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Reproduction biotechnologies in germplasm banking of livestock species: a review

Published online by Cambridge University Press:  24 August 2017

J.M. Morrell  and
I. Mayer
J.M. Morrell*
Affiliation:
Division of Reproduction, Clinical Sciences, Swedish University of Agricultural Sciences (SLU), Box 7054, SE- 75007 Uppsala, Sweden.
I. Mayer
Affiliation:
Norwegian University of Life Sciences, Faculty of Veterinary Medicine and Biosciences, P.O. Box 8146 Dep, N-0033 Oslo, Norway.
*
All correspondence to: J.M. Morrell. Division of Reproduction, Clinical Sciences, Swedish University of Agricultural Sciences (SLU), Box 7054, SE- 75007 Uppsala, Sweden. E-mail: jane.morrell@slu.se
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Summary

Many biotechnologies are currently used in livestock breeding with the aim of improving reproductive efficiency and increasing the rate of genetic progress in production animals. Semen cryopreservation is the most widely used cryobiotechnology, although vitrification techniques now allow embryos and oocytes to be banked in ever-increasing numbers. Cryopreservation of other types of germplasm (reproductive tissue in general) is also possible, although the techniques are still in the early stages of development for use in livestock species. Although still in their infancy, these techniques are increasingly being used in aquaculture. Germplasm conservation enables reproductive tissues from both animals and fish to be preserved to generate offspring in the future without having to maintain large numbers of living populations of these species. However, such measures need careful planning and coordination. This review explains why the preservation of genetic diversity is needed for livestock and fish, and describes some of the issues involved in germplasm banking. Furthermore, some recent developments in semen handling leading to improved semen cryopreservation and biosecurity measures are also discussed.

Keywords

BiodiversityEndangered breedsEpigeneticsFishLivestock
Type
Commentary
Information
Zygote , Volume 25 , Issue 5 , October 2017 , pp. 545 - 557
Copyright
Copyright © Cambridge University Press 2017 

Introduction

Animal reproduction has a central role in the production efficiency and genetic improvement of domestic animals. Therefore, advances in reproductive technologies to maximize reproductive efficiency will be crucial to meeting future demands of an increasing global population (food security), as well as helping to overcome future difficulties in animal production wrought by climate change. Modern techniques of reproduction encompass various assisted reproduction technologies (ART), as well as technologies such as genomic selection that are applied in animal breeding to identify animals with superior genotypes (Veerkamp & Beerda, Reference Veerkamp and Beerda2007). While ART enables us to bring gametes together to establish a pregnancy, genomic selection is used to identify which individuals should be selected as a source of those gametes (Humblot et al., Reference Humblot, Le Bourhis, Fritz, Colleau, González, Guyader Joly, Malafosse, Heyman, Amigues, Tissier and Ponsart2010). Epigenetics, a related area of study, endeavours to explain environmental effects on DNA that affect expression of genes and therefore the phenotype of the resulting offspring (Urrego et al., Reference Urrego, Rodriguez-Osorio and Niemann2014). The key to these technologies is that a variety of methods can be combined to improve reproductive efficiency in breeding animals, in an effort to obtain optimal reproductive performance while maximizing usage of natural resources. Cryopreserving semen and embryos is one way of maximizing the availability of reproductive material, facilitating reproductive procedures independently of time and geographic location. However, germplasm banking is not restricted solely to gametes or embryos but refers to the cryopreservation of reproductive cells in general (Woelders et al., Reference Woelders, Windig and Hiemstra2012). The application of these techniques in livestock husbandry is the subject of this review.

Materials and Methods

The literature used in this review has been sourced via PUBMED and Web of Science. Search terms included germplasm, cryopreservation, vitrification, aquaculture, rare breed conservation, and ART.

Why preserve genetic biodiversity?

Genetic biodiversity allows animals to adapt to different environments, both to changes imposed on animals by mankind in the guise of management or husbandry practices and, in the wider sense, to diseases and climate change (Woelders et al., Reference Woelders, Windig and Hiemstra2012). Selecting only high-producing genotypes may be counter-productive in the long-term if fertility is thereby impaired, as seems to have been the case for dairy cattle (Rodriguez-Martínez et al., Reference Rodriguez-Martinez, Hultgren, Båge, Bergqvist, Svensson, Bergsten, Lidfors, Gunnarsson, Algers, Emanuelson, Berglund, Andersson, Håård, Lindhé, Stålhammar and Gustafsson2008). Conservation of animal genetic resources is essential to provide the genetic biodiversity required to allow animals to adapt to future changes in the environment. As far as farm animals are concerned, this means conserving our indigenous breeds; currently some 20% of livestock breeds are at risk of extinction and data are lacking for a further 36% of breeds. Rather than trying to maintain viable populations of each breed of livestock species (in situ conservation), a more practical method of maintaining genetic diversity is to cryopreserve germplasm (ex situ conservation). Thus by conserving existing genetic diversity, the basis for selecting ‘desirable’ genotypes in the future can be maintained.

With the rapid expansion in global aquaculture, there has been an increased emphasis on the development of reproductive technologies directed towards increased production efficiency in fish farming (Weber & Lee, Reference Weber, Lee, Lamb and DiLorenzo2014). While procedures for sperm cryopreservation have been developed for most major aquaculture species, successful sperm management for many species is currently constrained by the high variability of sperm cryo-resistance, a lack of appropriate biosecurity safeguards, and the absence of cryopreservation technologies sufficiently validated for large-scale aquaculture (Martínez-Páramo et al., Reference Martínez-Páramo, Horváth, Labbé, Zhang, Robles, Herráez, Suquet, Adams, Viveiros, Tiersch and Cabrita2017). In contrast to mammalian vertebrates, fish spermatozoa remain immotile in seminal plasma (Dadras et al., Reference Dadras, Sampels, Golpour, Dzyuba, Cosson and Dzyuba2017), with motility being activated following release into the external environment (sea or freshwater). Following activation, spermatozoa from most fish species remain motile for a short time period, often 1 min or less. To address these challenges, protocols for fish semen processing have focused on developing species-specific extenders to facilitate the collection and storage of inactivated spermatozoa (Tiersch et al., Reference Tiersch, Yang, Jenkins and Dong2007). Recent studies have indicated that temperature affects the lipid composition of motile carp sperm, with greater temperatures being associated with reduced lipid content, increased sperm curvilinear velocity and a decreased duration of the period motility (Dadras et al., Reference Dadras, Sampels, Golpour, Dzyuba, Cosson and Dzyuba2017).

Assisted reproduction technologies

The technologies involved in mammalian ART include a number of methods of bringing together spermatozoa and oocytes, such as artificial insemination (AI), gamete intra-fallopian transfer (GIFT), in vitro fertilization (IVF) and embryo transfer (ET), intra-cytoplasmic sperm injection (ICSI). To facilitate carrying out these techniques, other technologies have been developed such as sperm preservation and cryopreservation, and in vitro maturation (IVM) of oocytes (usually from slaughterhouse material), for subsequent IVF and ET.

By far the most widely used ART for breeding food production animals is AI using fresh or frozen semen. The availability of preserved semen (either cooled or cryopreserved) enables semen to be inseminated into females that are isolated from the male, thus facilitating both genetic improvement and disease control. If frozen, the semen can be used at any time, including after the death of the donor. This feature is particularly important when rare breeds are concerned as the chances of having access to fresh semen exactly when it is needed for insemination are low. However, it is not always possible to collect semen from all individuals, particularly those that have not been trained to ejaculate into an artificial vagina. In some cases, the collection of epididymal spermatozoa after castration or death is feasible (Woelders et al., Reference Woelders, Windig and Hiemstra2012) and can yield high numbers of useable spermatozoa e.g. from rams.

Use of AI has the disadvantage that it focuses mainly on the genetic component of the male; ET should enable genetic progress to be made more rapidly than AI as it enables both the male and female genetic components to be transferred. Worldwide, ET is increasing considerably within the bovine livestock sector, mainly due to an increase in the transfer of in vitro produced (IVP) embryos. Figures from 2012 indicate a current annual transfer of around 500,000 embryos produced by superovulation and 400,000 by in vitro maturation (Galli et al., Reference Galli, Duchi, Colleoni, Lagutina and Lazzari2014). The vast majority of these transfers is occurring in South America, especially Brazil.

