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Open Access

Peer-reviewed

Research Article

First sex modification case in equine cloning

Abstract

Somatic cell nuclear transfer (SCNT) is an asexual reproductive technique where cloned offspring contain the same genetic material as the original donor. Although this technique preserves the sex of the original animal, the birth of sex-reversed offspring has been reported in some species. Here, we report for the first time the birth of a female foal generated by SCNT of a male nuclear donor. After a single SCNT procedure, 16 blastocysts were obtained and transferred to eight recipient mares, resulting in the birth of two clones: one male and one female. Both animals had identical genetic profiles, as observed in the analysis of 15-horse microsatellite marker panel, which confirmed they are indeed clones of the same animal. Cytogenetic analysis and fluorescent in situ hybridization using X and Y specific probes revealed a 63,X chromosome set in the female offspring, suggesting a spontaneous Y chromosome loss. The identity of the lost chromosome in the female was further confirmed through PCR by observing the presence of X-linked markers and absence of Y-linked markers. Moreover, cytogenetic and molecular profiles were analyzed in blood and skin samples to detect a possible mosaicism in the female, but results showed identical chromosomal constitutions. Although the cause of the spontaneous chromosome loss remains unknown, the possibility of equine sex reversal by SCNT holds great potential for the preservation of endangered species, development of novel breeding techniques, and sportive purposes.

Citation: Suvá M, Arnold VH, Wiedenmann EA, Jordan R, Galvagno E, Martínez M, et al. (2023) First sex modification case in equine cloning. PLoS ONE 18(1): e0279869. https://doi.org/10.1371/journal.pone.0279869

Editor: Wei Cui, University of Massachusetts Amherst, UNITED STATES

Received: June 16, 2022; Accepted: December 15, 2022; Published: January 4, 2023

Copyright: © 2023 Suvá et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Data Availability: All relevant data are within the paper and its Supporting Information files.

Funding: The authors received no specific funding for this work.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Somatic cell nuclear transfer (SCNT) is an asexual reproductive technique commercially available in horses. It is mainly applied to multiply elite individuals [1, 2], but also to reintroduce valuable genomic backgrounds to breeding programs in cases where the original horse has died or is no longer fertile [3]. General interest in SCNT technology is based on the fact that cloned offspring contain the same genomic information as the original donor. However, genomic alterations have been sporadically found in clones of some species. Some of the most striking examples are related to sex modification in the cloned offspring. In the mouse, a female offspring was born from a male nuclear donor as a consequence of the spontaneous loss of the Y chromosome [4]. In dogs, incomplete epigenetic reprogramming after SCNT led to a hypermethylated Y chromosome, resulting in genetically male (XY) animals with a female phenotype [5, 6]. A similar result was reported in wolves, although the cause of sex reversal was not defined [7]. In horses, and despite the numerous clones born to date, no sex-associated genetic alterations have been described to the best of our knowledge. Here, we report a viable female horse born by SCNT of a male nuclear donor. This is the first report of sex modification in equine cloning, which opens the door to sex manipulation by SCNT in this species.

Results

Passage-2 mesenchymal stem cells (MSCs) derived from a male horse were used as nuclear donors for a standard SCNT procedure performed in November 2019 (Table 1). Two live foals were born in November 2020, one male–as expected, considering the sex of the nuclear donor–and one female (Fig 1). At the time of birth, the female foal showed no anatomic abnormalities, although internal reproductive structures could not be observed yet given the animal’s young age. At the age of 2 years, it still shows normal external genitalia, with a normally sized and shaped vulva and clitoris. Ultrasonographic evaluation was performed, and showed a normal uterus but small underdeveloped ovaries (right: 10 x 6 mm; left: 7 x 5 mm), suggesting gonadal hypoplasia. In addition, there was no sign of corpora lutea.

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Fig 1. Foals born after a SCNT procedure using male-horse-derived MSCs as nuclear donors.

Male: left, female: right.

https://doi.org/10.1371/journal.pone.0279869.g001

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Table 1. In vitro and in vivo development of embryos obtained after a SCNT procedure using MSCs of a male donor.

https://doi.org/10.1371/journal.pone.0279869.t001

Genotyping of the born foals

In order to determine whether the two born clones are indeed genetically identical, hair samples from each foal were genotyped with a 15-horse microsatellite marker panel (Fig 2). Analyses rendered identical genotypes, which showed that both foals are indeed clones derived from the same donor. To evaluate possible mosaicism in the female clone, a blood sample was also analyzed, with results showing the same profile in both hair and blood samples.

