Reproductive Biotechnologies in Beef Cattle: Five Decades of Research in Mexico
Reproductive Biotechnologies in Beef Cattle: Five Decades of Research in Mexico
Reproductive Biotechnologies in Beef Cattle: Five Decades of Research in Mexico
5918
Review
a
Instituto Nacional de Investigaciones Forestales Agrícolas y Pecuarias (INIFAP). Sitio
Experimental Las Margaritas. Km 9.5 carretera federal Hueytamalco-Tenampulco,
Hueytamalco, Puebla. México.
b
INIFAP. Centro Nacional de Recursos Genéticos. Blvd. De la Biodiversidad Nº 400,
Tepatitlán de Morelos, Jalisco. México.
c
Universidad Autónoma de Querétaro. Facultad de Ciencias Naturales. Av. de las Ciencias
S/N, Juriquilla, Querétaro. México.
d
INIFAP. Campo Experimental Paso del Toro. Km 22.5 carretera federal Veracruz-Córdoba,
Medellín, Veracruz. México.
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Abstract:
The main bovine reproductive biotechnologies are recapitulated herein in five sections, and
their historical development and current status are analyzed, including the results generated
in Mexico. In the 1970s, estrus synchronization and ovulation induction began; thus, the
reproductive cycle started to be controlled with the resources available at that time, based on
the knowledge of bovine reproductive physiology. Over the years, hormone therapy evolved
as new compounds were discovered, refining methods to standardize the effect and
generating new methods for the release of hormones. The most widely used biotechnology
in the world, artificial insemination, owes its expansion to advances in semen processing,
among which the development of diluents, cryopreservation, semen sexing, and computer-
assisted sperm analysis stand out. The embryonic era began with the development of multi-
ovulation and methods for collecting, evaluating, transferring, and cryopreserving embryos.
The second embryonic era came with the fully in vitro production of embryos from immature
eggs and frozen sperm, known as in vitro embryo production. Great research and material
resources have been invested in this procedure, rendering it a pillar of genetic improvement
and productivity, in combination with two other tools: sexed semen and genomic evaluations.
A golden age of in vitro embryo production is on the horizon, with the possibility to produce
accurate modifications in the embryo genome, thanks to gene editing technology.
Received: 04/01/2021
Accepted: 30/04/2021
Introduction
The text of the FAO Convention on Biological Diversity (CBD)(1), in force since 1993, states
that the term "biotechnology" refers to any technological application that uses biological
systems, living organisms (or derivatives thereof) to make or modify products or processes
for a specific use. In this sense, and for the purposes of the topics to be covered in this review,
reproductive biotechnology will be understood as the technological applications that affect
the physiological processes of animal reproduction, their gametes and embryos, for the
purpose of achieving productive improvements.
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This document will cover only the bovine species and will place particular emphasis on the
research carried out by institutions and universities in Mexico, particularly the National
Institute for Research in Forestry, Agriculture and Livestock (INIFAP), in its 35 years of
existence, and its predecessor: the National Institute of Livestock Research (INIP).
While the authors do not claim this to be an exhaustive review of all the reproductive
biotechnologies that have been applied to cattle, it is address those that have had the greatest
impact on productivity and briefly mention those that have had minimal or no application in
Mexico, such as transgenesis and cloning.
The topics of estrus synchronization and ovulation induction are discussed first, as they are
the topics on which research has been conducted for the longest time (50 yr) and for which
INIP-INIFAP has generated the largest number of technologies. Biotechnologies developed
for semen collection, dilution, and cryopreservation have underpinned the massive use of
bulls of high genetic merit through artificial insemination (AI). This topic will be discussed,
with emphasis on recent developments such as semen sexing and computer-assisted sperm
analysis. Issues related to embryo manipulation, including multi-ovulation and embryo
transfer (MOET), in vitro embryo production (IVP), and transvaginal oocyte aspiration
(TVA) have seen important developments in recent years, which will be addressed in this
paper. In addition to including research results on these topics, in some cases, mention will
be made of government or producer organization programs that marked a milestone in the
dissemination and adoption of these reproductive biotechnologies.