Some in vitro technologies are better suited to particular species than others. The increasing use of bovine IVP embryos is indicative of the success of the technique in this species. However, in horses it has not been possible to develop a reliable method for equine IVF. Thus ICSI is more commonly used than IVF for equids, although the need for specialized equipment and highly trained personnel limit the use of this ART. Conversely, ICSI is not commonly used for bovine oocytes because of technical difficulties, such as inadequate oocyte activation (Malcuit et al., Reference Malcuit, Maserati, Takahashi, Page and Fissore2006) or cytoskeletal damage, e.g. from the large-diameter pipette needed to accommodate the bull spermatozoon (Galli et al., Reference Galli, Vassiliev, Lagutina, Galli and Lazzari2003). In other species, the lack of access to oocytes is a limiting factor in the potential development of an ET program. Protocols for cryopreserving embryos may not be suitable for oocytes, even in the same species; further research is needed to develop better methods of preserving oocytes. Thus it is important not only to choose the technique to fit the species but to develop as many forms of ART as possible, to increase the chances of success in any given species.

Germplasm banking

The term ‘germplasm’ encompasses all reproductive cells that, singly or in combination, lead to the production of offspring. The most commonly encountered form of germplasm banking is sperm cryopreservation, which has been used in livestock breeding for more than 50 years and is considered to be the backbone of modern dairy cattle production. It is also the most readily applicable biotechnology as spermatozoa are the reproductive cells that are most easily obtained and numerous. In contrast, obtaining oocytes is invasive, their numbers are limited and maturation is cycle-dependent in many livestock species. Whereas sperm cryopreservation protocols exist for approximately 300 species, protocols for oocytes and embryos have been developed for fewer than 50 species. Other sources of germplasm include spermatids, spermatogonial stem cells, testicular and ovarian tissue, as well as somatic cells for nuclear transfer.

Sperm cryopreservation

The technique for sperm cryopreservation in the presence of a permeating cryoprotectant, glycerol, was developed by Polge et al. (Reference Polge, Smith and Parkes1949) in the middle of the 20th century. Despite many decades of research the basic principles of this technique remain unchanged. In brief, the method for cryopreservation of semen is as follows: in some species, e.g. boar and stallion, the semen is centrifuged in extender first to remove most of the seminal plasma. The spermatozoa are cooled slowly in a hyperosmotic solution containing cryoprotectants to minimize ice-crystal formation. Water is drawn out of the sperm cells while permeating cryoprotectants enter (Watson, Reference Watson1995). Ice-crystal formation cannot be prevented completely, nor the increasing solute concentration caused by loss of water, leading to a certain amount of structural damage. Thus, only a proportion of the spermatozoa survive cryopreservation, depending on the individual and species.

Slight variations to this protocol have been made over the intervening decades, such as substituting plant-derived lecithins (Leite et al., Reference Leite, do Vale-Filho, de Arruda, de Andrade, Emerick, Zaffalon, Martins and de Andrade2010) or liposomes (Röpke et al., Reference Röpke, Oldenhof, Leiding, Sieme, Bollwein and Wolkers2011), for egg yolk or milk in the cryopreservation extender, to avoid including material of animal origin. Glycerol is still the main cryoprotectant used for freezing spermatozoa for most mammalian species although attempts have been made to find substances that are less toxic, with various amides attracting attention (Alvarenga et al., Reference Alvarenga, Papa, Landim-Alvarenga and Medeiros2005). However, there seems to be considerable variation within species regarding the suitability of different agents: a combination of dimethylformamide and glycerol was reported to be useful for stallion semen (Álvarez et al., Reference Álvarez, Gil, González, Olaciregui and Luño2014), although dimethylformamide was not superior to glycerol for freezing bull semen (Forero-González et al., Reference Forero-González, Celeghini, Raphael, Andrade, Bressan and Arruda2012). Moreover, including dimethylacetamide and glycerol as the cryoprotectant for boar spermatozoa did not offer any advantages over glycerol alone (Yang et al., Reference Yang, Wu, Cheng, Wang and Wu2016).

Recent advances in sperm cryopreservation have examined the effects of seminal plasma on sperm membranes, particularly in species in which there is considerable individual variation in sperm freezability. For instance, it was observed that adding seminal plasma from boars that were known to be good freezers improved motility and membrane integrity of other boars' spermatozoa (Hernández et al., Reference Hernández, Roca, Calvete, Sanz, Muiño-Blanco, Cebrián-Pérez, Vázquez and Martínez2007). Similar experiments with stallion spermatozoa, however, have achieved contradictory results; in some cases sperm quality is improved (e.g. Moore et al., Reference Moore, Squires and Graham2005) and in other cases there was no effect (e.g. Mari et al., Reference Mari, Castagnetti, Rizzato, Mislei, Iacono and Merlo2011).

The effects of other additives have also been studied. The survival of both stallion (Moore et al., Reference Moore, Squires and Graham2005) and bull spermatozoa (Amorim et al., Reference Amorim, Graham, Spizziri, Meyers and Torres2009) has been shown to be improved by including cholesterol in the cryopreservation medium. Various antioxidants have been shown to improve post-thaw sperm quality (Lindemann et al., Reference Lindemann, O'Brien and Giblin1988) e.g. glutathione peroxidase (Sławeta et al. Reference Sławeta, Waşowicz and Laskowska1988), and interest in other antioxidants has blossomed recently. Plant-derived substances with antioxidative activity such as rosmarinic acid have been used for boar spermatozoa (Luño et al. 2014). Virgin coconut oil was found to enhance post-thaw motility, morphology, membrane integrity and acrosome status of bull spermatozoa (Tarig et al., 2017). The flavonol quercetin, which is thought to suppress formation of superoxide and peroxy radical formation, as well as chelating iron, was reported to improve post-thaw motility and DNA integrity of stallion spermatozoa (Gibb et al., Reference Gibb, Butler, Morris, Maxwell and Grupen2013). These are only some examples of recent attempts to improve post-thaw sperm quality with various additives.

Embryos and oocytes

Embryos (and, to some extent, oocytes) can be frozen using permeating cryoprotectants and slow freezing protocols in programmable cell freezers, in a similar manner to spermatozoa. Vitrification, particularly of oocytes, is in many cases more successful than conventional slow freezing. Oocytes are particularly sensitive to slow freezing because of the low permeability of the plasma membrane to cryoprotectants but also because of premature cortical granule exocytosis leading to zona hardening, which renders them impenetrable by a spermatozoon for subsequent fertilization (Arav, Reference Arav2014). With vitrification, however, the cells are placed in a solution of high osmolarity but without permeating cryoprotectants, and are then plunged directly into liquid nitrogen. As no ice-formation takes place and the transition to a glass-like state occurs very rapidly, structural damage is minimized (Arav, Reference Arav2014). Table 1 provides a comparison of the two techniques. Despite the success with vitrification of human oocytes, those of cattle are proving more problematic, which may be due to the amount of cytoplasmic lipids and/or the composition of the plasma membranes (Sprícigo et al., Reference Sprícigo, Diógenes, Leme, Guimarães, Muterlle, Silva, Solà-Oriol, Pivato, Silva and Dode2015).

Table 1 Comparison of slow freezing and vitrification for embryos and oocytes

Vitrification has also been attempted with spermatozoa. The problems encountered with cryopreservation-induced sperm damage are well known and include physical damage from ice-crystal formation and dehydration, damage to the sperm mitochondria arising from cold-shock, damage to the plasma and acrosomal membranes (capacitation-like damage) and DNA, as well as toxicity of cryoprotectants (Agha-Rahimi et al., Reference Agha-Rahimi, Khalili, Nabi and Ashourzadeh2014). Theoretically, these problems could be circumvented by vitrification, in which there is no ice-crystal formation and very high rates of cooling are employed that are considered to be too rapid for cold-shock to occur (Isachenko et al., Reference Isachenko, Mallmann, Rahimi, Risopatròn, Schulz, Isachenko, Sànchez and Katkov2012). However, to date, the only species in which sperm vitrification is reported to be successful is the human (Isachenko et al., Reference Isachenko, Mallmann, Rahimi, Risopatròn, Schulz, Isachenko, Sànchez and Katkov2012). Considerable chromatin damage was induced in dog spermatozoa by vitrification, much more so than by conventional freezing (Sánchez et al., Reference Sánchez, Risopatrón, Schulz, Villegas, Isachenko, Kreinberg and Isachenko2011). Even with human spermatozoa there are conflicting reports about whether vitrification offers any advantages over conventional slow freezing (Agha-Rahimi et al., Reference Agha-Rahimi, Khalili, Nabi and Ashourzadeh2014). The size of the sperm head appears to be a crucial factor in determining cryosensitivity during vitrification, with smaller sperm heads being able to withstand the severe osmotic effects better than the larger, paddle-shaped sperm heads of most livestock species. Therefore, further developments are needed before this technique will be able to provide a real alternative to slow freezing of spermatozoa.

