![MSY haplotype spectra of North African horses. (a) HT frequency plot based on the MSY tree after [38,39]. HT determining variants used to construct the downscaled tree for genotyping are denoted on branches in red. Additional information is given in Supplement, Table S2. Clustering of 119 North African horses based on genotyping result is illustrated as pies. Pie radiuses are scaled to the number of allocated individuals and colors of the portions correspond to different breeds. HG names are labeled accordingly. HTs located on internal nodes are denoted with an asterisk (*) and trailed with dashed lines that originate from corresponding internal nodes. Unascertained variants that would determine * HTs are denoted with question marks (?). HTs framed with blue and/or red borders denote that they were detected previously in Arabian (blue border) and Thoroughbred (red border) horses [38,39]. Non-colored points express HTs that were not detected in the North African sample set. Gray list on the sides of the network indicates the breeds the HTs were previously reported [38,39,40]; (b) Number of individuals that allocate within detected HTs. Sample information details are given in Supplement Table S1.](https://www.researchgate.net/profile/Lara-Radovic/publication/363862947/figure/fig1/AS:11431281328520362@1743130447675/MSY-haplotype-spectra-of-North-African-horses-a-HT-frequency-plot-based-on-the-MSY_Q320.jpg)
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Citation: Radovic, L.; Remer, V.;
Krcal, C.; Rigler, D.; Brem, G.; Rayane,
A.; Driss, K.; Benamar, M.;
Machmoum, M.; Piro, M.; et al. Y
Chromosome Haplotypes Enlighten
Origin, Influence, and Breeding
History of North African Barb
Horses. Animals 2022,12, 2579.
https://doi.org/10.3390/
ani12192579
Academic Editors: Isabel Cervantes
and María Dolores Gómez Ortiz
Received: 26 August 2022
Accepted: 23 September 2022
Published: 27 September 2022
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animals
Article
Y Chromosome Haplotypes Enlighten Origin, Influence, and
Breeding History of North African Barb Horses
Lara Radovic 1,2 , Viktoria Remer 1, Carina Krcal 1, Doris Rigler 1, Gottfried Brem 1, Ahmed Rayane 3,
Khadija Driss 4, Malak Benamar 5, Mohamed Machmoum 6, Mohammed Piro 6, Diana Krischke 7,8,
Ines von Butler-Wemken 7and Barbara Wallner 1,*
1Institute of Animal Breeding and Genetics, University of Veterinary Medicine Vienna, 1210 Vienna, Austria
2Vienna Graduate School of Population Genetics, University of Veterinary Medicine Vienna,
1210 Vienna, Austria
3World Barb Horse Organization O.M.C.B., Organisation Mondiale Du Cheval Barbe, 148 Avenue de l’ALN
Caroubier Hussein Dey Alger, Algiers 16000, Algeria
4Tunisian Horse Breeding Organization F.N.A.R.C., Foundation Nationale pour l´Amélioration de la Race
Chevaline, Sidi Thabet 2020, Tunisia
5Royal Horse Breeding Association SOREC, SociétéRoyale d´Encouragement Du Cheval, Haras Regional la
Kasbah de Bouznika, B. P. 52, Bouznika 13100, Morocco
6Veterinary Genetic Laboratory, Hassan II, Agronomic and Veterinary Institute, B. P. 6202,
Rabat 10101, Morocco
7Barb Horse Breeding Organization VFZB e. V., Verein der Freunde und Züchter des Berberpferdes e.V.,
Kirchgasse 11, 67718 Schmalenberg, Germany
8Department of Animal Breeding, University of Kassel, Nordbahnhofstr. 1a, 37213 Witzenhausen, Germany
*Correspondence: barbara.wallner@vetmeduni.ac.at; Tel.: +43-1-25077-5625
Simple Summary:
Bred over centuries in the Maghreb region, on a corridor between the Arab and
the Western world, the North African Barb horse has been touched by many influences in the course
of history. The present study investigated the paternally inherited Y chromosome in today
´
s Barbs
and Arab-Barbs collected from North Africa and Europe, with the aim to link genetic patterns and
narrative history. A broad Y chromosomal spectrum was observed, as well as regional disparities
among populations. Y chromosomal patterns illustrated a tight connection of Barb horses with
Arabians and several other breeds, including Thoroughbreds. Besides, results depict footprints of
past migrations between North Africa and the Iberian Peninsula.
Abstract:
In horses, demographic patterns are complex due to historical migrations and eventful
breeding histories. Particularly puzzling is the ancestry of the North African horse, a founding horse
breed, shaped by numerous influences throughout history. A genetic marker particularly suitable to
investigate the paternal demographic history of populations is the non-recombining male-specific
region of the Y chromosome (MSY). Using a recently established horse MSY haplotype (HT) topology
and KASP
™
genotyping, we illustrate MSY HT spectra of 119 Barb and Arab-Barb males, collected
from the Maghreb region and European subpopulations. All detected HTs belonged to the Crown
haplogroup, and the broad MSY spectrum reflects the wide variety of influential stallions throughout
the breed’s history. Distinct HTs and regional disparities were characterized and a remarkable number
of early introduced lineages were observed. The data indicate recent refinement with Thoroughbred
and Arabian patrilines, while 57% of the dataset supports historical migrations between North Africa
and the Iberian Peninsula. In the Barb horse, we detected the HT linked to Godolphin Arabian, one
of the Thoroughbred founders. Hence, we shed new light on the question of the ancestry of one
Thoroughbred patriline. We show the strength of the horse Y chromosome as a genealogical tool,
enlighten recent paternal history of North African horses, and set the foundation for future studies
on the breed and the formation of conservation breeding programs.