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The first studies date back to 1948(14), when progesterone (50 mg/d, i.m.) was used to block
estrous cyclicity for a period of up to 13 d. It was observed that, at the end of its effect, a
good proportion of females presented estrus at 4 and 5 d. Later, with the addition of estrogens
to the treatment, estrus presentation increased, and the progesterone blocking time was
reduced(15). The use of hormonal products such as 19 alpha acetoxy-11 beta-methyl-19 norg
4-ene-3, 2-dione (a very potent progestogen known as SC21009), natural progesterone,
estradiol valerate (EV), and prostaglandin F2α (PGF2α) began in the 1970s; at this time,
work focused on estrus synchronization(16), the resolution of prolonged postpartum anestrus
in cows, and the attempt to advance puberty in heifers(17-21). Thus, heifers of European breeds,
Creole breeds, and pre-pubertal zebu crossbreeds, treated with 5 mg of EV (i.m.) + 3 mg of
SC21009 (i.m.) + 6 mg of SC21009 (auricular implant removed on d 9), had 79 % of estrus
presentation in the first 48 h of implant removal, compared to control heifers, of which only
6 % exhibited estrus(21). In another study(22) with anestrus cows and fattened zebu heifers, it
was observed that, in females treated with progesterone (25 mg i.m. for 5 d) + estradiol
cypionate (EC; 2 mg i.m. on the first day) or with SC21009 (3 mg for 5 d in subcutaneous
implant) + EC (2 mg i.m. on the first day), the estrus was synchronized at 72 h, with an estrus
rate (ER) of 61.1 and 73.7 %, and a conception rate (CR) of 44.4 and 31.3 %, respectively.
On the contrary, in females that received the control and individual treatments (progesterone,
SC21009 or EC) with the same doses, estrus was not synchronized at 72 h, and they had a
low TC, from 10.5 to 21.1 %, during the 30 d of the study.
In another experiment(23) with zebu cows with calf and at 60 d postpartum, the effectiveness
of SC21009 + EV was evaluated. In the first 48 d, the ER in treated cows was 24 %, and
0 % in untreated cows, while the CR was 12 and 0 %, respectively. However, at the end of
the AI period (d-48), 20 % of the treated cows were pregnant, and 12 % of the untreated cows
were pregnant; at the end of mating (d-68; AI + natural mating), 28 % of the treated cows
were pregnant, but only 12 % of the untreated cows were pregnant. However, in non-breeding
zebu cows, after applying 6 mg of EV + 3 mg of SC21009 via i.m. + 6 mg of SC21009 in
subcutaneous implant, it was observed that 100 % of the treated cows showed estrus in the
first 48 h after the implant was removed, in contrast to the untreated cows, of which only
29.4 % exhibited estrus. The CR was 42.8 % in treated cows, and 14.7 % in untreated cows.
This indicates that synchronization groups the estruses in order to facilitate AI and overall
herd management(24), but provides evidence that it is more difficult to reduce the anestrus
period in cows with calves, a circumstance that reveals the importance of reducing or
eliminating the effect of lactation on the return to estrous cyclicity.
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Progestogen melengestrol acetate (0.5 mg/d for 9 d) in feed, combined with EV (single dose
of 6 mg i.m. on d 1) and progesterone (single dose of 50 mg on d 1), was tested in Brown
Swiss x Zebu cows and heifers. It was observed that the percentage of cows inseminated at
48 days after mating was 38.9, 51.5, and 75.8 %, respectively, in control cows, in cows
conventionally inseminated at detected estrus, and in cows inseminated at any sign of estrus.
The percentage of cows inseminated was significantly higher when insemination was
performed before any sign of estrus. CRs were statistically similar between treatments (20.9,
28.8 and 37.1 %, respectively), despite the fact that the estruses were clustered among the
cows in each treatment(25). Estrus synchronization with melengestrol acetate is not a
widespread practice in Mexico, despite its proven efficacy, because it is not practical to
perform it in small groups of animals, and small herds are predominant in our country.
Because some females did not exhibit estrus even when treated hormonally, the decision was
made to research the convenience of inseminating at pre-established schedules. Thus, in
Brangus and Creole heifers, AI was performed at preset times in anestrus females because
the percentage of animals in estrus in the first 5 days after removal of the implant was very
low (53.1 %). Under this premise, heifers were inseminated at 48, 54 and 60 h after implant
removal, resulting in CRs of 54.5, 60.6 and 47.0 %, with higher CRs at 48 and 54 h after
implant removal(26). These results set the tone for the initiation of many studies on estrus
synchronization with FTAI.
On the other hand, studies were carried out with estrus synchronization in grazing beef cattle
during 85-d mating seasons (matings), when AI is difficult to perform. Thus, in humid
subtropical climate with non-breeding zebu cows, the ER in the first 60 h of mating was
higher in cows treated with SC21009 (9 or 6 mg for 9 d) + EV (6 mg on d 1 of the 9-d
treatment) than in untreated cows (84 vs 0 %). Similarly, CR at 26 ds after mating favored
treated cows over untreated cows (59 vs 40 %), although at the end of the mating period there
were no differences in CR between treatments(27).