Other germplasm

Recent research has examined the possibilities of transplanting spermatogonial stem cells, or testicular or ovarian tissue following cryopreservation. There are isolated reports of successful transplantation of spermatogonial stem cells in mice (Gouk et al., Reference Gouk, Loh, Kumar, Watson and Kuleshova2011), and of bovine testicular tissue into recipient bulls (Herrid et al., Reference Herrid, Vignarajan, Davey, Dobrinski and Hill2006); both techniques are reported to produce viable spermatozoa. The pattern of donor sperm production in the recipient bulls showed a decline in the proportion of spermatozoa from the donor up to 6 months following transplantation (Herrid et al., Reference Herrid, Vignarajan, Davey, Dobrinski and Hill2006). Donor-derived spermatozoa were detected in semen from 2% recipient goats for 5 to 8.5 months; in rams 1–30% spermatozoa were donor-derived for up to 30 months and 15% of the progeny from one of these recipient rams were donor-derived (Herrid & McFarlane, Reference Herrid and McFarlane2013). Post-transplantation production of ram spermatozoa of donor origin for at least 5 years was reported in other studies (Stockwell et al., Reference Stockwell, Hill, Davey, Herrid and Lehnert2013). These studies show that such transplantation is possible, even if further research is needed to refine the technique.

Interestingly, cryopreservation of testicular tissue requires a different cryoprotectant from those commonly used for spermatozoa or for embryos, dimethyl sulphoxide (DMSO) for tissue (Wu et al., Reference Wu, Hu, Guo, Yue, Yang and Zhang2011), as opposed to glycerol for spermatozoa and propanediol or ethylene glycol for embryos. Although convenience dictates that one protocol is optimal for any given species, it appears that the best results are obtained if the protocol is tailored to fit the gametes of each individual.

Cryopreserved ovarian tissue has apparently been transplanted successfully in mice and human patients as a means of retaining fertility despite chemotherapy. Similar studies have been attempted with bovine, ovine and caprine tissue. The use of in vitro follicular culture with cryopreserved tissue is preferred to transplantation in post-pubertal human patients because it helps to reduce the risk of reintroducing cancer cells into the patient. Again, the use of DMSO as the cryoprotectant for ovarian tissue gives much higher success rate than the use of glycerol (Lunardi et al., Reference Lunardi, Araújo, Bernuci, Lunardi, Gonçalves, Carvalho Ade, de Figueiredo and Rodrigues2012); it is hypothesized that the smaller molecular size of the cryoprotectant enables it to permeate the tissue more readily than larger molecules. An alternative method, vitrification of the tissue, also gives better results than slow freezing.

Fish germplasm

While significant advances have been made in the cryopreservation of mammalian oocytes and embryos the situation is far less advanced in all other vertebrates, including teleost fish. In comparison with mammals, oocytes and embryos of fish are substantially larger in volume (Seki et al., Reference Seki, Kouya, Tsuchiya, Valdez, Jin, Koshimoto, Kasai and Edashige2011) and are characterized by low membrane permeability, resulting in restricted movement of both water and cryoprotectants across cellular membranes during chilling, freezing and thawing (Saragusty & Arav, Reference Saragusty and Arav2011). Further, the oocytes and embryos of fish typically contain large yolk stores. The behaviour of yolk during cryopreservation differs markedly from that of other embryonic compartments, making cryopreservation very complex (Seki et al., Reference Seki, Kouya, Tsuchiya, Valdez, Jin, Koshimoto, Kasai and Edashige2011). As a consequence of these characteristics, the development of successful and reproducible procedures for the cryopreservation of oocytes and embryo from non-mammalian vertebrates, including fish, is extremely complex and remains one of the main challenges in the field of cryobiology.

Primordial germ cells (PGCs)

The conservation of both maternal and paternal genetic information is essential for conservation initiatives (germplasm banking). As successful cryopreservation of both oocytes and embryos in teleost fish remains prohibitively difficult, attention has switched to preserving alternative forms of germplasm, notably PGCs, which are the precursors of both oogonia and spermatogonia. PGCs are formed during the early stages of embryonic development and, in fish, these cells undergo active proliferation following migration to the genital ridges. Recent studies have now demonstrated that functional spermatozoa and eggs can be obtained following the transplantation of either PGCs or functionally similar spermatogonial stem cells in a number of fish species (Okutsu et al., Reference Okutsu, Suzuki, Takeuchi and Yoshizaki2006; Kobayashi et al., Reference Kobayashi, Takeuchi, Takeuchi and Yoshizaki2007; Morita et al., Reference Morita, Kumakura, Morishima, Mitsuboshi, Ishida, Hara, Kudo, Miwa, Ihara, Higuchi, Takeuchi and Yoshizaki2012). For example, thawed PGCs, isolated from adult rainbow trout (Oncorhynchus mykiss), when transplanted into the peritoneal cavity of newly hatched embryos differentiated into mature spermatozoa and eggs in the recipient gonads. Furthermore, the donor-derived spermatozoa and eggs obtained from the recipient fish were able to produce normal offspring.

Interest in PGC transplantation techniques increased further after it was demonstrated that PGCs from one species could be successfully transplanted into the embryo of another, in which they proliferate, yielding viable gametes of the donor species. This procedure, termed surrogate reproduction, was first demonstrated with trout PGCs successfully transplanted into triploid masu salmon (Oncorhynchus masou) embryos (Okutsu et al., Reference Okutsu, Shikina, Kanno, Takeuchi and Yoshizaki2007). The principle of this reproductive technology is relatively simple. Progenitor cells of eggs and sperm, either PGCs or spermatogonia, are isolated from the target species and transplanted into a closely related recipient species. Upon maturation, donor-derived eggs and sperm are then produced in the recipient (Fig. 1). Surrogate broodstocking has major implications to both aquaculture production and conservation, especially as studies now show that PGCs can be transplanted across species, genus, and even family barriers (Saito et al., Reference Saito, Goto-Kazeto, Fujimoto, Kawakami, Arai and Yamaha2010, Yoshizaki et al., Reference Yoshizaki, Okutsu, Morita, Terasawa, Yazawa and Takeuchi2012). There is now considerable interest in applying surrogate broodstock technologies in the aquaculture of species that are difficult or costly to breed in captivity, such as the sturgeons (family Acipenseridae) and the bluefin tuna (Thunnus thynnus). For example, transplantation of germ cells from the valuable bluefin tuna into the earlier maturing and easier to maintain chub mackerel (Scomber japonicus) is being viewed as a possible answer to the aquaculture production of this difficult species (Yoshizaki et al., Reference Yoshizaki, Okutsu, Morita, Terasawa, Yazawa and Takeuchi2012). It is envisaged that both conservation and efficient utilization of genetic resources (aquaculture) can now be more efficiently achieved in fish through surrogate production combined with the cryopreservation of PGCs.

Figure 1 Principle of surrogate reproduction in fish. Conservation of a threatened species can be achieved by transplanting frozen PGCs or spermatogonia into recipient embryos of a closely related species (adapted from Yoshizaki et al., Reference Yoshizaki, Okutsu, Morita, Terasawa, Yazawa and Takeuchi2012).

Given the current limitations in the ability to freeze fish oocytes and embryos there is increasing interest in cryobanking PGCs and spermatogonia of threatened fish species. Thus PGCs have been successfully transplanted from the critically endangered Chinese sturgeon to a closely related but not endangered species, the Dabrey's sturgeon (Ye et al., Reference Ye, Li, Yue, Du, Yang, Yoshino, Hayashida, Takeuchi and Wei2017). While there is still much work to do to develop this technique, these results show that transplantation of PGCs, and their survival in the recipient, is possible.