Keywords: North African horse; Barb; Arab-Barb; Y chromosome; haplotype
Animals 2022,12, 2579. https://doi.org/10.3390/ani12192579 https://www.mdpi.com/journal/animals
Animals 2022,12, 2579 2 of 13
1. Introduction
The history and origin of the North African horse have been long debated [
1
]. Still,
there is no confirmation of horses inhabiting Africa, or evidence of domesticated horses
roaming around the continent in early prehistoric time, but discussions about an “Equus
Algericus” found near Tiaret (Algeria) still remain [
1
,
2
]. However, historical and archeolog-
ical findings indicate that the introduction of the domesticated horse to North Africa was
likely in the late second millennium BCE, via several routes following human migrations
and conquests (e.g., through Strait of Gibraltar or Egypt) [3–5].
The origin stories of the North African Barb horse lead off the Barbary coast in the
Maghreb region (today’s Algeria, Tunisia, Morocco), hence the name “Barb”. Foremost,
Numidian horses and their crosses are especially discussed as founders of the breed [
6
,
7
].
Complex patterns of human and horse migrations in the North African region peaked
around the 7th century, concurrent with the Muslim conquests [
8
,
9
]. Later, during the
occupation of the Iberian Peninsula by the Moors, from the early 8th to the late 15th century,
migrations between North Africa and Iberian Peninsula were frequently ongoing [
3
,
8
,
10
,
11
]
and the influence of the North African horses onto Iberian stocks was substantial [12,13].
Numerous myths exist on the multilayer history of the Barb horse, for example,
phenotypic traits relate the discussion about the progenitors to Mongolian horses, as well
as the rare light-colored (cream-gene) and piebald (sabino) horses, corresponding to the
Turkoman and the Akhal Teke breed [
1
,
14
]. Barbs had a prominent role as war horses
and for breeding in Europe [
1
,
12
]. Notably, Barb horses were used in the Punic wars
(264–146 BCE)
that were fought between Romans and Carthage, and later exported to
Europe by Carthaginian conquests [
14
]. Likewise, more heavy horses were introduced
to the Maghreb region first by Romans (from 146 BCE) and later in the 17th century by
Louis XIV [
7
]. However, after the 18th century, breeding declined dramatically because
Barb horses were no longer used for the military cavalry, due to the shift of military tactics
that began in the 19th century [
1
,
15
]. More recently, from the end of the 19th century
onwards, cross-breeding of North African and coldblooded horses from France resulted
in the “Breton-Barb”. In addition, crosses of the Barb horse with Thoroughbreds, Anglo-
Arabs, and French Trotters in North Africa were reported [
1
,
12
,
15
]. Above all, systematic
cross-breeding with Arabian horses founded the “Arab-Barb” breed in the Maghreb region.
In the 20th century during both world wars, French colonial cavalry and later also under
Rommel
´
s regime, captured Barb horses and this contributed to their diffusion throughout
Europe [
16
]. Moreover, from 1965 onwards, the African horse sickness significantly reduced
North African Barb horse populations and prevented horse export to Europe for over ten
years from Algeria [17], and from Morocco during 1987–1991 [18].
In 1987, the “Organisation Mondiale du Cheval Barbe (OMCB)” was founded to
preserve the purebred Barb horse and its cross populations (“derivates”), especially the
Arab-Barb horse [
19
]. The OMCB is nowadays recognized as a competent authority for
setting up the breeding programs. Breed registries were only recently established for
Barbs and Arab-Barbs in the Maghreb region (1886 in Algeria, 1896 Tunisia, and 1914
Morocco) [
1
,
14
]. Since then, the studbooks remained open so that phenotypically classified
horses can be entered retrospectively, even if no known ancestry can be proven (defined
as “Inscription àTitre Initial”, “ITI”) [
20
]. Additionally, European registries are established
(in France in 1989, Germany 1992, Switzerland 1993, and in Belgium from 1992–2017)
and their studbooks are closed. Barb horses and the Arab-Barb horses are separated in
different studbooks or studbook sections according to the OMCB stud-book regulations.
The stud-book section for Arab-Barbs is still open for Arab/Barb crosses as well as crosses
of Arab-Barbs with either Barbs or Arabs. All over, studying ancestry and breeding histories
in North African horses via pedigree documentation is limited.
The census population size in the Maghreb countries is about 5500 for Barbs and
180,000 for Arab-Barbs [
21
,
22
]. Out of those, 1800 Barbs and 26,000 Arab-Barbs are regis-
tered in studbooks. In contrast, the European subpopulation constitutes about 2800 Barbs
and 4000 Arab-Barbs, out of which 520 and 440 horses (Barbs and Arab-Barbs, respec-
Animals 2022,12, 2579 3 of 13
tively) are registered for breeding in the OMCB recognized studbooks. They produce about
160 foals per year [
21
,
22
]. The breeding programs for Barbs and Arab-Barbs are mainly
based on characteristic phenotypic traits, robustness, and behavior rather than uniform
breeding goals. Today, these horses are used for “Fantasia” (also known as “Tbourida” in
Morocco and “Mchef ” in Tunisia) a traditional equestrian war game dating back to the
16th century, as well as for agricultural work, carriage, riding, dressage, and equestrian
art, as well as racing (only Arab-Barbs) in North Africa [
1
,
12
,
19
]. In Europe, they are
used as leisure horses, for endurance-riding, historical dressage, jumping, and working
equitation [1,16].
According to the diverse use and breeding areas, the North African Barb and Arab-
Barb horse populations are characterized by broad phenotypic variation [
1
,
22
,
23
]. Within
the Arab-Barbs, this strongly depends on the percentage of Arabian ancestry [
24
,
25
]. In-
vestigation of blood group markers, protein, and DNA polymorphisms in North African
subpopulations showed a pronounced genetic variation within the Barbs and the Arab-
Barbs. Private alleles and high levels of heterozygosity were noted, however, no significant
genetic differentiation was observed between Barb and Arab-Barb populations [
26
–
29
].