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Fig 2. Microsatellite profiles from the foals.

Results from the analysis of a 15-panel of microsatellites, used for routine parentage and identity purposes.

https://doi.org/10.1371/journal.pone.0279869.g002

Cytogenetic and molecular analysis of the sex chromosomes

After confirming that the female and male foals are clones, cytogenetic analyses were carried out to elucidate the cause of this sex modification. Fibroblast (n = 30) and blood samples (n = 100) obtained from the female and male clones were evaluated by conventional Giemsa staining, C banding and G banding to determine the chromosome number and sex chromosome constitution. In addition, the MSCs used as nuclear donors (n = 80) were also analyzed. The MSCs (Fig 3A and 3B) and the samples from the male foal (Fig 3C) showed the expected 64,XY chromosome set, whereas the samples from the female foal presented a 63,X chromosome set (Fig 3D). In addition, fluorescence in situ hybridization (FISH) using X and Y specific probes on the MSCs (n = 268) and blood samples from the male (n = 278) and female (n = 309) clones confirmed the X monosomy in the female foal (Fig 4A and 4B), and the normal male sex chromosome configuration in the male foal and donor MSCs (Fig 4C and 4D, respectively).

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Fig 3. Representative metaphase spreads from the foals and the donor MSCs.

(A) G banding and (B) C banding from the MSCs used as nuclear donors (64,XY). (C) C banding from the male clone (64,XY). (D) C banding from the female clone (63,X). Arrows indicate the Y chromosome and arrowheads indicate the X chromosome. Magnification 1000X.

https://doi.org/10.1371/journal.pone.0279869.g003

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Fig 4. Specific identification of the X and Y chromosomes by FISH.

(A) and (B) Blood cells from the female foal. (C) Metaphase spread derived from the blood sample of the male foal. (D) Interphase cells from the MSC culture used as nuclear donor. Red color indicates the X chromosome probe and green color indicates the Y chromosome probe. Magnification 1000X.

https://doi.org/10.1371/journal.pone.0279869.g004

Moreover, PCR analysis of X- and Y-linked markers was performed using genomic DNA derived from hair samples of the male foal, and hair and blood samples of the female foal (Fig 5). The sample from the male foal amplified the AMEL-X and AMEL-Y chromosome markers, whereas the samples from the female foal amplified only the AMEL-X chromosome marker. In addition, the female clone showed the profile expected for a female genotype, without amplification of the SRY gene or any of the Y-linked short tandem repeats (STR) markers. X-linked STRs in the female and male clones showed homozygous genotypes, as expected for genotypes carrying only one X chromosome.

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Fig 5. Characterization of X- and Y-linked markers.

Results of microsatellite analysis in the female and male horses. Boxes indicate the Y-linked markers.

https://doi.org/10.1371/journal.pone.0279869.g005

Discussion

In SCNT, sex is determined by the genotype of the nuclear donor. However, alterations involving the sex chromosome pair have been found in clones of some species. Here, we report the first sex modification in cloned horses, opening the door to sex manipulation through SCNT in this species.

Cytogenetic and molecular analysis of the female foal showed that the sex modification was the consequence of a Y chromosome loss that led to an X monosomy. This alteration might have occurred in the cell culture, or during early embryo development. Previous studies report a 10.2% incidence of X monosomy on mouse established XX and XY embryonic stem cell cultures [8], and around 15–18% of aneuployd cells in passage 2 human MSC cultures [9]. Different factors are thought to induce alterations in the chromosome number of cells in culture, including passage number [9, 10], Mycoplasma infection [11] and stress [12]. The MSCs used as nuclear donors in this work were at passage 2, and Mycoplasma contamination is periodically evaluated in our lab. Therefore, these factors were excluded as possible causes of chromosomal alterations. Nevertheless, cell samples were maintained at ambient condition for several hours before SCNT. According to the literature, the room temperature could have induced a stress response [13], which led to genome instability. In addition, the high oxygen tension triggers an oxidative stress response in MSC cultures as a consequence of a high oxygen consumption rate, which is strongly related to DNA damage and unstable chromosomal aberrations [9]. Nevertheless, the MSCs used as nuclear donors contained an euploid chromosome count according to the cytogenetic analysis. Alternatively, a spontaneous chromosome loss may have occurred during the early embryonic stages. In this case the result would be a mosaic embryo and, consequently, a mosaic female foal with 63,X and 63,XY cells. However, the two tissues evaluated in this study–blood and skin, which represent two different embryonic layers–showed the same genetic constitution according to karyotyping and PCR genotyping. Therefore, this alteration occurred in the cell culture at a rate below 1/348 and could not be detected, the female is indeed mosaic and presents 63,XX cells in tissues different from blood and skin, or the Y chromosome was lost during the earliest embryonic stage.

