 0.163 0 0.087 0.273 0 0.159 0.236 0 0.146 0.005 1E − 05
OR16C11:c.294 G > A 0.143 0.233 0.185 0.132 0.205 0.167 0.123 0.184 0.153 0.590 0.388 0.329
OR16C11:c.368 C > A 0 0.093 0.043 0 0.090 0.043 0 0.086 0.042 0.749 0.831
OR16C11:c.391 A > G 0.061 0 0.033 0.060 0 0.031 0.058 0 0.031 0.825 0.874
DOPRX09:c.479 G > A 1 1 1 0.5 0.5 0.5 0.375 0.375 0.375 3E − 12 5E − 11 9E − 22
DOPRX09:c.481 T > G 1 1 1 0.5 0.5 0.5 0.375 0.375 0.375 3E − 12 5E − 11 9E − 22
DOPRX09:c.486 T > G 0.918 0.605 0.772 0.497 0.422 0.474 0.373 0.333 0.362 3E − 09 0.004 2E − 09
DOPRX09:c.889 G > A 0.204 0 0.109 0.183 0 0.102 0.166 0 0.097 0.426 0.581
OR7215:c.251-C > T 0 0 0 0.273 0.472 0.466 0.236 0.360 0.358 3E − 12 5E − 11 9E − 22
OR7215:c.578-A > T 0 0 0 0 0.273 0.140 0 0.236 0.131 5E − 11 9E − 22
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Asterisks marked out the breed-specific SNPs. No asterisks meant that the SNPs could be found in other dog breeds besides Labs. Observed heterozygosity (Ho), expected heterozygosity (He), polymorphism information content (PIC), and Hardy–Weinberg equilibrium (HWE) values.

P values of HWE tests for 18 SNP loci were given in Table 5. The total number of genotyped Labs was 92 and so HWE P = 0.0005 emphasized the need for multiple comparisons by applying Bonferroni correction (the significant level = 0.05/92). Except 12 homozygous monogenotype loci, the results revealed that 5 SNP loci were out of HWE (P < 0.0005) and 5 SNP loci were in the state of Hardy–Weinberg balance (P > 0.0005) for all Labs. The other eight SNP loci showed either significant departure or no significant deviations from HWE between working populations, while six of the eight SNP loci were in HWE in the collective. After the two working groups and the collective were analyzed, respectively, there was a higher ratio 73.3% not in HWE in sniffer dogs than 66.7% in guide dogs and 63.3% in the collective. Furthermore, the value of genetic differentiation between the two working populations was 0.054 (0.05﹤FST﹤0.15) when the loci OR0006:c.524 G > T, OR0007:c.331 T >C, OR0007:c.430 G > A, OR0007:c.793 G > C, and OR16C11:c.294 G > A in HWE were considered.

The F-values of average inbreeding coefficient were −0.226 for guide dogs and −0.241 for sniffer dogs given in Table 6. Linkage disequilibrium values for OR0007 gene, OR16C11 gene, DOPRX09 gene, and OR7215 gene were calculated for every working dog population. The results displayed that the r2 value that was more than 0.80 was shown only within OR0007 gene for the two working dog groups (see Figure 1).

Table 6.

F-value of an inbreeding coefficient in sniffer dogs and guide dogs.

Population Num F-value SE
Guide 49 −0.226 0.038
Sniffer 43 −0.241 0.044
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Figure 1.

Figure 1

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Linkage disequilibrium analyses were performed between pairwise SNP loci in OR0007 gene in the two working populations of Labs. Actual correlation coefficient (r2) values were magnified 100 times in the small box.

Nonsynonymous mutations are divided into two kinds of being tolerated (>0.05) and deleterious (≤ 0.05) with SIFT. The biological impact effects of amino acid substitution induced by nonsynonymous SNPs were considered “deleterious” (<−2.5) and “neutral” (>−2.5) by PROVEAN v.1.1.3. We estimated 24 nonsynonymous SNPs using SIFT, PROVEAN, and Align GVGD. 6 SNPs were predicted to be “untolerated” with a score below 0.05 by SIFT, 7 SNPs are predicted to be “deleterious” by PROVEAN and 10 SNPs were classified as a class C65 change, the first highest pathogenicity category by Align GVGD (see Table 7). OR0006:c.524 G > T, OR16C11:c.368 C >A, OR7215:c.251 C >T, and OR04B06 : 215T >G were considered to affect protein function or structure with all of the three analysis software.