While public concern has focused primarily on the conservation of terrestrial species, especially iconic mammalian species, aquatic species including teleost fishes are considered more vulnerable to anthropogenic impacts. Indeed, according to the IUCN Red List of Threatened Species (International Union for Conservation of Nature, 2016), 58 ray-finned fish species (Actinopterygii), as well as one lamprey species, have become extinct in recent years. As such, further advances in the cryopreservation of fish germ cells and reproductive technologies such as surrogate broodstocking will be a major benefit not only to aquaculture, but also for the conservation of threatened fish species (Comizzoli & Holt, Reference Comizzoli, Holt, Holt, Brown and Comizzoli2014). The principle of surrogate reproduction in fish is depicted in Fig. 1.

Pitfalls with germplasm cryopreservation

Although there are many indications for the use of germplasm banking in livestock production, major technological limitations still exist in its application to all types of germplasm and to all species. Cryopreservation tends to decrease the viability and fertilizing capability of germplasm, and this is more so where pieces of tissue are frozen rather than gametes. In addition, there may be epigenetic changes brought about by the cryoprotective agents and techniques used (Urrego et al., Reference Urrego, Rodriguez-Osorio and Niemann2014) which cannot be studied effectively until enough offspring are produced from these procedures to provide a representative population. A complicating factor in such studies with rare breeds or endangered species is the lack of suitable breeding animals to provide gametes, or to test the effect of proposed changes in handling procedures on fertility (Woelders et al., Reference Woelders, Windig and Hiemstra2012).

Species-specific protocols may be needed as existing ones cannot be extrapolated to all other species. Tissue-specific protocols may be needed: for example, cryopreserving epididymal spermatozoa may require a different protocol to ejaculated samples. Cryopreserving embryos allows the full genetic complement of both sire and dam to be preserved whereas sperm freezing preserves only the male genetic component, but the transfer of the material to recipient animals may be technically more demanding for embryos than for spermatozoa, depending on the species. In many sheep, for example, it is not possible to pass a catheter through the cervix; while semen can be deposited vaginally, deposition of embryos requires a surgical or laparoscopic approach, which is more technically demanding than vaginal deposition of semen. In addition, awareness of biosecurity has increased considerably over the last few decades; it is now known that not only must the donor animals be free of disease but also that material of animal origin in the cryopreservation medium should be avoided or, when this is impossible, the material should be from specific pathogen-free sources. Furthermore, liquid nitrogen itself may act as a vector for transmitting pathogens (Bielanski & Vajta, Reference Bielanski and Vajta2009). Relying on antibiotics to control bacterial contamination is not a sustainable course of action and may result in many of the stocks of frozen germplasm being unusable in the future if legislation on antimicrobials changes. Use of cryopreserved tissues (as opposed to gametes or embryos) necessitates surgical transplantation of the tissue to the recipient, which is not a trivial procedure.

Cloning

The cloning of domestic livestock by somatic cell nuclear transfer (SCNT) has been possible for several years but the procedure remains technically demanding and expensive. In this procedure, a donor cell is injected into, and fused with, a mature, good quality, enucleated oocyte, followed by activation and culture of the product. However, there are high rates of pregnancy loss and also abnormal placental development and pathologies during the neonatal period, which is a major limiting factor in the adoption of this technique. As biobanking of somatic cells is increasing around the world, material from rare livestock breeds could be available for SCNT. While the technology is still in its infancy for conservation purposes with low success rates in wild species (Holt, Reference Holt2008), it is possible that it could provide a means of rescuing rare livestock breeds because of the availability of oocytes and recipient females for the cloned embryos among production animals. Several wild species of cattle and sheep have already been cloned (Ryder & Benirschke, Reference Ryder and Benirschke1997; Critser et al., Reference Critser, Riley, Prather, Holt, Pickard, Rodger and Wildt2003; Holt et al., Reference Holt, Pickard and Prather2004). However, it should be noted that many attempts are needed in order to obtain some success; only 1–5% of porcine SCNT embryos develop into piglets (Grupen, Reference Grupen2014). Production of offspring unfortunately does not mean that a healthy adult animal, capable of reproducing, will result (Holt, Reference Holt2008). Furthermore, the production of a few cloned individuals is unlikely to conserve much genetic diversity; an extensive biobank of material from existing individuals would be needed to ensure that as much as possible of the current gene pool is retained. Such biobanking for all livestock species is likely to require considerable commitment in time and resources.

Epigenetics

Epigenetic changes can be defined as stable alterations of DNA-associated molecules that may cause gene expression to be altered. This alteration is brought about by changes in methylation that affect gene expression (Jovanovic et al., Reference Jovanovic, Ronneberg, Tost and Kistensen2010; Munro et al., Reference Munro, Farquhar, Mitchell and Ponampalam2010). It is now known that factors such as nutrition (under- or over-nutrition) can affect methylation, as can various environmental toxins (Schagdarsurengin & Steger, Reference Schagdarsurengin and Steger2016). It is not known, however, if sperm handling procedures such as preservation or cryopreservation, may have an epigenetic effect. Certainly the more handling procedures to which germplasm is subjected, the more chances there are that an epigenetic effect will occur. Speculation exists of a link between various ART and imprinting disorders, occurring via altered DNA-methylation patterns and histone coding (Urrego et al., Reference Urrego, Rodriguez-Osorio and Niemann2014).

Epigenetic effects can influence reproductive efficiency through alterations in the viability of embryos, foetuses and the neonate, and also through control of endometrial gene expression which may alter implantation. They may also influence health, especially the occurrence of cancer through regulation of proto oncogenes and suppression of tumour suppressor genes, and phenotypic performance for a variety of functions or traits. Some epigenetic modifications can even be transmitted to subsequent generations (Schagdarsurengin & Steger, Reference Schagdarsurengin and Steger2016).

Recent advances in sperm handling for livestock species

The spermatozoa of some species, e.g. stallions, survive cryopreservation better if most of the seminal plasma is removed before the cryoprotectant is added (Loomis & Graham, Reference Loomis and Graham2008). Further improvements can be seen if living spermatozoa are separated from dead and dying cells prior to freezing (Hoogewijs et al., Reference Hoogewijs, Morrell, Van Soom, Govaere, Johannisson, Piepers, De Schauwer, de Kruif and De Vliegher2011). Various methods have been advocated for selecting viable spermatozoa and removing them from seminal plasma (Morrell & Rodriguez-Martínez, Reference Morrell and Rodriguez-Martinez2016) but, to date, only colloid centrifugation of stallion spermatozoa seems to be feasible for field use. These methods select spermatozoa based on certain functional attributes, such as motility or intact plasma or acrosomal membranes and are, therefore, believed to mimic the selection occurring in the female reproductive tract (Suarez, Reference Suarez2007). Some of these techniques will now be described briefly.

In migration techniques, e.g. ‘swim-up’, motile spermatozoa swim away from the bulk of the sample to an area containing few spermatozoa. Passage through glass wool or Sephadex gel physically impedes spermatozoa with reacted acrosomes, damaged membranes or abnormal morphology. Colloid centrifugation selects motile spermatozoa with intact membranes and also those with mature chromatin from those with immature or damaged chromatin. Magnetic activated cell sorting (MACS) has been used in combination with a marker, such as annexin V, to remove apoptotic spermatozoa from the sample. Annexin V has a high affinity for phosphatidylserine, which is thought to be externalized on the sperm plasma membrane in the early stages of apoptosis. When conjugated to magnetic microspheres, annexin V can bind to, and retain, apoptotic spermatozoa within an affinity column. This selection technique has been reported for processing of human spermatozoa for fertility treatments (reviewed by Gil et al., Reference Gil, Sar-Shalom, Sivira, Carreras and Checa2013) but has not been widely adopted for processing of animal spermatozoa, apart from occasional research reports, e.g. for rabbit (Vasicek et al., 2013), bull (Faezah et al., 2014) and Senegalese sole spermatozoa (Valcarce et al., Reference Valcarce, Herráez, Chereguini, Rodríguez and Robles2016). The method may not be amenable for processing large volumes of semen.