The horse is an attractive model for sex manipulation, as the X0 sex chromosome condition is well tolerated in this species. In fact, horses present the second-highest incidence, only after humans, of viable X chromosome monosomy. The negative correlation between the incidence of viable X0 individuals and the size and gene content of the pseudoautosomal region (PAR) of the sex chromosomes suggests that horses present a permissive genetic background towards this chromosomal alteration compared to other species [14].

Different strategies can be evaluated in horses to specifically eliminate a sex chromosome, according to previous reports in other species. For example, human chromosome 21 was functionally eliminated by insertion of a XIST transgene, which led to a stable chromatin modification and the silencing of the extra chromosome in human Down syndrome pluripotent stem cells [15]. In addition, targeted chromosome elimination was achieved through the insertion of oppositely oriented loxP sites and Cre-mediated sister chromatid recombination [16], or through the insertion of a TKNEO transgene into a targeted chromosome followed by selection of cells that spontaneously lost the edited chromosome [17]. More recently, the complete Y chromosome has been deleted using CRISPR/Cas9 technology in the mouse [18]. Furthermore, sex-reversal has been achieved in mice [19], rabbits [20], and pigs [21] through SRY gene knock-out, which yielded phenotypic females with an XY genotype. However, the use of these strategies involves gene editing techniques that would require approval from regulatory entities.

Alternatively, chromosome instability can be induced in cell cultures to promote spontaneous chromosome losses as described above while avoiding the use of molecular tools. Derivation of clonal cell lines, as achieved previously by our group in horses [22], may enable the isolation, identification, and replication of the X0 cells. Therefore, establishing X0 cell cultures, which might additionally be combined with specific X or Y chromosome transfer to zygotes [23, 24], could result in sex modification in horses by SCNT.

Equine sex manipulation can be applied to the preservation of endangered species, Turner syndrome research, and reproductive and sportive purposes. To date, conservation breeding programs are the main strategy applied for the preservation of wild horses. However, advanced assisted reproductive technologies (ARTs) are a powerful tool to be included in conservation programs for endangered species [2527]. Derivation of X0 cell lines combined with specific sex chromosome transfer and SCNT might enable the production of individuals of both sexes from cryopreserved samples of endangered and even extinct species. The horse stands as a particularly attractive model in this case, as the genetic plasticity shared among Equus [27] could enable the sex modification of individuals using X or Y chromosomes from a different equid species. Regarding medical research, 63,X mares show phenotypic features similar to those of Turner syndrome in humans, unlike those found in X0 mice [14], which makes the horse an attractive model for the study of this syndrome. Moreover, sex manipulation could be used as a breeding tool. If a female clone can be derived from a male horse and then bred, the genetic material from two original males could be combined. Finally, regarding commercial application, sex modification could be applied to sporting individuals. Polo, for example, is a sport practiced worldwide for which female horses are preferred over males. Considering that advanced biotechnologies are popular within this equine discipline (see the Argentine Polo Pony Breeder’s Association Statute at www.criapoloargentino.com.ar), obtaining a female clone from an exceptional male player may be of interest.

In conclusion, although the cause of the spontaneous chromosome loss reported in this work and how to intentionally reproduce it in the laboratory remain to be elucidated, the present report shows that sex manipulation by SCNT is feasible in horses, a finding of great potential for the preservation of endangered species, development of novel breeding techniques, and sportive purposes.

Materials and methods

Animal care and use of research animals

This study was carried out following the Guide for the Care and Use of Agricultural Animals in Agricultural Research and Teaching. The protocols involving animal manipulations were approved by the Institutional Committee for the Care and Use of Experimental Animals of the San Martin National University, Buenos Aires, Argentina (CICUAE-UNSAM, Permit Number: 001/16).