Likewise, apparent phenotypic differences distinguish the purebred Barb horse from the
Arabian horse [
1
,
23
,
25
,
30
,
31
]. Microsatellite analysis showed similarities between the
Arab-Barb and Arabian horses and a clear genetic separation of both breeds from Thor-
oughbreds [
27
–
29
]. The maternally inherited mitochondrial DNA showed close genetic
relationships between Iberian breeds and Barb horses [
11
,
32
]. Nevertheless, the relationship
between the North African Barb and the Arab horse has been continuously debated, till
today [33].
A prominent genetic marker for inferring the ancestry of populations is the non-
recombining, male-specific region of the Y chromosome (MSY). The MSY is inherited
exclusively from the father to his sons and thus MSY haplotypes (HTs) mirror the paternal
lineages in a population. MSY analysis is best established in humans where it is widely
used in population genetics, genealogical research, and forensics [
34
–
36
]. In domestic
horses, the MSY was long excluded from population genetic studies due to the lack of
informative sequence polymorphism (reviewed in [
37
]). Nevertheless, a stable MSY HTs
topology based on slowly evolving biallelic markers was constructed by mapping next
generation sequencing (NGS) data to a 6.5 Mb horse MSY draft reference [
38
]. The MSY
HTs of domestic horses are clearly distinct from those in the extant Przewalski’s horses. The
most pronounced MSY signature among domestic horses is the ~2000-year-old “Crown”
haplogroup (HG), recounting various breeds from Central and South Europe, East Asia,
North and South America [
38
,
39
]. It was proposed that the dominance of the Crown HG is
a hallmark of the recent breeding influence of stallions of Oriental origin [
38
,
40
]. The crown
topology supports the hypothesis [
41
,
42
] that only a limited number of stallions contribute
to today
´
s horse population. Only some Asian horses [
43
,
44
] and Northern European
breeds (e.g., [
45
]) seemed to be unaffected by the recent Oriental introgression, and thus
kept their autochthonous HTs outside the Crown (“Non Crown”). Within the Crown, three
HGs were defined (H, A, and T) and the HT signatures of three English Thoroughbred
founders [38], as well as Arabian patrilines [39] were recently successfully delineated.
In horses, MSY analysis can unmask patrilines that contributed to a breed; thus, impart
motifs of their male demography, and shed light on complex breeding histories. In this
study, we investigated MSY HTs in North African Barb horses with the aim to link Y-
chromosomal patterns to narratively known historical events. We hypothesize that the
long-lasting input of foreign blood and complex migrations in the Maghreb region will be
mirrored in their MSY HT spectrum. In addition, due to indigenous origin, regional and
less intensive selection strategies [
1
], we might detect the preservation of autochthonous
HTs in some North African horses’ patrilines.
Animals 2022,12, 2579 4 of 13
2. Materials and Methods
2.1. Sample Set
Biological samples were collected from 119 males, of Barbs (n = 84) and Arab-Barbs
(n = 35)
in Morocco, Algeria, Tunisia, and the European subpopulations. To ensure that
many patrilines were represented in the dataset, pedigree information (available for
86 horses
), provided by breeding authorities and associations, was considered in the sam-
pling strategy as previously described [39]. Hence, oversampling of relatives was averted
from the dataset by keeping six males per foundation sire at maximum. Additionally,
we included 33 randomly sampled horses without pedigree information (10 European
and 23 North African samples) to complement and capture population variation beyond
documented patrilines. The dataset including individual male tail line information for
ancestors born prior to 1990 is given in a string format in Table S1.
2.2. MSY Genotyping
We inferred MSY haplotype spectrum of 119 samples according to the previously
reported horse Y phylogeny [
38
,
39
]. For genotyping, we created a downscaled HT structure
based on 65 selected HT-determining variants as markers (61 SNVs, 3 short Indels, and
1 microsatellite, see Supplementary Table S2). The resulting tree served as the backbone
and samples were placed onto branches of the tree via MSY marker screening.
For variant screening, genomic DNA was isolated from hair roots or blood with the
nexttec
®
DNA Isolation Kit. The DNA was then diluted with TE buffer to the uniform
concentration of 5 ng/
µ
L. Genotyping of variants was performed using competitive allele-
specific PCR SNV genotyping assays (KASP
™
, lgcgroup.com (accessed on 2 July 2021)),
following the standard protocol on a CFX96 Touch
™
Real-Time PCR Detection System.
Samples with known allelic state were included as positive controls, while DNA from
females and non-template controls were used as negative controls. Information on variants
(coordinates on LipY764, alleles, and flanking regions) are published in [38,39].
Genotyping of the amplicon length of the tetranucleotide microsatellite fBVB (GATA14
/GATA15) was performed on an ABI 3130xl Genetic Analyzer, as previously described [
38
].
In synopsis, for the fragment analysis, one PCR primer was tagged with FAM fluores-
cent dye (fwd_FAM: ACAACCTAAGTGTCTGTGAATGA; rev: CCCAATAATATTCCACT-
GCGTGT, expected amplicon length 204 bp). PCR was carried out in a 20
µ
L reaction
volume containing 0.4
µ
M of each primer. The reaction temperature was increased to 95
◦
C
for 5 min for initial DNA denaturation, followed by 35 cycles of 30 s at 95
◦
C, 40 s at 58
◦
C
annealing temperature and 40 s at 72
◦
C, and a final extension step of 30 min at 72
◦
C.
Finally, GeneMarker®was used to size the alleles relative to the internal size standard.