Table 7.

Prediction of the deleterious effect of the nonsynonymous polymorphism in OR genes by SIFT, PROVEAN, and Align GVGD.

SNP Amino acid variant SIFT PROVEAN Align GVGD
GV GD Prediction
OR0006:c.524 G > T p.R175 L 0 −6.292 0.00 101.88 Class C65
OR0007:c.331 T > C p.F111 L 0.41 −2.834 0.00 21.82 Class C15
OR0007:c.430 G > A p.G144S 1 2.354 0.00 55.27 Class C55
OR0007:c.508 G > A p.V170 M 0.07 −1.330 0.00 21.52 Class C15
OR0007:c.691 G > C p.V231 L 1 1.909 0.00 31.78 Class C25
OR0007:c.730 T >C p.W244 R 1 3.875 0.00 101.29 Class C65
OR0007:c.793 G > C p.V265 L 1 2.075 0.00 31.78 Class C25
OR0007:c.829 C >T p.P277S 1 0.799 0.00 73.35 Class C65
OR0007:c.830 C > T p.P277 L 0.13 4.918 0.00 97.78 Class C65
OR16C11:c.368 C >A p.A123D 0 −5.989 0.00 125.75 Class C65
OR16C11:c.391 A >G p.T131 A 0.19 −2.605 0.00 58.02 Class C55
DOPRX09:c.479 G > A p.S160 N 0.11 −0.423 0.00 46.24 Class C45
DOPRX09:c.481 T >G p.S161 A 0.06 −0.009 0.00 99.13 Class C65
DOPRX09:c.486 T >G p.F162 L 1 −1.589 0.00 21.82 Class C15
DOPRX09:c.889 G > A p.V297I 0.02 −0.826 0.00 29.61 Class C25
OR7215:c.251 C >T p.P84 L 0.01 −7.578 0.00 97.78 Class C65
OR7215:c.286 G > A p.G96S 1 0.866 0.00 55.27 Class C55
OR7215:c.299 A >G p.Y100 C 1 10.826 0.00 193.72 Class C65
OR7215:c.339 G > A p.M113I 0.19 −1.904 0.00 10.12 Class C0
OR7215:c.413 G > A p.R138H 0.01 −4.234 0.00 28.82 Class C25
OR7215:c.578A>T∗ p.N193I N/A −0.888 0.00 148.91 Class C65
OR04B06:215T>G p.L72R 0 −5.605 0.00 101.88 Class C65
OR04B06:394A>G p.A132T 0.08 −2.476 0.00 58.02 Class C55
OR04B06:411A>T p.F137L 0.77 1.195 0.00 21.82 Class C15
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Asterisks marked out the breed-specific SNPs. No asterisks meant that the SNPs could be found in other dog breeds besides Labs. SIFT scores range from 0 to 1. The amino acid substitution is predicted to be damaging if the score is ≤0.05 and tolerated if the score is > 0.05. N/A: not available, GD ≥ C65 = most likely affected, and GD ≥ C0 = less likely affected. The amino acid substitution is predicted to be deleterious (<−2.5) and neutral (>−2.5) by PROVEAN.

4. Discussion

The aim of this study was to explain how use-oriented selection could lead to phenotypic changes of olfactory behavior in Labs. Olfactory traits of guide Labs and sniffer Labs are expected to play a role in canine behavioral genetics [27]. We focused on 26 SNPs, 2 deletions, and 2 insertions in 7 OR genes from the two Labs working dog populations. The genotyping test found that one population presented only one type of homozygote compared with the other population presenting two or three genotypes in 7 loci, suggesting that the alleles were purified and needed for working traits of guide dogs and sniffer dogs by rapid evolution [3]. These regions of extended homozygosity might be best explained by selection rather than genetic drift [28]. On the contrary, heterozygotes or one type of homozygote in a certain locus could occur in any working dog group, which indicated that putative SNP alleles and genotypes were chosen and possibly contributed to the common working traits under artificial selection. The significant differences between sniffer dogs and guide dogs happened to 36.7% of these loci, which explained that behavioural phenotypes in a dog breed might be affected by genetic background and controlled by multiple SNP alleles with large effects, which were preserved by artificial selection. So, special alleles might play functional roles that shaped working dog traits within a dog breed [28]. Moreover, functional loss or alternation of OR genes resulted from deleterious mutations could have been avoided through maintaining a large population size that enabled the effects of genetic drift to be negligible [29, 30]. Because the differences of these alleles were analyzed in small volume samples and the association between the alleles and olfactory behavior phenotypes was not analyzed, their effects remained potential.