Isolation and culture of MSCs

MSCs were obtained from bone marrow aspirates of an adult male as described previously [2] with slight modifications. Briefly, aspiration was performed under sedation using 1 mL acepromazine maleate (Holliday-Scott SA, Buenos Aires, Argentina) and local anesthesia with 2% lidocaine. By pressing on the sternum, 200–300 ml of bone marrow aspirate was collected into a blood bag treated with sodium citrate. After discarding the blood through an infusion guide and washing with PBS, MSCs were collected through enzymatic treatment of the filter and blood bag with 0.25% Trypsin-EDTA (25200–56; Gibco, Waltham, MA, US) at 37°C for 10–15 min and vigorously shaking the bag and filter of the infusion guide. Finally, cells were collected by washing twice with 25 ml of DMEM-high glucose (10569–010; Gibco, Waltham, MA, US) supplemented with 20% fetal bovine serum (FBS, 10499–044; Gibco, Waltham, MA, US), 2% antibiotic–antimycotic (ATB; penicillin, streptomycin, and amphotericin B; 15240–096; Gibco), 1 μL/ml insulin-transferrin-selenium (ITS; 51300–044, Gibco) and 10 μl/ml MEM non-essential amino acids (11140–050; Gibco, Waltham, MA, US) and plated into a 150 mm cell culture dish (430599, Corning). Culture medium was changed twice a week until culture reached 70–80% confluence, when cells were cryopreserved in DMEM-high glucose supplemented with 20% FBS and 10% DMSO. At the moment of shipping this samples in particular, cells were thawed and plated on T25 flasks at 30% confluence, where they were kept for around 55 h at room temperature during transportation. When cells were received at the laboratory, flasks were immediately put at 38°C and 5% CO2 until 80% confluence, when cells were cryopreserved as described above.

SCNT and embryo transfer

The cloning procedure was performed as described previously [1] with some modifications. Briefly, equine oocytes were in vitro matured in HEPES-buffered TCM-199 (12340–030; Gibco) supplemented with 10% FBS, 1 μl/ml ITS, 1 mM sodium pyruvate (P2256), 100 mM cysteamine (M-9768), 0.1 mg/mL of follicle-stimulating hormone (NIH-FSH-P1, Folltropin1; Bioniche, Belleville, ON, Canada), and 2% ATB at 38°C. Cumulus cells were removed by vortex in hyaluronidase solution (H4272, 1 mg⁄ml) and only those oocytes with a visible first polar body were depleted of the zona pellucida by enzymatic digestion with 1.5 mg/ml pronase (P-8811). Zona-free (ZF) oocytes were stained with 1 μg/ml Hoechst bisbenzimide 33342 (H33342) and enucleated by micromanipulation under UV light. Enucleation was confirmed by direct observation of the stained metaphase plate inside the pipette. Each ooplast was coupled with a MSC using phytohemagglutinin (PHA; L8754) and fused by a double direct current pulse of 1.2 kV/cm, each pulse for 30 μs, separated by 0.1 s. Fused oocytes rested in 5 μl droplets of DMEM/F12 (D8062, Sigma, St Louis, MO, US) for 2.5 h to allow somatic cell reprogramming. Reconstructed embryos were activated with a 4-min incubation in 8.7 μM ionomycin (I24222; Invitrogen, Carlsbad, CA, USA) followed by individual culture in 5 μl droplets of DMEM/F12 with 1 mM 6-dimethylaminopurine (6-DMAP; D2629) and 5 mg/ml cycloheximide (CHX; C7698) for 4 h. Activated embryos were cultured in groups of three in micro-wells similar to the well of the well system [28] into 100 μl droplets of DMEM/F12 supplemented with 10% FBS and 1% ATB, in a humidified gas mixture (5% CO2, 5% O2, 90% N2) at 39°C. Cleavage was evaluated after 4 d of in vitro culture and medium was supplemented with 10% FBS. Blastocyst formation was observed between days 7 and 9.

The blastocysts were transferred to synchronized mares as described previously [1]. Briefly, blastocysts were transferred non-surgically in pairs, in 0.5 ml straws with DMEM-F12. Seven to fifteen days after the embryo transfer, pregnancies were diagnosed by transrectal ultrasonography, and fetal monitoring was performed once a week. Three to four weeks before expected parturition, the pregnant mares were transported to an equine hospital (KAWELL, Equine Rehabilitation Center, Solis, Argentina) to give birth.

Clone genotype identification

Both male and female clones were genotyped with a 15-horse panel of microsatellites, used for routine parentage and identity purposes and standardized according to the International Society of Animal Genetics (ISAG) (https://www.isag.us/committees.asp; S1 Table).