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The availability of PGF2α in the early 1970s made it possible to start work on estrus
synchronization in cycling females, a status that was confirmed through the detection of a
corpus luteum(28,29). A CR of 34.8 % was obtained in cycling Brangus, Gyr and Charolais
heifers treated with PGF2α and artificially inseminated 80 h after treatment; this percentage
was similar to that of heifers synchronized and inseminated 12 h after estrus was observed
(CR= 26.1 %). At the end of mating (90 d), in heifers inseminated at 80 h, a TC of 69.6 %
was obtained, similar to the TC (56.5 %) of heifers artificially inseminated 12 h after
estrus(30). Studies on estrus synchronization facilitated the reproductive management of
grazing cattle, since it allows females to be served in the first days of mating(13,23-26).
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The introduction of the PIDR into the market revolutionized estrus synchronization(37), and,
therefore, researchers from INIFAP(38,39) started using this device in cows in anestrus and
cycling cows with good body condition (BC), obtaining a CR of 44.8, 77.1 and 100.0 % at
3, 30 and 60 d after PIDR withdrawal, respectively(38). In Bos taurus x Bos indicus(39) heifers,
the CR with PIDR and FTAI at 84 h after the removal of the device was higher than with
conventional AI at 12 h after the detection of estrus (36.4 vs 18.2 %, respectively). Similarly,
the CR with CRESTAR and FTAI at 84 h after device removal was higher than with
conventional AI (27.3 vs 18.2 %, respectively). In this work, the advantage of FTAI at 84 h
after the removal of the device was demonstrated, since pregnancy was achieved in some
heifers that did not exhibit estrus. A frequent practice in estrus and ovulation synchronization
protocols with FTAI in which PIDR and PGF2α are used in association with estradiol
benzoate (EB) (which is applied when inserting the PIDR on d 0 and the day after its removal)
is the substitution of GnRH for EB. This is because, like EB, GnRH synchronizes the
emergence of a new wave of follicular development, which culminates in the ovulation of
the mature follicle, giving good results. However, if a significant proportion of the cows are
suspected to be in anestrus, it is recommended to additionally apply 400 IU of equine
chorionic gonadotropin eCG on d 7 of the protocol. Furthermore, EB can be replaced with
GnRH (100 µg i.m.), on the first application (d 1 of PIDR), but the second application must
be carried out at the time of FTAI. An example for cycling cows is shown in Figure 1(40).
It has been shown that body condition (BC) is an indicator of the cow's nutritional status and
that, if the cow has a good BC before and after calving, her fertility improves soon after
giving birth(41). In addition, this has been shown to be associated with high concentrations of
insulin-like growth factor-1 (IGF-1), leptin and insulin, allowing early resumption of
postpartum estrous activity(42). Therefore, other research focused on studying changes in the
blood concentration of these three hormones as metabolic indicators of the nutritional status
of the animals, observing that a low BC in females (<6.0 units; scale 1 to 9) is associated
with a reduction in the blood concentration of insulin and IGF-1, without changes in leptin,
which diminishes the response to postpartum estrus induction in beef cows(43,44). Therefore,
females that are synchronized and enter mating should have good BC (of no less than 3.0),
in order to favor the occurrence of estrus and achieve gestation(45).
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Kisspeptins are peptides that are named for their number of amino acids: kisspeptin-54,
kisspeptin-14, kisspeptin-13 and kisspeptin-10(46). Synthesizing neurons are considered to be
integrators of signals that modulate the functionality of the somatotropic and gonadal axis(47).
Studies with intravenous kisspeptin-10 (kiss-10) (5 µg/kg bw) produced increases in LH,
FSH, and growth hormone secretion in prepubertal male and female calves(48,49), LH
increased with age in all calves, with mean values of 6.1, 7.2 and 11.6 ng/ml at 4, 7 and 11
mo of age, respectively(50). The highest LH concentration was found in 11-month-old calves.
In an attempt to understand the sensitivity of the gonadotropic axis to kiss-10, other studies
tested intravenous doses of 0.1, 1.0, 2.0, 3.0, 4.0 and 5.0 µg/kg bw(51) and 50.0 µg/kg(52) in
prepubertal calves, showing that effective doses for inducing LH release ranged from 1.0 to
5.0 µg/kg. Therefore, the application of low doses, less than 5 µg/kg body weight, could
considerably reduce the cost of treatment with this peptide(51). In a subsequent experiment
with prepubertal calves using kisspeptin-10 at a dose of 5 µg/kg-bw applied every 2 h for 84
h (3.5 d), ovulation and corpus luteum formation were induced in 28.5 % of the calves;
however, the corpus luteum disappeared and the calves returned to their prepubertal state(53).