Genotyping was conducted in a consecutive manner by first testing the Crown deter-
mining variant rAX. If a sample carried the derived C-allele for this variant, allocation of the
sample into main Crown HGs H, A, or T was conducted by testing markers fYR, rW, and rA.
Each sample was then typed for the markers determining the substructure of the HG it clus-
ters into. We then merged the genotyping information of all tested variants and imputed
the allelic state of markers that were not tested or detected in the sample set according to
the previously published HT structure [
38
,
39
] (see Figure 1and
Supplementary Table S2
).
We generated a median-joining HT network with program Network 10.2 [
46
] and redrew
it as a HT frequency plot (Figure 1) in Canva Pro (https://www.canva.com (accessed on
29 June 2022
)). Pie charts were drawn and scaled to the respective number of samples with
RStudio version 4.0.3. [47].
Animals 2022,12, 2579 5 of 13
Animals 2022, 12, x 5 of 13
Figure 1. MSY haplotype spectra of North African horses. (a) HT frequency plot based on the MSY
tree after [38,39]. HT determining variants used to construct the downscaled tree for genotyping are
denoted on branches in red. Additional information is given in Supplement, Table S2. Clustering of
119 North African horses based on genotyping result is illustrated as pies. Pie radiuses are scaled to
the number of allocated individuals and colors of the portions correspond to different breeds. HG
names are labeled accordingly. HTs located on internal nodes are denoted with an asterisk (*) and
trailed with dashed lines that originate from corresponding internal nodes. Unascertained variants
that would determine * HTs are denoted with question marks (?). HTs framed with blue and/or red
borders denote that they were detected previously in Arabian (blue border) and Thoroughbred (red
border) horses [38,39]. Non-colored points express HTs that were not detected in the North African
sample set. Gray list on the sides of the network indicates the breeds the HTs were previously re-
ported [38–40]; (b) Number of individuals that allocate within detected HTs. Sample information
details are given in Supplement Table S1.
3. Results
To investigate the MSY HT spectra of North African horses, 119 males representing
84 Barbs and 35 Arab-Barbs were genotyped. The results showed that all samples allo-
cated into the Crown HG. In total, we distinguished 18 HTs and all three previously de-
fined Crown HGs (A, H, and T) were represented in our sample set. The broad Crown
MSY HT spectra was comparable in Barbs and Arab-Barbs (Figure 1). This is in contrast
to patterns in other today`s breeds [38,39] that showed distinct clustering on the tree. Re-
markably, only half of the males analyzed carried defined HTs, whereas 61 males got
placed at internal nodes of the backbone topology (See Figure 1 and Table S2). The sam-
ples allocated at inner nodes are marked with an asterisk (*) in their HT identifier and
distinguished with dashed lines in Figure 1. For instance, the sample that allocates into
Tb-oB* HT carried the derived allele for the fUJ marker and was placed onto the branch
Tb-oB, but it carried the ancestral allele at the markers determining subsequent HTs in
our backbone tree (rP, qFM, fQI, and fBVB). The inner node clustering of samples occurs
when the HT of the horse is not represented by the tree due to ascertainment bias, and
only the HG and the branching point could be determined.
More than half (56%, n = 67) of the analyzed individuals are distributed across two
HGs, Am (n = 34) and Hs-b (n = 33), respectively (see Figure 1). Other than North African
horse, these HGs were so far only detected in some South American and Iberian breeds
Figure 1.
MSY haplotype spectra of North African horses. (
a
) HT frequency plot based on the MSY
tree after [
38
,
39
]. HT determining variants used to construct the downscaled tree for genotyping are
denoted on branches in red. Additional information is given in Supplement, Table S2. Clustering of
119 North African horses based on genotyping result is illustrated as pies. Pie radiuses are scaled to
the number of allocated individuals and colors of the portions correspond to different breeds. HG
names are labeled accordingly. HTs located on internal nodes are denoted with an asterisk (*) and
trailed with dashed lines that originate from corresponding internal nodes. Unascertained variants
that would determine * HTs are denoted with question marks (?). HTs framed with blue and/or
red borders denote that they were detected previously in Arabian (blue border) and Thoroughbred
(red border) horses [
38
,
39
]. Non-colored points express HTs that were not detected in the North
African sample set. Gray list on the sides of the network indicates the breeds the HTs were previously
reported [
38
–
40
]; (
b
) Number of individuals that allocate within detected HTs. Sample information
details are given in Supplement Table S1.
3. Results
To investigate the MSY HT spectra of North African horses, 119 males representing
84 Barbs and 35 Arab-Barbs were genotyped. The results showed that all samples allocated
into the Crown HG. In total, we distinguished 18 HTs and all three previously defined
Crown HGs (A, H, and T) were represented in our sample set. The broad Crown MSY HT
spectra was comparable in Barbs and Arab-Barbs (Figure 1). This is in contrast to patterns
in other today‘s breeds [
38
,
39
] that showed distinct clustering on the tree. Remarkably, only
half of the males analyzed carried defined HTs, whereas 61 males got placed at internal
nodes of the backbone topology (See Figure 1and Table S2). The samples allocated at
inner nodes are marked with an asterisk (*) in their HT identifier and distinguished with
dashed lines in Figure 1. For instance, the sample that allocates into Tb-oB* HT carried the
derived allele for the fUJ marker and was placed onto the branch Tb-oB, but it carried the
ancestral allele at the markers determining subsequent HTs in our backbone tree (rP, qFM,
fQI, and fBVB). The inner node clustering of samples occurs when the HT of the horse is
not represented by the tree due to ascertainment bias, and only the HG and the branching
point could be determined.