One selection technique that is showing promise in the preparation of spermatozoa for ART is colloid centrifugation. This technique has been available for preparing spermatozoa, mainly human spermatozoa for fertility treatments or bovine spermatozoa for IVF, for at least 20 years but the technique has only been adopted more generally for sperm preparation with the development of single layer centrifugation (SLC) in the last few years (Morrell & Wallgren Reference Morrell and Wallgren2011). The chronology of these techniques is shown in Table 2. The reasons for this late adoption were mainly that the method first described – density gradient centrifugation – was considered to be too impractical for use when preparing large volumes of semen or for ejaculates with a high sperm concentration. The development of a technique using only a single layer of colloid has revolutionised sperm preparation as it is much easier to use and allows the technique to be scaled up to process large volumes of semen (Morrell et al., Reference Morrell and Rodriguez-Martinez2009). This technique was named single layer centrifugation by its developer, one of the authors of the present paper (Morrell & Rodriguez-Martínez, 2011).

Table 2 Chronology of colloid centrifugation as a sperm preparation technique

Centrifugation of sperm samples through a colloid allows robust spermatozoa i.e. motile spermatozoa with normal morphology, intact plasma membranes and intact chromatin, to be selected from the rest of the ejaculate. The colloid works by presenting a physical barrier to the passage of immotile spermatozoa or those with abnormal morphology and damaged membranes; thus such spermatozoa are prevented from pelleting during centrifugation. Spermatozoa are also separated from seminal plasma and any non-sperm cells in the semen, such as epithelial cells from the lining of the reproductive tract or bacteria contaminating the ejaculate during semen collection. Removal of dead or dying spermatozoa and cellular debris aids survival of living spermatozoa and may also improve sperm cryosurvival in some species (Hoogewijs et al., Reference Hoogewijs, Morrell, Van Soom, Govaere, Johannisson, Piepers, De Schauwer, de Kruif and De Vliegher2011; Martínez-Alborcia et al., Reference Martinez-Alborcia, Morrell, Barranco, Maside, Gil, Parrilla, Vazquez, Martinez and Roca2013). Various ready-to-use species-specific colloid formulations have been produced; these formulations are adjusted according to the semen characteristics of different species and therefore it is important to use the correct formulation for the species in question.

Apart from improving sperm survival there are other reasons for using colloid centrifugation to prepare sperm samples: if the spermatozoa are to be used for IVF, they should first be separated from seminal plasma which contains decapacitating factors, and from cryoprotectants (Morrell & Rodriguez-Martínez, Reference Morrell and Rodriguez-Martinez2009). Traditionally this separation has been achieved with a technique known as ‘swim-up’, wherein motile spermatozoa swim away from the mixture of seminal plasma and cryoprotectant into fresh medium. However, this method does not select spermatozoa with normal morphology or with intact chromatin, and usually only 10–20% of the spermatozoa are recovered (Hallap et al., Reference Hallap, Håård, Jaakma, Larsson and Rodriguez-Martínez2004). Colloid centrifugation with Percoll was suggested as a means of selecting the best spermatozoa for IVF as well as separating them from the seminal plasma but lost favour when it was reported that some batches of Percoll were toxic to spermatozoa (Avery & Greve, Reference Avery and Greve1995). A further disadvantage of the original Percoll protocol was that it did not take into account species differences in semen characteristics (physical properties such as osmolarity and pH, as well as chemical composition) that affect the yield of spermatozoa recovered after the centrifugation (Morrell et al., Reference Morrell, van Wienen and Wallgren2011). The SLC technique with our colloid has also been used to separate sturgeon spermatozoa from cryomedium (Y. Horokhovatskyi & B. Dzyuba, unpublished data).

Colloid centrifugation selects sperm with intact chromatin, which can be important in species such as horses and some exotic animals. Spermatozoa with damaged chromatin are still capable of moving and of fertilizing oocytes, which means that they effectively compete with normal spermatozoa. At some stage after fertilization, however, development is halted and the pregnancy fails. In AI trials, SLC-selected stallion sperm samples produced more pregnancies than their corresponding control samples (Morrell et al., Reference Morrell, Richter, Martinsson, Stuhtmann, Hoogewijs, Roels and Dalin2014), which may be due, at least in part, to the selection of spermatozoa with intact chromatin. In addition, colloid centrifugation separates spermatozoa from pathogens in the ejaculate, which may enable a reduction in the use of antibiotics (Morrell & Wallgren, Reference Morrell and Wallgren2014). The inclusion of antibiotics in semen extenders represents a non-therapeutic use of antimicrobials, which is not consistent with current policies to reduce antibiotic usage. It has become apparent that using any antibiotics can lead to the development of resistance in bacterial species other than the target species, which is readily transferred to bacterial populations in other animal species, including potentially humans. As such, the application of procedures such as SLC will result in increased biosecurity, and importantly will facilitate the reduction in antibiotic use in trading and use of animal semen.

Conclusions and future perspectives

Conservation of genetic diversity in livestock breeds is needed to ensure that there is sufficient genetic flexibility to meet future environmental or husbandry challenges. The most practical way to implement this conservation is by cryopreserving semen and embryos, because functional techniques already exist for these procedures in most livestock species and the thawed material can be transferred to recipient animals by non-invasive means, at least in some species. Further research is needed to develop non-invasive transfer methods for the remaining livestock species. Cryopreservation of oocytes is less common because of the difficulty in obtaining material and in overcoming structural differences between oocytes and embryos. In addition, the development of methods for preserving testicular and ovarian tissue should be continued, especially if the tissue fragments can be used for the in vitro generation of gametes in the future rather than being transferred to recipient animals. Ovarian and testicular tissues constitute a wealth of untapped, arrested or developing germ cells, most of which never participate in fertilization. Advances in our ability to preserve gonadal tissues, and to successfully mature early stage oocytes and spermatogonia in culture or by xenografting could provide an unlimited source of germplasm to generate embryos, including from animals that are prepubertal, outside their breeding season, nearing the end of their reproductive lifespan or that die unexpectedly. The use of gonadal tissue as a source of germplasm, for use in both ARTs and genetic resource banking, would be particularly beneficial to non-mammalian vertebrates (fishes, birds, reptiles and amphibians), due to the current lack of success in cryopreserving both oocytes and embryos in these animals groups. Finally, sperm cryosurvival can be enhanced by simple handling procedures such as SLC that not only select the most robust spermatozoa but also may improve the chances of fertilization and pregnancy.

Acknowledgements

JMM is funded by grants from the Foundation for Equine Research, Stockholm, and the Swedish Farmers’ Foundation; IM is funded by the Norwegian Research Council.

Conflict of interest

JMM is the inventor and one of the patent holders of a colloid formulation and the technique of SLC mentioned here.