Later, it was found that, in (European x zebu) beef cows, at 78 d postpartum, with anestrus,
and nursing their calf, kisspeptin-10 at a dose of 1 μg/kg-bw every 2 h for 24 h also
augmented the serum LH concentration, an increase that emulated a brief LH pulse(54). This
result prompted an ovulation synchronization study, such that kisspeptin-10 was tested at a
total dose of 500 µg at the time of FTAI, compared to GnRH (100 µg at the time of FTAI)
and eCG (400 IU on withdrawal of PIDR on d 7), in a protocol in which each hormone was
combined with PIDR, BE (2 mg at PIDR application + 1 mg the day after PIDR withdrawal),
and cloprostenol (total dose of 500 µg at PIDR withdrawal), in non-calving, 180-d
postpartum beef cows inseminated between 54 and 56 h after PIDR withdrawal. The
ovulation rate for the eCG, GnRH and kisspeptin-10 treatments was 89.2, 96.5 and 93.8 %,
while the conception rate was 43.6, 73.8 and 54.3 % respectively, with no significant
statistical differences between treatments in either case(55). This result could be of interest to
the pharmaceutical industry as an alternative for ovulation synchronization and induction.
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Figure 1: General outline of estrous synchronization in cows and heifers with FTAI(40)
AI was the first reproductive biotechnology applied to improve production through the more
efficient use of bulls of high genetic merit. The widespread use of this technique and the
achievement of its full potential required the cryopreservation of semen for long periods of
time.
The first report of semen cryopreservation was made in 1776(56), where it was observed that
when spermatozoa from human, guinea pig and frog were cooled in snow for up to 30 min,
they became inactive, but could be reactivated. In 1940(57), egg yolk began to be used to
protect bull sperm cells from thermal shock upon cooling. In 1941 (58), the sperm extender
was improved by using egg yolk with sodium citrate, which allowed semen preservation at 5
°C for up to 3 d. In 1949, bull spermatozoa were frozen for the first time by using glycerol
in the diluent. The great discovery of the cryoprotective action of glycerol opened a
successful era in the cryopreservation not only of gametes of various species, but also of
other cells and tissues(59). The so-called Cornell diluent, created by Foote and Bratton in
1950(60), contained a mixture of the antibiotics penicillin, streptomycin, and polymyxin B,
and was used for many years as standard. In 1952, in Cambridge, the first calf was born from
frozen-thawed bovine sperm(61).
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Reports of fertility with frozen spermatozoa from bulls led to an intense development of
cryopreservation methods to try to improve the results obtained, so other disciplines (such as
molecular biology) associated with the cryopreservation process began to be used. Such is
the case of proteomics(62) and genetic engineering(63). On these issues, a study was carried
out in Mexico with INIFAP researchers, where the addition of recombinant FAA (fertility-
associated antigen) and recombinant TIMP-2 (tissue inhibitor of metalloproteinases 2) to
frozen bovine semen was evaluated and proved to significantly increase its fertility(64).
Sperm sexing
Advances in AI have generated interest in using AI for sex selection in dairy cattle. For this
reason, over time, many researchers have tried to separate spermatozoa with "X" and "Y"
chromosomes using various techniques(65). In the 1980s, flow cytometry began to be applied,
making it possible to separate spermatozoa according to their sex chromosomes and amount
of DNA. It took about 20 yr for this technology to be commercialized for use in AI in cattle.
This technique is based on the fact that spermatozoa with an "X" chromosome in cattle
contain 3.8 % more DNA than "Y" spermatozoa(66). This technology had an efficiency of 85
to 95 % (in terms of separation of sperm with X or Y chromosome); however, it had not been
fully perfected(67).
The first commercial production of sexed semen took place at the Cogent company in the
United Kingdom(65). Although it had a relatively slow start, bovine sexed semen production
increased exponentially with an estimated 4 million doses in 2008(68).
The sexed semen was marketed in 0.25 ml straws at a concentration of 2.1 million
spermatozoa(69). This concentration was due to the fact that, at the time of semen sexing,
approximately 80 % of the ejaculate was lost between the sperm of the unwanted sex and the
sperm that could not be differentiated, in addition to the long time that the separation process
took(70). Despite the limitations of sexed semen, it was clearly a welcomed development(68).
Acceptable gestation percentages were achieved with the reduced dose (2.1 x 106 sperm) of
sexed semen in heifers, but little work was done with lactating cows(66). Nowadays, sperm
sexing technology has evolved, modifying the techniques, increasing the speed of sexing,
decreasing stress on spermatozoa, increasing concentration and, therefore, improving sperm
viability parameters.
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In 1997, research was conducted with two objectives: 1) to evaluate conception rates of
heifers inseminated (in the uterine horn, ipsilateral to the ovary with the largest follicle) with
reduced doses of semen (1 x 105; 2.5 x 105; 2.5 x 106 sperm/0.21 ml) chilled at 5 °C under
ideal conditions at the field level; 2) to evaluate conception rates of heifers inseminated (in
the uterine horn, ipsilateral to the ovary with the largest follicle) with reduced doses of sexed
semen (1-2 x105 sperm/0.1 ml) refrigerated at 5 °C. In experiment 1, gestation percentages
at 40 d were 41, 50 and 61 % for 1 x 105; 2.5 x 105; 2.5 x 106 spermatozoa/IA respectively.