Animals 2022,12, 2579 6 of 13
More than half (56%, n = 67) of the analyzed individuals are distributed across
two HGs, Am (n = 34) and Hs-b (n = 33), respectively (see Figure 1). Other than North
African horse, these HGs were so far only detected in some South American and Iberian
breeds [
35
,
36
]. Besides, we observed grouping of 28 (24%) males into Ao-aA1a* and Ao-
aD2 HTs. Those HTs were designated recently as signatures for Arabian horses [
39
]. The
arrangement of the internal branching points in the strictly hierarchical MSY HT tree
topology reflects the emergence of the mutations over time. Hence, the HTs Ao-aA* (n = 2)
and Ao-aA3 (n = 2) can be interpreted as hints to earlier introduced lines of presumably
Arabian origin, that evolved and are still preserved in the North African Barb horse. We
further aggregated ten males in the Tb HG. Among those, two males clustered onto early
branching points (T2* and Tb-oB*) and six were allocated in the HT Tb-oB1*. This HT
was previously reported in Akhal Teke, Turkoman, Thoroughbreds, as well as Arabian
horses [
38
–
40
]. The Tb-oB1* in North African horses can be explained as the recent influ-
ence of stallions from that region. Noteworthy, we detected Tb-oB3b1*, the HT basal to
the HTs detected in the progeny of the Thoroughbred
´
s founder sire ‘Godolphin Arabian’,
which are (Tb-oB3b1a/b/c) [
38
], in a Barb breeding stallion from Morocco. We found the
signature of recent influence of Warmblood or Thoroughbred in a single horse from France
carrying Tb-oB3b1b, but did not observe the typical Thoroughbred and Trotter HGs Tb-dW
and Tb-dM [
38
,
40
]. Moreover, ten males carried HGs, which are today mainly found in
Coldbloods and European Ponies [
39
,
40
], namely Ad-h (8), Ad-b (1), and Ao-n (1). Here,
we again observed well resolved HTs (for example Ad-hA1), as well as earlier branching
off HTs (Ad-bN*, Ad-h*).
Roughly half of our sample set was collected in Europe and the other half in Algeria,
Morocco, and Tunisia (see Figure 2and Table S1). The samples from Algeria and Morocco
clustered in 8 HTs each. The European samples clustered into 16 HTs. Seven HTs were
represented only within this population group in our sample set, noting that two HTs,
Ad-hA* and Tb-oB*, were detected in ITI horses directly imported from, respectively,
Algeria and Morocco. The broad HT spectrum detected in samples collected in Algeria,
Morocco, and Europe was not corroborated by Tunisian data. All collected Barbs (n = 9)
and Arab-Barbs (n = 2) from Tunisia and all males exported from Tunisia to Europe (see
below) allocated into HT Hs-bL.
Animals 2022, 12, x 6 of 13
[35,36]. Besides, we observed grouping of 28 (24%) males into Ao-aA1a* and Ao-aD2 HTs.
Those HTs were designated recently as signatures for Arabian horses [39]. The arrange-
ment of the internal branching points in the strictly hierarchical MSY HT tree topology
reflects the emergence of the mutations over time. Hence, the HTs Ao-aA* (n = 2) and Ao-
aA3 (n = 2) can be interpreted as hints to earlier introduced lines of presumably Arabian
origin, that evolved and are still preserved in the North African Barb horse. We further
aggregated ten males in the Tb HG. Among those, two males clustered onto early branch-
ing points (T2* and Tb-oB*) and six were allocated in the HT Tb-oB1*. This HT was previ-
ously reported in Akhal Teke, Turkoman, Thoroughbreds, as well as Arabian horses [38–
40]. The Tb-oB1* in North African horses can be explained as the recent influence of stal-
lions from that region. Noteworthy, we detected Tb-oB3b1*, the HT basal to the HTs de-
tected in the progeny of the Thoroughbred´s founder sire ‘Godolphin Arabian’, which are
(Tb-oB3b1a/b/c) [38], in a Barb breeding stallion from Morocco. We found the signature of
recent influence of Warmblood or Thoroughbred in a single horse from France carrying
Tb-oB3b1b, but did not observe the typical Thoroughbred and Trotter HGs Tb-dW and
Tb-dM [38,40]. Moreover, ten males carried HGs, which are today mainly found in Cold-
bloods and European Ponies [39,40], namely Ad-h (8), Ad-b (1), and Ao-n (1). Here, we
again observed well resolved HTs (for example Ad-hA1), as well as earlier branching off
HTs (Ad-bN*, Ad-h*).
Roughly half of our sample set was collected in Europe and the other half in Algeria,
Morocco, and Tunisia (see Figure 2 and Table S1). The samples from Algeria and Morocco
clustered in 8 HTs each. The European samples clustered into 16 HTs. Seven HTs were
represented only within this population group in our sample set, noting that two HTs,
Ad-hA* and Tb-oB*, were detected in ITI horses directly imported from, respectively, Al-
geria and Morocco. The broad HT spectrum detected in samples collected in Algeria, Mo-
rocco, and Europe was not corroborated by Tunisian data. All collected Barbs (n = 9) and
Arab-Barbs (n = 2) from Tunisia and all males exported from Tunisia to Europe (see below)
allocated into HT Hs-bL.
Figure 2. Geographical representation of MSY haplotypes. Populations analyzed are denoted with
different colors and circles on the map correspond to the sample size. Details are given in Supple-
ment, Table S1. Summary information of genotyping results and regional differences are visualized
Figure 2.
Geographical representation of MSY haplotypes. Populations analyzed are denoted with different
Animals 2022,12, 2579 7 of 13
colors and circles on the map correspond to the sample size. Details are given in
Supplement, Table S1
.
Summary information of genotyping results and regional differences are visualized with bar plots.