References

Abraham, M.C., Johannisson, A. & Morrell, J.M. (2016). Effect of sperm preparation on development of blastocyst in vitro . Zygote 24, 825–30.CrossRefGoogle ScholarPubMed
Agha-Rahimi, A., Khalili, M.A., Nabi, A. & Ashourzadeh, S. (2014). Vitrification is not superior to rapid freezing of normospermic spermatozoa: effects on sperm parameters, DNA fragmentation and hyaluronan binding. Reprod. Biomed. Online 28, 352–8.CrossRefGoogle ScholarPubMed
Alvarenga, M.A., Papa, F.O., Landim-Alvarenga, F.C. & Medeiros, A.S. (2005). Amides as cryoprotectants for freezing stallion semen: a review. Anim. Reprod. Sci. 89:105–13.CrossRefGoogle ScholarPubMed
Álvarez, C., Gil, L., González, N., Olaciregui, M. & Luño, V. (2014). Equine sperm post-thaw evaluation after the addition of different cryoprotectants added to INRA 96® extender. Cryobiology 69:144–8.CrossRefGoogle ScholarPubMed
Amorim, E.A., Graham, J.K., Spizziri, B., Meyers, M. & Torres, C.A. (2009). Effect of cholesterol or cholesteryl conjugates on the cryosurvival of bull sperm. Cryobiology 58, 210–4.CrossRefGoogle ScholarPubMed
Arav, A. (2014). Cryopreservation of oocytes and embryos. Theriogenology 81, 96102.CrossRefGoogle ScholarPubMed
Avery, B. & Greve, T. (1995). Impact of Percoll on bovine spermatozoa used for in vitro insemination. Theriogenology 44, 871–8.CrossRefGoogle ScholarPubMed
Bielanski, A. & Vajta, G. (2009). Risk of contamination of germplasm during cryopreservation and cryobanking in IVF units. Hum. Reprod. 24, 2457–67.CrossRefGoogle ScholarPubMed
Blomqvist, G., Persson, M., Wallgren, M., Wallgren, P. & Morrell, J.M. (2011). Removal of virus from boar semen spiked with porcine circovirus type 2. Anim. Reprod. Sci. 126, 108–14.CrossRefGoogle ScholarPubMed
Bolton, V.N. & Braude, P.R. (1984). Preparation of human spermatozoa for in vitro fertilization by isopycnic centrifugation on self-generating density gradients. Arch. Androl 13, 167–76.CrossRefGoogle ScholarPubMed
Comizzoli, P. & Holt, W.V. (2014). Recent advances and prospects in germplasm preservation of rare and endangered species. In: Reproduction Sciences in Animal Conservation (eds Holt, W.V., Brown, J.L. & Comizzoli, P.), pp. 331–56. New York, USA: Springer Science.CrossRefGoogle Scholar
Critser, J.K., Riley, L.K., Prather, R.S. (2003). In Reproduction Science and Integrated Conservation (eds Holt, W.V., Pickard, A.R., Rodger, J.C. & Wildt, D.E.), pp. 195208. Cambridge, UK: Cambridge University Press.Google Scholar
Dadras, H., Sampels, S., Golpour, A., Dzyuba, V., Cosson, J. & Dzyuba, B. (2017). Analysis of common carp Cyprinus carpio sperm motility and lipid composition using different in vitro temperatures. Anim. Reprod. Sci. 180, 3743.CrossRefGoogle ScholarPubMed
de Vries, A.C. & Colenbrander, B. (1990). Isolation and characterization of boar spermatozoa with and without a cytoplasmic droplet. Int. J. Biochem. 22, 519–24.CrossRefGoogle ScholarPubMed
Edmond, A.J., Teague, A.R., Brinsko, S.P., Comerford, K.L., Waite, J.A., Mancill, S.S., Love, C.C. & Varner, D.D. (2008). Effect of density gradient centrifugation on quality and recovery of equine spermatozoa. Anim. Reprod. Sci. 107(Abst. 16), 318.CrossRefGoogle Scholar
Faezah, S.S., Zuraina, F.M., Farah, J.H., Khairul, O., Hilwani, N.I., Iswadi, M.I., Fang, C.N., Zawawi, I., Abas, O.M. & Fatimah, S.I. (2014). The effects of magnetic separation on cryopreserved bovine spermatozoa motility, viability and cryo-capacitation status. Zygote 22, 378–86.CrossRefGoogle ScholarPubMed
Forero-González, RA, Celeghini, EC, Raphael, CF, Andrade, AF, Bressan, FF & Arruda, RP. (2012). Effects of bovine sperm cryopreservation using different freezing techniques and cryoprotective agents on plasma, acrosomal and mitochondrial membranes. Andrologia 44, 154–9.CrossRefGoogle ScholarPubMed
Galli, C., Vassiliev, I, Lagutina, I., Galli, A. & Lazzari, G. (2003). Bovine embryo development following ICSI: effect of activation, sperm capacitation and pre-treatment with dithiothreitol. Theriogenology 60, 1467–80.CrossRefGoogle ScholarPubMed
Galli, C., Duchi, R., Colleoni, S., Lagutina, I. & Lazzari, G. (2014). Ovum pick up, intracytoplasmic sperm injection and somatic cell nuclear transfer in cattle, buffalo and horses: from the research laboratory to clinical practice. Theriogenology 81, 138–51.CrossRefGoogle ScholarPubMed
Gil, M., Sar-Shalom, V. Sivira, Y.M., Carreras, R. & Checa, M.A. (2013). Sperm selection using magnetic activated cell sorting (MACS) in assisted reproduction: a systematic review and meta-analysis. J. Assist. Reprod. Genet. 30, 479–85.CrossRefGoogle ScholarPubMed
Gibb, Z, Butler, T.J., Morris, L.H.A., Maxwell, W.M.C., Grupen, C.G. (2013). Quercetin improves the postthaw characteristics of cryopreserved sex-sorted and nonsorted stallion sperm. Theriogenology 79, 1001–9.CrossRefGoogle ScholarPubMed
Gouk, S.S., Loh, Y.F., Kumar, S.D., Watson, P.F. & Kuleshova, L.L. (2011). Cryopreservation of mouse testicular tissue: prospect for harvesting spermatogonial stem cells for fertility preservation. Fertil. Steril. 95, 2399–403.CrossRefGoogle ScholarPubMed
Grupen, C.G. (2014). The evolution of porcine embryo in vitro production. Theriogenology 81, 2437.CrossRefGoogle ScholarPubMed
Hallap, T., Håård, M., Jaakma, U., Larsson, B. & Rodriguez-Martínez, H. (2004). Does cleansing of frozen–thawed bull semen before assessment provide samples that relate better to potential fertility? Theriogenology 62, 702–13.CrossRefGoogle ScholarPubMed
Hernández, M., Roca, J., Calvete, J.J., Sanz, L., Muiño-Blanco, T., Cebrián-Pérez, J.A., Vázquez, J.M., Martínez, E.A. (2007). Cryosurvival and in vitro fertilizing capacity postthaw is improved when boar spermatozoa are frozen in the presence of seminal plasma from good freezer boars. J. Androl. 28, 689–97.CrossRefGoogle ScholarPubMed
Herrid, M. & McFarlane, J. (2013). Application of testis germ cell transplantation in breeding systems of food producing species: a review, Anim. Biotechnol. 24, 293306.CrossRefGoogle ScholarPubMed
Herrid, M., Vignarajan, S., Davey, R., Dobrinski, I. & Hill, J.R. (2006). Successful transplantation of bovine testicular cells to heterologous recipients. Reproduction 132, 617–24.CrossRefGoogle ScholarPubMed
Holt, W.V. 2008. Cryobiology, wildlife conservation and reality. Cryolett. 29, 4352.Google Scholar
Holt, W.V., Pickard, A.R. & Prather, R.S. (2004). Reproduction 127, 317–24.CrossRefGoogle Scholar
Hoogewijs, M., Morrell, J.M., Van Soom, A., Govaere, J., Johannisson, A., Piepers, P., De Schauwer, C., de Kruif, A. & De Vliegher, S. (2011). Sperm selection using single layer centrifugation prior to cryopreservation can increase post thaw sperm quality in stallions. Equine Vet. J., 43 (Suppl 40), 3541.CrossRefGoogle Scholar
Humblot, P., Le Bourhis, D., Fritz, S., Colleau, J.J., González, C., Guyader Joly, C., Malafosse, A., Heyman, Y., Amigues, Y., Tissier, M. & Ponsart, C. (2010). Reproduction technologies and genomic selection in cattle. Vet. Med. Int. Article ID 192787, doi:10.4061/2010/192787 CrossRefGoogle ScholarPubMed
International Union for Conservation of Nature (IUCN) (2016). IUCN Red List of Threatened Species. Version 2016-1. http://www.iucnredlist.org. Accessed 30 June 2016.Google Scholar