In experiment 2, out of 67 heifers inseminated, 22 % were pregnant, and 82 % of the offspring
were of the selected sex(71). Research indicates that AI with lower than conventional sperm
doses is possible when using sexed sperm, 2.1 x 106 spermatozoa being most commonly used
in the insemination dose, against at least 10x106, which is used with unsexed sperm.
Subsequently, in 1999, another research was carried out with the objective of evaluating the
freezing process of the sexed semen; this was achieved because the semen was processed in
a MoFlow SX™ flow cytometer, that allowed to have sufficient quantity of spermatozoa,
unlike when working with the EPICS V flow cytometer. In this work it was determined that
the use of the laser at a power of 100 mW had a lower impact on the progressive motility of
post-thawed semen than when it was used at 150 mW. It was also observed that post-thawing
progressive motility was higher when using a TRIS-based diluent than when using citrate-
egg yolk or TEST. Regarding the equilibration time (adaptation to the cryoprotectant) at 5
°C prior to freezing, it was concluded that progressive motility was better after thawing for
3 to 6 h than when this took 18 h. On the other hand, it was determined that it was better to
keep fresh semen for 4 to 7 h at 22 °C than to dilute it with TALP medium added with Hoechst
33342 fluorochrome. These new sperm sexing procedures yielded slightly lower results in
terms of motility and acrosomal integrity than conventional semen. With these results, it was
considered that the use of sexed semen for commercial AI would be available in
approximately 2 yr(72).
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The Monsanto Company, located in St. Louis, Mo., USA, developed a unique sperm sorting
system that used 16 sorting nozzles instead of just one as in the case of the MoFlow SX™
cytometer. This equipment was intended to be commercialized, but, apparently, due to
problems with low conception percentages detected in its first tests, the company decided not
to commercialize it. In 2003, Genetic Resources International/Sexing Technologies in
Navazota TX, USA purchased the intellectual property and the sperm sexing equipment
developed by Monsanto, as well as the entire infrastructure of XY Inc. (the first company to
own the intellectual property of sperm sexing and the creator of the MoFlowTM
cytometers)(69). The company has since changed its name to STgenetics®(72).
The difference in fertility between conventional semen and sexed semen did not improve
with increasing sperm concentration by AI. The causes of lower fertility of sexed semen have
been attributed to the various biochemical changes that sperm undergo during sexing. The
XY technology described in previous publications(73,74) has been modified and is now a
totally new sexing system called SexedULTRA™ (Navazota, TX, USA). The
SexedULTRA™ technology has been designed to be more sperm-friendly during the most
critical points of the process, particularly improving pH changes (buffer system) and
oxidative stress.
Although there is currently very little data on this new technology, it has been reported that
it facilitates the entry of the Hoechst 33342 fluorochrome and retains it inside the cell,
allowing for greater fluorescence and thus better discrimination between "X" and "Y"
populations. The protocol was modified, with a pretreatment prior to the staining process, in
addition to the use of a new staining medium that maintains the pH stable for a longer period
of time. The freezing medium was also modified, taking into account the dose of sexed semen
per straw(72).
The success of the ultrasexing process was mainly influenced by two factors: modifications
in the means and equipment used to perform sexing. The MoFlo SX™ cytometers
(Cytomation Inc., Fort Collins, CO, USA) were very expensive, bulky, had low throughput
and required highly trained personnel to operate them. Modern Genesis cytometers
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developed by Cytonome ST™ (Boston, MA, USA) have advanced and automated electronic
features with multiple heads on one machine for parallel separation. The Genesis III™
cytometer uses a solid state laser, two orthogonal detectors (0° and 90° to the laser), an
orientation nozzle and a subpopulation separation of ~8000 spermatozoa/second with ~90%
purity, reaching a maximum separation rate of 500 million sperm per hour(75).
The aforementioned modifications brought about sperm motility and acrosome integrity were
increased with respect to the XY Legacy technology (conventional sexing) considering the
same sperm concentrations(76).
On the other hand, in 2018(77), sperm quality was evaluated considering plasma membrane
integrity, percentage of intact acrosomes and DNA fragmentation index of SexedULTRA™
semen compared to conventional (non-sexed) semen. In SexedULTRA™ semen at 3 h post-
thawing, the percentage of intact acrosomes was significantly higher than in conventional
semen. In addition, SexedULTRA™ semen had a significantly lower DNA fragmentation
index at all evaluation points compared to conventional semen. The authors conclude that
SexedULTRA™ technology maintains semen quality and, in many cases, has greater in vitro
longevity compared to conventional semen.