The x axis on the bar plots corresponds to detected HTs, while the y axis indicates number of samples
that correspond to each of the bars (HTs). The samples assigned to inner nodes are marked with
an asterisk (*) in their HT identifier. Red stars indicate HGs that were found exclusively in the
corresponding subpopulation (e.g., seven HGs denoted with red stars in the European subpopulation
are found only among samples collected in European countries, and were not observed in samples
from Maghreb countries).
Among the 66 European samples, nine were collected from horses imported from
Algeria (4), Morocco (4), or Tunisia (1). Complementing pedigree information was available
for another 56 European samples (see Supplementary Table S1). This documentation reveals
that the majority, namely 50, of the European males also directly trace back paternally
to Maghrebian stallions exported from Algeria, Morocco, and Tunisia to Europe during
the last 35 years (see Figure 3and Supplementary Table S1). Hence, only seven out of
the 66 males in the European dataset could not be linked explicitly to a hitherto known
Maghrebian line from documented records. Among those, five individuals descend from
four stallions, who were inscripted as ITI in the course of the foundation of the French
studbook in 1989. For one sample, we had no pedigree information, and for one founder,
the country of origin was unknown (see Supplementary Table S1).
Overall, the full dataset (n = 119) included 33 individuals without pedigree information
(10 European and 23 horses from Maghreb) and the HT pattern in horses with and without
pedigree were comparable (Supplementary Table S1).
Animals 2022, 12, x 7 of 13
with bar plots. The x axis on the bar plots corresponds to detected HTs, while the y axis indicates
number of samples that correspond to each of the bars (HTs). The samples assigned to inner nodes
are marked with an asterisk (*) in their HT identifier. Red stars indicate HGs that were found exclu-
sively in the corresponding subpopulation (e.g., seven HGs denoted with red stars in the European
subpopulation are found only among samples collected in European countries, and were not ob-
served in samples from Maghreb countries).
Among the 66 European samples, nine were collected from horses imported from
Algeria (4), Morocco (4), or Tunisia (1). Complementing pedigree information was avail-
able for another 56 European samples (see Supplementary Table S1). This documentation
reveals that the majority, namely 50, of the European males also directly trace back pater-
nally to Maghrebian stallions exported from Algeria, Morocco, and Tunisia to Europe dur-
ing the last 35 years (see Figure 3 and Supplementary Table S1). Hence, only seven out of
the 66 males in the European dataset could not be linked explicitly to a hitherto known
Maghrebian line from documented records. Among those, five individuals descend from
four stallions, who were inscripted as ITI in the course of the foundation of the French
studbook in 1989. For one sample, we had no pedigree information, and for one founder,
the country of origin was unknown (see Supplementary Table S1).
Figure 3. Maghrebian roots of European stallions. Fifty-nine European individuals, who were im-
ported or their patrilines trace back to North Africa, are grouped based on their current registry
(blue boxes). Number of horses included from Austria (n = 8), Switzerland (n = 2), Germany (n = 28),
and France (n = 21) are denoted in square brackets. The paternal ancestors of the sampled individ-
uals several generations back in time, as well as present individuals imported to France and Ger-
many, are shown as colored boxes. The opacity of boxes indicates temporal layers whereas the
brightest boxes on the bottom are present ITI horses, followed by recent ancestors born after 1990
(Ancestor A, B, C, D, and E), and lightest colored distant ancestors, in the middle. Name and year
of the birth of ancestors is given for distant ancestors. MSY HTs, revealed from the European prog-
eny, are shown within each stallion’s box. HT identifiers attributed with asterisk (*) denote inner
node clustering. The grey lines connect the stallions with their descendants sampled in the respec-
tive European countries. Numbers in the brackets and adjacent to the left side of connection lines
represent the number of descendants from each stallion found in European samples, if different
from one. Pedigree details and full list of samples are given in Supplementary Table S1.
Figure 3.
Maghrebian roots of European stallions. Fifty-nine European individuals, who were
imported or their patrilines trace back to North Africa, are grouped based on their current registry
(blue boxes). Number of horses included from Austria (n = 8), Switzerland (n = 2), Germany (n = 28),
and France (n = 21) are denoted in square brackets. The paternal ancestors of the sampled individuals
several generations back in time, as well as present individuals imported to France and Germany, are
shown as colored boxes. The opacity of boxes indicates temporal layers whereas the brightest boxes
on the bottom are present ITI horses, followed by recent ancestors born after 1990 (Ancestor A, B, C, D,
and E), and lightest colored distant ancestors, in the middle. Name and year of the birth of ancestors
is given for distant ancestors. MSY HTs, revealed from the European progeny, are shown within each
stallion’s box. HT identifiers attributed with asterisk (*) denote inner node clustering. The grey lines
Animals 2022,12, 2579 8 of 13
connect the stallions with their descendants sampled in the respective European countries. Numbers
in the brackets and adjacent to the left side of connection lines represent the number of descendants
from each stallion found in European samples, if different from one. Pedigree details and full list of
samples are given in Supplementary Table S1.
4. Discussion
The significant role of North Africa, as a transit route, during the Islamic conquest and
migratory movements between countries of the region [
3
,
14
], raised our interest on the Y
chromosomal signature of North African Barb horses. While the MSY HT signatures of the
Arabian and the Thoroughbred and their recent breeding influences are well described [
38
,
39
],
the historically impactful North African horse remains enigmatic. We applied MSY haplotyping
in a total of 84 Barbs and 35 Arab-Barbs, whereas half of our samples were collected in Europe
and the other half in Algeria, Tunisia, and Morocco (see Figure 2and Supplementary Table S1)
and hypothesized that the MSY signature will mirror the variety of encountered influences. On
the other hand, due to the documented indigenous origin and regional subgroups in North
Africa, we expected partial representation of autochthonous patrilines.