DNA was extracted from 5 hair roots using 100 μL of lysis buffer (10 mM Tris HCl, pH 8.0, 50 mM KCl, 2.5 mM MgCl2, 0.5% Tween 20, 10 μg proteinase K; Invitrogen) and incubated at 60°C for 45 min followed by heating at 95°C for 45 min. When a blood sample from the female clone was genotyped, DNA was isolated using the DNeasy Blood & Tissue Kit (Qiagen, Hilden, Germany).

Microsatellites were multiplexed into 2 mixes, as described previously (mix 1: VHL20, HTG4, AHT4, HMS7, ASB17, AHT5, HMS6, ASB23, TKY28; mix 2: ASB2, HMS2, HTG10, HMS3, UCDEQ425, TKY325), grouped by their annealing temperatures –60°C and 56°C, respectively–[29].

Each 25-μL reaction contained 20 ng genomic DNA, 1× PCR buffer, 2.2 mM MgCl2, 0.3 mM dNTPs (PCR buffer, MgCl2, and dNTPs; Invitrogen), 2% DMSO (dimethylsulfoxide; Millipore, Sigma), 0.15–0.5 μM of each primer (Applied Biosystems, Waltham, MA, US), and 1 U Platinum Taq DNA polymerase (Invitrogen). The PCR protocol consisted of 10 min at 95°C, followed by 31 cycles of 30 s at 95°C, 30 s at appropriate annealing temperature, 30 s at 72°C, and a final extension step of 72°C for 60 min. PCR products were separated by electrophoresis (3130xl; Applied Biosystems) and analyzed using GeneMapper v.4.0 (Applied Biosystems).

Sex molecular analysis

Both hair and blood from the female and the male clones, along with female and male control samples, were tested with a sex panel of X- and Y-linked markers (S2 Table) that were multiplexed into: mix 1 (X-linked microsatellites: TKY38, TKY270, Lex0003, and Lex026; Y-linked microsatellite: ECAYA16; annealing temperature 50°C), and mix 2 (AMEL gene, Y-linked microsatellites: ECAYH12, ECAYM2, and SRY gene; X-linked microsatellites: Lex0003 and UCDEQ502; annealing temperature 58°C) [30, 31]. PCR was carried out and fragments were analyzed as described in the previous section.

Cytogenetic analysis

The chromosome set was determined according to standard cytogenetic procedures. MSCs and fibroblasts were harvested from cells cultured as described previously. Phytohaemagglutinin stimulated lymphocytes were obtained from peripheral blood and cultured in RPMI-1640 supplemented with 20% FBS [32]. CBG-banding was performed according to the method of Sumner [33].

FISH analysis

Cell spreads were obtained from the donor MSCs used for the cloning procedure or from peripheral blood of the foals, and prepared as described above. The probes used were EQ-ENX (ZFX—Zinc Finger Protein X-Linked) labelled with rhodamine, and EQ-ENY (TSPY2—Testis Specific Protein Y-Linked 2) labelled with FITC (LEXEL SRL, Buenos Aires, Argentina). Slides were first incubated for 1 h at 45°C. During this time, 1 μl of each probe was mixed with 7μl of hybridization buffer, according to the manufacturer´s instructions. Both mixes were placed on the cell spreads and preparations were then covered and sealed with removable glue. The DNA samples and the probes were simultaneously denatured at 71°C for 8 min, followed by hybridization at 37°C overnight. After hybridization, the glue was carefully removed, and slides were immersed in 2xSSC (0.3M NaCl, 0.03M C6H5Na3O7.2H2O) at room temperature for 5 min or until the cover glass detached. Preparations were then placed for 2 min in 0.4xSSC + 0.3% Tween a 71°C, and immediately transferred to 2xSSC + 0.1% Tween for 2 min at room temperature. The excess of liquid was removed. Diamino-phenylindole (100ng/ml) and antifade (p-phenylenediamine 1mg/ml) were used as mounting media, and spreads were covered with a cover glass.

Images were taken using an Olympus IX71 epi-fluorescence microscope and Olympus DP-72 camera. Rhodamine and FITC signals were captured in separate images using Cell-Sence Viewer software (Olympus Corporation) and merged using Image-Pro Plus (Media Cybernetics).

Supporting information

S1 Table. Primer sequences for the genotype identification of the cloned foals.

https://doi.org/10.1371/journal.pone.0279869.s001

(DOCX)

S2 Table. Primer sequences of the sex chromosomes molecular analysis.

https://doi.org/10.1371/journal.pone.0279869.s002

(DOCX)

Acknowledgments

The authors thank MV. Victoria Witowsky, Emilia Gimenez and Abigail Costamagna for their technical assistance.

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