In the first field evaluation using SexedULTRA™ technology for AI(78,79), there was a 7.4 %
increase in heifer conception rates over XY Legacy technology (conventional sexing). The
second test was conducted in collaboration with the commercial company Select Sires, using
eight bulls from which semen was collected and processed using both SexedULTRA™
technology and XY Legacy technology, inseminating 6,930 heifers. The results showed that
SexedULTRA™ semen increased the conception rate 4.5 % over XY Legacy semen, 46.1
and 41.6 % respectively.
With these tests it was observed that the deleterious effects of the XY Legacy technology
were partially ameliorated with the new SexedULTRA™ technology, so the next logical step
was to increase the sperm concentration per dose, although in the past increasing sperm
concentration did not improve fertility. The following test was performed in collaboration
with German Genetics International: semen was collected from five bulls; each ejaculate was
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divided into 4 parts and processed with XY Legacy technology of 2.1 million sperm,
SexedULTRA™ of 2.1, 3 and 4 million sperm per dose. In addition, semen from these same
bulls was used from contemporary conventionally frozen ejaculates, with a concentration of
15 million spermatozoa per dose. Non-return to estrus rates (NRR) at 65 d were calculated
from 7,855 AI with sexed semen and 62,398 AI with conventional semen. Overall, the XY
Legacy semen of 2.1 million sperm per dose resulted in lower NRRs (55.9 %) compared to
all SexedULTRA™ treatments (2.1 million 59.9; 3.0 million 60.0 %; 4.0 million 66.7 %)
and conventional semen (65.7 %). SexedULTRA™ treatments of 2.1 and 3 million sperm
per dose were similar (59.9 and 60.0 % respectively), but lower than conventional semen
(65.66 %); however, the SexedULTRA™ treatment of 4 million sperm per dose had NRRs
similar to conventional semen of 15 million sperm per dose(79). The data obtained
demonstrated for the first time the effect of the response to the dose when using sexed semen.
The use of SexedULTRA-4M™ semen was evaluated in FTAI(80) using beef cows and
heifers. The results show that there was no significant difference in the percentage of
pregnancies between conventional semen (61.9 %) and SexedULTRA-4M™ semen (63.8 %)
when the females were in heat prior to FTAI.
There is little research on the effectiveness of the use of sexed semen in Mexico, although it
is already available from several semen processing companies and is routinely used,
especially in dairy production units. Experiments have used Legacy sexed semen and found
it to work for both Holstein cows and heifers, with a pregnancy rate between 80 to 90 % of
that recorded for females inseminated with conventional semen and with values of 85 to
93.6 % of offspring born with the predicted sex (82-85). It was also found that the use of sexed
semen does not influence the occurrence of miscarriages or dystocic births(86).
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Fertility is a multiparametric event related to semen quality and quantity, the exact timing
and method of AI, the intrinsic fertility of the bull and proper herd management(87).
Morphology, motility, viability, acrosome, and DNA concentration and integrity have been
used as parameters to evaluate the sperm quality of bovine semen(87-90). Some of these
parameters (such as morphology and motility) can be assessed manually by conventional
methods using a visible light microscope. However, these evaluations are subject to
subjective criteria and technical errors that diminish their accuracy and repeatability.
Motility is one of the most important sperm characteristics associated with the ability to
fertilize(92). With the use of the CASA system, various motility parameters describing specific
sperm movements are obtained. Total and progressive motility percentages are the most
important parameters in the evaluation of sperm kinetics(87). Total motility refers to the
fraction of spermatozoa that show any movement, whereas spermatozoa with progressive
motility have a forward movement, essentially in a straight line.
Other specific kinetic parameters determined by the CASA system are useful to evaluate
several sperm characteristics simultaneously and objectively. These kinetic parameters
consist mainly of three values of the speed of movement, three speed indices, and three
parameters that reflect the oscillation characteristics of the spermatozoa(93). The three values
of the velocity of motion are the curvilinear velocity (VCL), the rectilinear velocity (VSL)
and the mean trajectory velocity (VAP). From these three values, three indices are calculated,
linearity (LIN=VSL/VCL), straightness (STR=VSL/VAP) and trajectory oscillation
(VAP/VCL), thus characterizing the quality of sperm movement. The parameters that show
the oscillation characteristics of spermatozoa are the lateral displacement of the head, the
frequency of tail beating, and the mean angular displacement.
CASA system movement parameters have been used for the identification of sperm
subpopulations and their subsequent correlation with freezing resistance(94,95). In addition,
the effects of different media during in vitro processing on sperm function have evaluated(96).
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On the other hand, with the use of the CASA system, several groups have reported a
significant correlation between the total (r=0.26-0.61) and progressive (r=0.26-0.33) motility
of bull semen and its field-associated fertility(97-101). The CASA system collects a wide range
of sperm kinetics parameters. Some research groups showed a positive correlation between
VSL (r=0.17-0.67), LIN (r=0.28-0.46) and STR (r=0.33), and field fertility(98,102,103).