Isachenko, E., Mallmann, P., Rahimi, G., Risopatròn, J., Schulz, M., Isachenko, V. & Sànchez, R. (2012). Vitrification technique – new possibilities for male gamete low-temperature storage. In Current Frontiers in Cryobiology (ed. Katkov, I.I.), InTechOpen. ISBN: 978-953-51-0191-8.Google Scholar
Jovanovic, J., Ronneberg, J.A., Tost, J. & Kistensen, V. (2010). The epigenetics of breast cancer. Mol. Oncol. 4, 242–54.CrossRefGoogle ScholarPubMed
Kobayashi, T., Takeuchi, Y., Takeuchi, T. & Yoshizaki, G. (2007). Generation of viable fish from cryopreserved primordial germ cells. Mol. Reprod. Dev. 74, 207–13.CrossRefGoogle ScholarPubMed
Leite, T.G., do Vale-Filho, V.R., de Arruda, R.P., de Andrade, A.F., Emerick, L.L., Zaffalon, F.G., Martins, J.A. & de Andrade, V.J, (2010). Effects of extender and equilibration time on post-thaw motility and membrane integrity of cryopreserved Gyr bull semen evaluated by CASA and flow cytometry. Anim. Reprod. Sci. 120, 31–8.CrossRefGoogle ScholarPubMed
Lindemann, C.B., O'Brien, J.A. & Giblin, F.J. (1988). An investigation of the effectiveness of certain antioxidants in preserving the motility of reactivated bull sperm models. Biol Reprod. 38, 114–20.CrossRefGoogle ScholarPubMed
Loomis, P.R. & Graham, J.K. (2008). Commercial semen freezing: Individual male variation in cryosurvival and the response of stallion sperm to customized freezing protocols. Anim. Reprod. Sci. 105, 119–28.CrossRefGoogle ScholarPubMed
Lunardi, F.O., Araújo, V.R., Bernuci, M.P., Lunardi, L.O., Gonçalves, R.F., Carvalho Ade, A., de Figueiredo, J.R. & Rodrigues, A.P. (2012). Restoring fertility after ovarian tissue cryopreservation: a half century of research. Zygote 21, 394405.CrossRefGoogle ScholarPubMed
Luño, V., Gil, L., Olaciregui, M., González, N., Jerez, R.A. & de Blas, I. (2014). Rosmarinic acid improves function and in vitro fertilising ability of boar sperm after cryopreservation. Cryobiology 69, 157–62.CrossRefGoogle ScholarPubMed
Machado, G.M., Carvalho, J.O., Filho, E.S., Caixeta, E.S., Franco, M.M., Rumpf, R. & Dode, M.A. (2009). Effect of Percoll volume, duration and force of centrifugation, on in vitro production and sex ratio of bovine embryos. Theriogenology 71, 1289–97.CrossRefGoogle ScholarPubMed
Malcuit, C., Maserati, M., Takahashi, Y., Page, R. & Fissore, R.A. (2006). Intracytoplasmic sperm injection in the bovine induces abnormal Ca2+ responses and oocyte activation. Reprod. Fertil. Dev. 18, 3951.CrossRefGoogle ScholarPubMed
Mari, G., Castagnetti, C., Rizzato, G., Mislei, B., Iacono, E. & Merlo, B. (2011). Density gradient centrifugation of sperm from a subfertile stallion and effect of seminal plasma addition on fertility. Anim. Reprod. Sci. 126, 96100.CrossRefGoogle ScholarPubMed
Marrs, R.P., Serafini, P.C., Kerin, J.F., Batzofin, J., Stone, B.A., Brown, J., Wilson, L. & Quinn, P. (1988). Methods used to improve gamete efficiency. Ann. NY Acad. Sci. USA 541, 310–6.CrossRefGoogle ScholarPubMed
Martinez-Alborcia, M.J., Morrell, J.M., Barranco, I., Maside, C., Gil, M.A., Parrilla, I., Vazquez, J.M., Martinez, E.A. & Roca, J. (2013). Suitability and effectiveness of single layer centrifugation using Androcoll-P in the cryopreservation protocol for boar spermatozoa. Anim. Reprod. Sci. 140, 173–9.CrossRefGoogle ScholarPubMed
Martínez-Páramo, S., Horváth, A., Labbé, C., Zhang, T., Robles, V., Herráez, P., Suquet, M., Adams, S., Viveiros, A., Tiersch, T.R. & Cabrita, E. (2017). Cryobanking of aquatic species Aquaculture 472, 156–77.CrossRefGoogle ScholarPubMed
Moore, A.I., Squires, E.L. & Graham, J.K. (2005). Effect of seminal plasma on the cryopreservation of equine spermatozoa. Theriogenology 63, 2372–81.CrossRefGoogle ScholarPubMed
Morita, T., Kumakura, N., Morishima, K., Mitsuboshi, T., Ishida, M., Hara, T., Kudo, S., Miwa, M., Ihara, S., Higuchi, K., Takeuchi, Y. & Yoshizaki, G. (2012). Production of donor-derived offspring by allogenic transplantation of spermatogonia in the yellowtail (Seriola quinqueradiata). Biol. Reprod. 86, 111.CrossRefGoogle ScholarPubMed
Morrell, J.M., Dalin, A-M & Rodriguez-Martinez, H. (2008a). Prolongation of stallion sperm survival by centrifugation through coated silica colloids: a preliminary study. Anim. Reprod. 5, 121–6.Google Scholar
Morrell, J.M., Peña, F.J., Johannisson, A., Dalin, A.-M., Samper, J.C., Rodriguez-Martinez, H. (2008b). Techniques for sperm clean-up and selection of stallion spermatozoa. Anim. Reprod. Sci. 107, 333–4.CrossRefGoogle Scholar
Morrell, J.M. & Rodriguez-Martinez, H. (2009). Biomimetic techniques for improving sperm quality in animal breeding: a review. Open Androl. J. 1, 19.Google Scholar
Morrell, J.M., Johannisson, A., Dalin, A-M. & Rodriguez-Martinez, H. (2009). Single layer centrifugation with Androcoll™-E can be scaled-up to allow large volumes of stallion ejaculate to be processed easily. Theriogenology 72, 879–84.CrossRefGoogle ScholarPubMed
Morrell, J.M. & Rodriguez-Martinez, H. (2011). Practical applications of sperm selection techniques as a tool for improving reproductive efficiency. Vet. Med. Int. Article ID 894767. doi:10.4061/2011/894767.CrossRefGoogle Scholar
Morrell, J.M. & Wallgren, M. (2011). Colloid centrifugation of boar semen. Reprod. Domest. Anim. 46, 1822.CrossRefGoogle ScholarPubMed
Morrell, J.M., Johannisson, A. & Rodriguez-Martinez, H. (2011). Effect of osmolarity and density of colloid formulations on the outcome of SLC-selection of stallion spermatozoa. ISRN Vet. Sci. 2011, Article ID 128984, 5 pp. doi:10.5402/2011/128984.CrossRefGoogle ScholarPubMed
Morrell, J.M., van Wienen, M. & Wallgren, M. (2011). Single layer centrifugation can be scaled-up further to process up to 150 mL semen. ISRN Vet. Sci. Article ID 183412, doi: 10.5402/2011/183412.CrossRefGoogle ScholarPubMed
Morrell, J.M. & Wallgren, M. (2011). Removal of bacteria from boar ejaculates by single layer centrifugation can reduce the use of antibiotics in semen extenders. Anim. Reprod. Sci. 123, 64–9.CrossRefGoogle ScholarPubMed
Morrell, J.M., Richter, J., Martinsson, G., Stuhtmann, G., Hoogewijs, M., Roels, K. & Dalin, A.-M. 2014. Pregnancy rates are higher after artificial insemination with cooled stallion spermatozoa selected by single layer centrifugation than with control semen doses. Theriogenology 82, 1102–5.CrossRefGoogle Scholar
Morrell, J.M. & Wallgren, M. (2014). Alternatives to antibiotics in semen extenders: a review. Pathogens 3, 934–46.CrossRefGoogle ScholarPubMed
Morrell, J.M. & Rodriguez-Martinez, H. (2016). Colloid centrifugation of semen: applications in assisted reproduction. Am. J. Anal. Chem. 7, 597610.CrossRefGoogle Scholar
Mortimer, D. (2000). Sperm preparation methods. J. Androl. 21, 357–66CrossRefGoogle ScholarPubMed
Munro, S.K., Farquhar, C.M., Mitchell, M.D. & Ponampalam, A.P. (2010). Epigenetic regulation of endometrium during the menstrual cycle. Mol. Hum. Reprod. 16, 297310.CrossRefGoogle ScholarPubMed
Nicholson, C.M., Abramsson, L., Holm, S.E. & Bjurulf, E.X. (2000). Bacterial contamination and sperm recovery after semen preparation by density gradient centrifugation using silane-coated silica particles at different g forces. Hum. Reprod. 15, 662–6.CrossRefGoogle ScholarPubMed
Okutsu, T., Suzuki, K., Takeuchi, Y. & Yoshizaki, G. (2006). Testicular germ cells can colonize sexually undifferentiated embryonic gonad and produce functional eggs in fish. Proc. Natl. Acad. Sci. USA 103, 2725–9.CrossRefGoogle ScholarPubMed