Meanwhile, the loss of genomic diversity (PIC<0.375) resulted from strong selective pressures of olfactory behavior through gene pathways [31]. In addition, the data sets that Ho values were higher than He values except the locus OR7215:c.578 A >T in any Labs group showed that selective breeding in working dog populations had tried to gain popular hereditary features and avoid inbreeding in a limited degree. Furthermore, the mean F-values of inbreeding coefficients verified the negative regression in the two working dog groups. Low levels of linkage disequilibrium obtained for every working dog subpopulation were consistent with homogeneity within a dog breed [32, 33]. This highlighted that the most of SNP alleles within individual OR genes were not inherited as a block and suggested an ongoing gene conversion process for desirable working traits although it took people about 150 years to develop a dog breed.

The analysis of 26 SNPs by the collective and two working Labs groups showed that the proportions of being in HWE were lower than 52.6% in a former study of Labs that was a lower proportion among dog breeds [34]. It was a possible explanation that the selection of desirable phenotypic traits depending on alleles had screened the disqualified Labs out of the populations. Consequently, the artificial selection concurrently indirectly caused assortative mating and worsened the state of being out of HWE since a large number of working dogs had not made up for the shortcoming of olfactory behavior selection thoroughly in the relatively closed populations. The degree of genetic differentiation (Fst) between the two working Labs groups was 0.054, a little higher than the borderline 0.05 above which a dog breed showed moderate differentiation among its subpopulations [35]. An important reason was that breeders introduced ideal sires and dams from other Labs' subpopulations which had the improvement of some working characteristics instead of some other dog breeds with very close genetic relationship.

In silico prediction tools, SIFT, PROVEAN, and Align GVGD evaluated the pathogenicity of missense variants of 24 SNPs because bioinformatics analysis alone was usually not sufficient [36]. In order to decrease the proportion of false positive results, the positive judgments in agreement with each other were accepted. So the four missense variants residing in EC1, EC2, and TM2 domains of OR protein were not tolerated on the basis of the comprehensive analysis. Substituting amino acids by missense mutations in OR genes could contribute to increase or decrease in the sensitivity towards target odorants [37]. Among them, OR16C11:p.A123D residing in EC1 domain showed a significant difference and OR7215:p.P84 L residing in TM2 domain showed a severely significant difference between the two working Labs groups. In addition, OR7215:p.P84 L showed a possible functional role in typing working Labs subpopulations. So the functional allele is possibly related to working capacities of Labs, which might help breeders to pick out Labs of different levels in olfactory acuity early and accurately and set up different working Labs' strains. But the similar study is not still carried out in other sniffer dogs, for example, Springer Spaniels and bloodhounds. Additionally, the functions of these alleles might be examined by the transduction of the olfactory message in the future [38].

5. Conclusion

A number of analyses were conducted to reveal canine breed phylogeny or relation with some complicated qualities due to SNP variation. However, few studies aimed at subpopulation differentiations within a same dog breed. The strong artificial selection was only performed urgently to gain working attributes. Labs working in different fields acted as the sample model. SNP loci in OR genes presented indexes on the positive and negative selection, namely, a preference for acute sniffing and being numb about odor. Our analysis demonstrated that possibly functional alleles were quickly evolving in compliance with people's intentions though the changes were limited in decades of artificial selection.

Acknowledgments

This work was supported by the National Natural Science Foundation of China (31702028).

Data Availability

The data used to support the findings of this study are included within the article and the supplementary information file.

Conflicts of Interest

The authors declare that they have no conflicts of interest regarding the publication of this paper.

Supplementary Materials

Supplementary Materials

Table S1. Primer sequences of 7 OR genes.

Click here for additional data file. (37.5KB, doc)

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Associated Data

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

Supplementary Materials

Supplementary Materials

Table S1. Primer sequences of 7 OR genes.

Click here for additional data file. (37.5KB, doc)

Data Availability Statement

The data used to support the findings of this study are included within the article and the supplementary information file.

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