Correlations between motility parameters and fertility tend to be low to medium, and their
use in isolation to predict the fertility of a semen sample is not recommended(101-103).
However, the combination of several motility parameters provides a better tool for predicting
fertility, as the multi-parameter regression of the CASA system explained up to 0.98 (r2
value) of the variation in fertility, compared to 0.34 explained by total motility alone(103). On
the other hand, recent analyses of sperm movement in the third dimension and the study of
flagellar movement are new functional parameters that could be related to fertility(104).
Sperm morphology is one of the most important tests in semen quality control, as it reflects
the physiological or pathological state of the functionality of the testicles, epididymis and
accessory glands of the reproductive tract(105); is also considered a better test to evaluate
sperm DNA and genetic characteristics, compared to sperm motility(106,107). Several studies
have shown a significant correlation between sperm morphology (r=0.22-0.76) and field
fertility(94,98,108). However, most of the morphological analyses are performed through
conventional methods, which remains a problem due to the subjectivity in the evaluation, as
well as the inconsistency observed within and between technicians(109,110). For this reason,
morphological analysis has not been considered reliable in predicting field fertility(94, 98). The
development of specific modules for the morphological analysis of spermatozoa within the
CASA system has allowed the individual evaluation of morphometric characteristics of the
sperm head in terms of size (area, perimeter, length and width) and shape (ellipticity,
elongation, regularity and roughness)(111). Some systems even provide information about the
mid piece (area and width) and data concerning the insertion of the mid piece into the head,
such as distance and angle of insertion(112). Within these parameters, the width of the sperm
head showed a significant correlation (r=0.53) with field fertility(113). On the other hand,
sperm subpopulations have been reported based on their morphometric structure(114). The
evaluation of new parameters, as well as the identification of sperm subpopulations, could
provide information on an optimal fertility-enhancing population(90).
There are other parameters in the study of sperm function, such as vitality, acrosome
integrity, and DNA fragmentation. Viability classifies spermatozoa as alive or dead and
shows the existence of damage to the sperm plasma membrane(115). Acrosome integrity is
one of the most important sperm function tests, since only a spermatozoon with an intact
acrosome can penetrate the oocyte(116). In the case of sperm DNA integrity, its importance in
fertilization and in the early stages of embryonic development has been demonstrated, having
been recognized as a parameter indicative of sperm fertilization potential(117,118). Several
studies have shown a significant correlation between vitality (r=0.19-0.40), acrosome
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integrity (r=0.52) and DNA fragmentation (r=-0.49), and the field fertility of bulls(94,95,97,99).
In addition, when several parameters (sperm kinetics, vitality, DNA fragmentation and
morphology) were combined in regression models, the correlation with fertility increased to
more than 90%(12). Although most of these tests are performed through the use of flow
cytometry, new generations of CASA system modules have been developed for the automatic
assessment of vitality, acrosome integrity, and DNA fragmentation(92). However, few studies
have been conducted in cattle using these new modules. Therefore, motility and morphology
are shown to be the most important modules of the CASA system in terms of use.
These studies show the great potential of CASA systems for estimating semen quality,
studying sperm function, and predicting fertility. However, the parameters provided by the
CASA system have also been shown to have limitations and cannot be used in isolation as
reliable predictors of the fertilization ability of the sperm. In addition, spermatozoa are
complex cells that require a large number of criteria in order to be considered to achieve
fertilization(119). Therefore, the use of various parameters provided by the CASA system
within a regression model is presented as the best option to attempt to predict the fertility of
a semen sample. However, there is no consensus as to which parameters of sperm
functionality to use in the spermatozoa(99), perhaps due to the differences found between
working groups with respect to the parameters correlated with fertility.
Currently, sperm analysis through a CASA system is widely used within the quality control
protocols of semen processing centers, mainly the motility module. These protocols establish
thresholds for certain variables such as total and progressive motility; ejaculates below these
thresholds are usually discarded before or after freezing(99).
In Mexico, several associations, institutions and companies related to the livestock sector
utilize CASA systems on a regular basis mainly in the quality control of commercial doses
of bovine, ovine, and porcine semen. However, studies of post-cryopreservation sperm
kinetics of Pelibuey and Blackbelly rams(120), Mexican Pelon pigs(121) and Merino sheep from
Socorro Island(122), and evaluations of cryopreserved semen samples from Chiapas sheep(123)
and Tamaulipas Creole cattle(124) stored at the National Center for Genetic Resources of
INIFAP (CNRG-INIFAP) have also been carried out. On the other hand, CASA systems
have become more attractive as part of the practical evaluation of the sperm quality in semen
samples of many domestic species. However, there are multiple reasons why a semen
evaluation using a CASA system may vary, including system and equipment maintenance,
sample handling, and technician experience(89). For this reason, it is vitally important to
corroborate the effectiveness of the analysis. To ensure that the CASA system works
properly, validation of technicians, protocols and equipment is crucial. In this sense, the
CNRG-INIFAP has a test validated before the Mexican accreditation entity called
“Evaluation of semen from domestic animals”, which is carried out with a CASA system.