The results of haplotyping indicate that no distantly related lineages were retained
in the collected sample set since all horses clustered within the Crown HG. In line with
previously determined time to the most recent common ancestor [
38
], we can state that
the MSY of North African horses only reflects the last 1500 years of population history.
The sole detection of the Crown mirrors influences of Oriental stallions [
40
]. Interestingly,
we report a broad HT spectrum of North African horses across the Crown HGs (18 HTs).
However, unlike other breeds (like Arabians and Thoroughbreds), for which it was possible
to pin-point characteristic HGs and even discriminate discrete sublines with the use of
pedigrees [
38
,
39
], the diffused HT distribution result in a tangled MSY footprint of North
African horses. The observed preservation of a variety of HTs may be the consequence
of less intensive selection on males and different breeding goals in North African regions.
Interestingly, MSY results were comparable in Barbs and Arab-Barbs. This verifies the
inter-crossing and gene flow till today between the North African horse populations, as
already depicted with autosomal genetic markers [27,28,48].
However, the broad HT spectrum was not supported from Tunisian samples
(n = 11)
,
where all nine Barbs and two Arab-Barbs were monomorphic, carrying a single HT (Hs-bL)
(Figure 2). This may demonstrate geographical disparities in breeding goals, supported
by regional differences reported in the phenotype [
1
,
23
,
30
], as well as genetic spatial
interpolation (e.g., [
27
]). In contrast, the analysis of microsatellites resulted in similarity of
Moroccan and Tunisian Barb horse populations [
29
]. Regional differences are highlighted
when we compare the HTs represented in Europe to the Maghreb region. Samples from
European countries harbored seven HTs that were not represented in the samples collected
in North Africa. Three of those patrilines were imports from North Africa after 2001 and
four HTs trace back to the French ITI-inscriptions in 1989. Their private HTs may be
explained with geographical separation of former exports to France. Additionally, we
found two HTs each private for Moroccan and Algerian Barbs (Tb-oB3b1* and Ad-bN*,
respectively). Compared to Tunisia, we observe similar MSY patterns in Europe, Morocco,
and Algeria. One explanation for greater similarity of HTs among the latter three could be
the tighter historical connection between those regions (export especially of ITI horses from
Morocco and Algeria to Europe as seen in Figure 3). Nevertheless, we should interpret these
findings with caution since it is possible that despite our efforts to collect a representative
sample set from the Maghreb, the numbers of horses available from Tunisia was lower
(n = 11). Hence, we could have underestimated HT diversity in that region.
All we see today is what is left throughout the time, and the MSY is a perfect tool
to trace patrilines that shaped present populations. The relationship between the North
African Barb and the Arabian horse has been continuously debated [
33
]. We noted a
prominent clustering to Ao-aA1*, a HG previously detected in Arabian lines [
39
]. The
detection of numerous Arabian HTs demonstrates the significant influence of Arabian
Animals 2022,12, 2579 9 of 13
stallion lines in Barbs and Arab-Barbs. A clear Arabian signature was visible in about a
third of the analyzed samples. For the Arab-Barbs, the results are not surprising since
the breed is based on Barbs refined with Arabians [
49
]. On the other hand, assignment of
“purebred Barbs” to Arabian HGs may reflect, as hypothesized, recent historical migratory
movements resulting in admixture, because the studbooks for the “purebred Barbs” are
still open in North Africa and stallions without pedigrees are used for breeding.
Two third of the analyzed samples (85 North African horses) did not carry the Arabian
signature HTs. Particularly interesting is that among those were 27 Arab-Barbs. In addition,
we detected indications of recent upgrading with European Coldbloods in four males
(Ad-hA1), which could be explained with the discussed influence of Coldblood stallions
imported to North Africa [
12
]. Moreover, only a single individual carried an unambiguous
sign of Warmblood or Thoroughbred male ancestry (Tb-oB3b1b) [38].
Barbs were used for upgrading and formation of many modern breeds [
12
,
50
]. There
have also been reports on their contribution to Thoroughbreds, Anglo-Arabs, and French
Trotters. Interestingly, North African horses
´
HTs share branching points basal to the HTs
observed in many todays Coldblood, British and European Ponies (Figure 2; detected in
Ad-h, Ad-b, and Ao-n HTs) [
39
,
40
], which can be interpreted as the influence of the North
African horses had on those breeds further back in time. Deeper investigation is needed to
validate the proposed correlation.
A particularly remarkable finding was the observation of the HT basal to the HTs
spread through the Godolphin Arabian sire line (Tb-oB3b1*) [38] in a Barb horse. There is
still controversy about the ancestry of Godolphin Arabian, one of the foundation sires of the
English Thoroughbred (exported from Tunisia to France in 1731). He is often referred to as
Godolphin Barb due to his North African origin [
51
] and phenotypic marks different from
the Arabian horse [
1
,
12
,
13
]. The MSY finding, namely detection of the basal Godolphin Barb
HT in a Barb horse, again fuels the discussion on the origin of Godolphin Arabian, whether
he was a Turkoman stallion with partial Arabian blood [
52
] or corroborates the hypothesis
that the Tb-oB3b1 HG made its way into the Thoroughbred via the Barb horse [1,49].
When we look further back in time, from the Carthaginian civilization in the 1st
century and Muslimic conquests in the 7th century to recurrent migrations with Iberian
Peninsula (8th to 15th century), North Africa served as a main migratory route for many
cultures [
3
,
14
]. Every culture that was present in the region could have left footprints
in the horses’ genomes, and this was depicted on the MSY. Notably, influence from the
Middle East could be attributed to inner clustering of individuals to Ao-aA* and Tb-oB*, as
well as allocation to Ao-aA3, Ao-aD2, Tb-oB1*, and T2* HGs. This grouping may indicate
previously discussed influence of the ancestors of Arabian and Turkoman lineages on North
African horses.