Okutsu, T., Shikina, S., Kanno, M., Takeuchi, Y. & Yoshizaki, G. (2007). Production of trout offspring from triploid salmon parents. Science 317, 1517.CrossRefGoogle ScholarPubMed
Polge, C., Smith, A.U. & Parkes, A.S. (1949). Revival of spermatozoa after vitrification and revival at low temperature. Nature 164, 666.CrossRefGoogle Scholar
Rodriguez-Martinez, H., Hultgren, J., Båge, R., Bergqvist, A-S., Svensson, C., Bergsten, C., Lidfors, L., Gunnarsson, S., Algers, B., Emanuelson, U., Berglund, B., Andersson, G., Håård, M., Lindhé, B., Stålhammar, H. & Gustafsson, H. (2008). Reproductive performance in high-producing dairy cows: can we sustain it under current practice? In IVIS Reviews in Veterinary Medicine (ed.). International Veterinary Information Service, Ithaca NY (www.ivis.org), Last updated: 12 December 2008; R0108.1208 (Open Journal), 23 pp.Google Scholar
Röpke, T., Oldenhof, H., Leiding, C., Sieme, H., Bollwein, H. & Wolkers, W.F., (2011). Liposomes for cryopreservation of bovine sperm. Theriogenology 76, 1465–72.CrossRefGoogle ScholarPubMed
Ryder, O.A. & Benirschke, K. (1997). The potential use of ‘cloning’ in the conservation effort. Zoo Biol. 16, 295300.3.0.CO;2-5>CrossRefGoogle Scholar
Saito, T., Goto-Kazeto, R., Fujimoto, T., Kawakami, Y., Arai, K. & Yamaha, E. (2010). Inter-species transplantation and migration of primordial germ cells in cyprinid fish. Int. J. Dev. Biol. 54, 1479–84.CrossRefGoogle ScholarPubMed
Sánchez, R., Risopatrón, J., Schulz, M., Villegas, J., Isachenko, V., Kreinberg, R. & Isachenko, E. (2011). Canine sperm vitrification with sucrose: effect on sperm function. Andrologia 43, 233–41.CrossRefGoogle ScholarPubMed
Saragusty, J. & Arav, A. (2011). Current progress in oocyte and embryo cryopreservation by slow freezing and vitrification. Reproduction 141, 119.CrossRefGoogle ScholarPubMed
Schagdarsurengin, U. & Steger, K. (2016). Epigenetics in male reproduction: effect of paternal diet on sperm quality and offspring health. Nat. Rev. Urol. 13, 584–95.CrossRefGoogle ScholarPubMed
Seki, S., Kouya, T., Tsuchiya, R., Valdez, D.M., Jin, B., Koshimoto, C. Kasai, M. & Edashige, K. (2011). Cryobiological properties of immature zebrafish oocytes assessed by their ability to be fertilized and develop into hatching embryos. Cryobiology 62, 814.CrossRefGoogle ScholarPubMed
Serafini, P., Blank, W., Tran, C., Mansourian, M., Tan, T. & Batzofin, J. (1990). Enhanced penetration of zona-free hamster ova by sperm prepared by Nycodenz and Percoll gradient centrifugation. Fertil. Steril. 53, 551–5.CrossRefGoogle ScholarPubMed
Sharma, R.K., Seifarth, K. & Agarwal, A. (1997). Comparison of single- and two-layer Percoll separation for selection of motile spermatozoa. Int. J. Fertil. Womens Med. 42, 412–7.Google ScholarPubMed
Sławeta, R., Waşowicz, W. & Laskowska, T. (1988). Selenium content, glutathione peroxidase activity, and lipid peroxide level in fresh bull semen and its relationship to motility of spermatozoa after freezing-thawing. Zentralbl Veterinarmed. 35, 455–60.CrossRefGoogle ScholarPubMed
Sprícigo, J.F.W., Diógenes, M.N., Leme, L.O., Guimarães, A.L., Muterlle, C.V., Silva, B.D.M., Solà-Oriol, D., Pivato, I., Silva, L.P. & Dode, M.A.N. (2015). Effects of different maturation systems on bovine oocyte quality, plasma membrane phospholipid composition and resistance to vitrification and warming. PLoS One 10, e0130164.CrossRefGoogle ScholarPubMed
Stockwell, S., Hill, J.R., Davey, R., Herrid, M., Lehnert, S.A. (2013). Transplanted germ cells persist long-term in irradiated ram testes. Anim. Reprod. Sci. 142, 137–40.CrossRefGoogle ScholarPubMed
Suarez, S. (2007). Interactions of spermatozoa with the female reproductive tract: inspiration for assisted reproduction. Reprod. Fertil. Dev. 19, 103–10.CrossRefGoogle ScholarPubMed
Tarig, A.A., Wahid, H., Rosnina, Y., Yimer, N., Goh, Y.M., Baiee, F.H., Khumran, A.M., Salman, H. & Ebrahimi, M. (2017). Effect of different concentrations of egg yolk and virgin coconut oil in Tris-based extenders on chilled and frozen–thawed bull semen. Anim. Reprod. Sci. 182, 21–7.CrossRefGoogle ScholarPubMed
Tiersch, T.R., Yang, H., Jenkins, J.A. & Dong, Q. (2007). Sperm cryopreservation in fish and shellfish. Soc. Reprod. Fertil. Suppl. 65, 493508.Google ScholarPubMed
Urrego, R., Rodriguez-Osorio, N. & Niemann, H. (2014). Epigenetic disorders and altered gene expression after use of assisted reproductive technologies in domestic cattle, Epigenetics 9, 803–15.CrossRefGoogle ScholarPubMed
Valcarce, D.G., Herráez, M.P., Chereguini, O., Rodríguez, C. & Robles, V. (2016). Selection of nonapoptotic sperm by magnetic-activated cell sorting in Senegalese sole (Solea senegalensis). Theriogenology 86, 1195–202CrossRefGoogle ScholarPubMed
Vasicek, J., Makarevich, A.V. & Chrenek, P. (2013). Impact of the MACS on elimination of apoptotic spermatozoa from rabbit ejaculates. Slovak J. Anim. Sci. 46, 8792.Google Scholar
Veerkamp, R.F. & Beerda, B. (2007). Genetics and genomics to improve fertility in high producing dairy cow. Theriogenology 68 (Suppl 1), S266–73.CrossRefGoogle Scholar
Watson, P.F. (1995). Recent developments and concepts in the cryopreservation of spermatozoa and the assessment of their post-thawing function. Reprod. Fertil. Dev. 7, 871–91.CrossRefGoogle ScholarPubMed
Weber, G.M. & Lee, C.-S. (2014). Current and future assisted reproductive technologies for fish species. In Current and Future Reproduction Technologies and World Food Production (eds Lamb, G.C. & DiLorenzo, N.), pp. 3376. New York USA: Springer Science.CrossRefGoogle Scholar
Woelders, H., Windig, J. & Hiemstra, S.J. (2012). How developments in cryobiology, reproduction technologies and conservation genomics could shape gene banking strategies for (farm) animals. Reprod. Domest. Anim. 47 (Suppl. 4), 264–73.CrossRefGoogle ScholarPubMed
Wu, J., Hu, T., Guo, B., Yue, Z., Yang, Z. & Zhang, X. (2011). Cryopreservation of adult bovine tissue for spermatogonia enrichment. CryoLetters 32, 402–9.Google ScholarPubMed
Yang, C.H., Wu, T.W., Cheng, F.P., Wang, J.H. & Wu, J.T. (2016). Effects of different cryoprotectants and freezing methods on post-thaw boar semen quality. Reprod. Biol. 16, 41–6.CrossRefGoogle ScholarPubMed
Ye, H., Li, C.J., Yue, H.M., Du, H., Yang, X.G., Yoshino, T., Hayashida, T., Takeuchi, Y. & Wei, Q.W. (2017). Establishment of intraperitoneal germ cell transplantation for critically endangered Chinese sturgeon Acipenser sinensis . Theriogenology 94, 3747.CrossRefGoogle ScholarPubMed
Yoshizaki, G., Okutsu, T., Morita, T., Terasawa, M., Yazawa, R. & Takeuchi, Y. (2012). Biological characteristics of fish germ cells and their application to developmental biotechnology. Reprod. Domest. Anim. 47, 187–92.CrossRefGoogle ScholarPubMed
Figure 0

Table 1 Comparison of slow freezing and vitrification for embryos and oocytes

Figure 1

Figure 1 Principle of surrogate reproduction in fish. Conservation of a threatened species can be achieved by transplanting frozen PGCs or spermatogonia into recipient embryos of a closely related species (adapted from Yoshizaki et al., 2012).

Figure 2

Table 2 Chronology of colloid centrifugation as a sperm preparation technique