From the viewpoint of interactions between the North African regions and the Iberian
Peninsula, previous research delineated homogenous mtDNA patterns within ancient [
53
]
and modern [
11
,
32
] horse populations in Iberia and North Africa. Particularly, it is specu-
lated that Barb and Iberian horses have a common origin [
54
]. A great number of North
African horses that were analyzed [
32
] shared mtDNA HTs reported in South American
and Iberian breeds. Accordingly, we note that two highly frequent HGs (Am and Hs-b) rep-
resented in our dataset also allocate Iberian and New World horse breeds, like Marchador
(Am), Lusitano, and Sorraia (Hs-b) [
39
]. Iberian and New World breeds are not yet compre-
hensively studied for their MSY HTs, but the preliminary joint clustering could reflect the
gene flow and recent shared ancestry of North African Barb and Iberian horses. However,
to fully explain the assumed shared ancestry further back in time, as well as the magnitude
of gene flow, and indices on New World horses
´
ancestry, we should complement the
dataset with additional Iberian and New World horse breeds in the future. Early separated
populations, like the West African Barb, the Spanish Barb (USA), and South American
breeds, as well as ancient DNA samples from the Maghreb, should enlighten another
chapter in horse history. Additionally, basal allocation of samples in the tree topology and
underrepresentation of private HTs (Figure 1) raises a discussion on technical limitation
Animals 2022,12, 2579 10 of 13
of our analysis. The MSY backbone topology was constructed based on the ascertainment
panel from [
39
], where five Barbs and one Arab-Barb were sequenced. However, it seems
this is still insufficient, and more individuals need to be sequenced in order to clarify MSY
signatures private for North African horses, in particular in HGs Hs-b, and Am.
Overall, North African horses retained the print of the “early Oriental influence”
starting with the Muslim conquests. With the observed broad HT spectrum, these horses
could be a reservoir of genetic diversity—although their population is small. Further
investigation of additional males, especially from the Maghreb regions, is needed to precise
influential patrilines, as this is of particular practical interest for breeding. The MSY
patterns should be considered together with autosomal markers, as well as mitochondrial
DNA, while constructing necessary conservation breeding programs, to preserve the North
African Barb horse.
5. Conclusions
Our study highlights the value of the Y chromosome analysis for horse population
genetics and for the first time, enlightens recent paternal population history of the North
African Barb horses. Obtained MSY HT spectra point to, on the one hand, that stallions
were probably wide-spread hundreds of years preceding the formation of modern horse
breeds, and on the other hand, indicate the impact on historical migrations and recent
upgrading. However, with our approach, it is at the moment not possible to pin-point
where and when the ancestors of North African Barbs came from, as well as the direction
of gene flow. Future analysis on ancient DNA, as well as inclusion of more diverse Barb
populations, are essential for dating of the origin of HGs, and exact inference of genetic
influences. In addition, the ascertainment bias represented with HTs that are not fully
resolved indicates that, even though the Crown is well described, there is still a lot left
to explore in future research. Finally, our findings enhanced our knowledge of paternal
ancestry of the breed and provided basis for future work and establishment of conservation
breeding programs.
Supplementary Materials:
The following supporting information can be downloaded at: https:
//www.mdpi.com/article/10.3390/ani12192579/s1, Table S1: Sample set information; Table S2:
Genotyping results; Table S3: Variant information.
Author Contributions:
Conceptualization of the project was completed by L.R., V.R., I.v.B.-W. and
B.W. Funding acquisition was performed by B.W. Methodology was determined by L.R. and B.W.
Data collection was performed by L.R., V.R., C.K. and D.R. Resources were provided by A.R., K.D.,
M.B., D.K., I.v.B.-W. and B.W. Data analysis was performed by L.R., V.R. and B.W. The original draft
was written by L.R. and B.W. Writing—review and editing was done by L.R., V.R., D.R., G.B., A.R.,
K.D., M.B., M.M., M.P., D.K., I.v.B.-W. and B.W. Supervision of the project was performed by B.W. All
authors have read and agreed to the published version of the manuscript.
Funding: This research received no external funding.
Institutional Review Board Statement:
The study was discussed and authorized by the University
of Veterinary Medicine Vienna
´
s institutional ethics and welfare committee in accordance with GSP
guidelines and national legislation (ETK-10/05/2016). The study was carried out in compliance with
the applicable guidelines specified in the preceding document.
Informed Consent Statement:
The biological material (hair roots or blood samples) and permission
of use were obtained from breeding associations and private horse owners. If pedigree data were
available, informed consent was acceded. All samples used in the study are coded.
Data Availability Statement: Not applicable.
Acknowledgments:
The authors thank all horse owners who contributed with samples. We thank
GeneControl GmbH Grub, Germany for providing retained hair samples from the VFZB registered
male horses, and especially Petra Jürgens (Germany), Jessica Pfeiffer (Austria), Veronika Leichtfried
(Austria), Claudia Lazzarini (Switzerland), Caroline Duffeau (France), Claire Martin (France), and
Animals 2022,12, 2579 11 of 13
Bénédicte Fournel (France). We also thank Royal Horse Breeding Association (SOREC, Morocco) for
the support.; Open Access Funding by the University of Veterinary Medicine Vienna.
Conflicts of Interest:
The authors declare no conflict of interest. The funders had no role in the design
of the study; in the collection, analyses, or interpretation of the data; in the writing of the manuscript
or in the decision to publish the results. The statements made herein are solely the responsibility of
the authors.
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