This allows semen evaluations to be performed with high quality standards(125).
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CASA systems have evolved in recent years to become powerful tools for rapid and objective
evaluation of sperm quality and function of bovine semen samples. CASA systems will
continue to be developed to perform new, repeatable and increasingly accurate tests in order
to contribute to fertility improvement in the field.
The first birth from embryo transfer in mammals was achieved in 1890 with rabbit
embryos(129), and the first successful surgical transfer in cattle was achieved in 1951(130). The
set of biotechnologies involving MOET developed between 1940 and 1960, laying the
foundation for the embryo transfer industry, which began in 1970 as a tool for the mass
introduction of continental European breeds to North America(131). The modern activity of
the MOET is the result of the efforts of two groups: a) scientists, who initially developed the
procedures and techniques of embryo transfer, and b) field veterinarians, who applied this
technology commercially, making it practical and available for the cattle industry, and later
for other productive species as well(131).
In the early 1970s, the first embryo transfer centers were established in North America,
including Alberta Livestock Transfer (Alberta, Canada), Modern Ova Trends (Ontario,
Canada), Colorado State University (Colorado, United States), Carnation Genetics
(California, United States), and Codding Embryological Science, Inc. (Oklahoma, United
States)(132). In our country, the first embryo transfers (ET) in cattle were performed in 1978
by North American technicians, but the results are unknown. In February 1979, the Embryo
Transfer Clinic was inaugurated in Ajuchitlán, Querétaro, as part of the National Center for
Animal Reproduction, under the National Institute for Artificial Insemination and Animal
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The Center for Genetic Improvement and Embryo Transplantation (CEMEGEN), which is
attached to the state-owned dairy company Leche Industrializada Conasupo (LICONSA),
began its activities in November 1986, producing embryos of the Holstein Friesian, Brown
Swiss, Jersey, Simmental, Simbrah, and F1 Holstein x Gyr dairy (Gyrholando) and Holstein
x Guzerat breeds. It was estimated that, by 1993, 20,000 embryos per year would be produced
from 2,200 donors. The center ceased operations in 1994; between 1987 and 1993 it produced
almost 42,000 embryos. In addition, 18 training courses in the technique were given to
approximately 300 professionals, and work was carried out for 23 Bachelor's and 4 Master's
degree theses. Most of the embryos produced were frozen and subsequently transferred to
different states of Mexico(134). In 1990, the National Center for Animal Reproduction became
part of the National Commission for Genetic Improvement and Animal Reproduction
(CONAMEGRA), established through an agreement between the Ministry and the National
Livestock Confederation (CNG). Several TE works were carried out for farmers in different
parts of the country, and an agreement was established with LICONSA for the
commercialization, between 1993 and 1994, of 1,343 embryos produced at CEMEGEN, at a
price of $100.00 per embryo ―an amount well below the cost of production. CONAMEGRA
sold this genetic material to 33 producers from 11 Mexican states, its own technicians thawed
447 embryos, transferred them, and obtained 51 % of pregnancies(135). In 1993, INIFAP
received a donation of 1,558 embryos from CEMEGEN; these were F1 and ¾ Holstein x
Zebu embryos, destined for the genetic programs of its experimental stations in the tropics.
That same year, 800 embryos and 300 head of cattle were donated to the College of
Posgraduates (Colegio de Posgraduados).
In 1994, LICONSA terminated the loan agreement with UNAM, auctioned the livestock,
dismissed and paid off its staff, and returned its facilities to UNAM, thus putting an end to
the operation of CEMEGEN(135).
The collection and transfer of embryos was initially a very complex process, since both the
collection of embryos from the donor and their subsequent transfer to recipient females was
done by surgical methods and using general anesthesia; this involved an enormous logistical
effort, as the donors and the recipients had to be prepared for surgery at the same time(132). In
the first instance, both donor and recipient surgeries were performed under local anesthesia;
subsequently, procedures for the non-surgical collection of embryos and their transfer to
recipients were developed, which facilitated the more widespread use of the technique(136).
The results obtained using non-surgical methods gradually approached those obtained with
surgical methods, which is why the latter fell into disuse(131).
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Regarding ovarian stimulation to induce multiovulation, there has always been a high
variability in the superovulatory response, despite efforts to control the sources of variation,
which is one of the main problems affecting the efficiency and profitability of MOET at the
commercial level(137). A study carried out with successive superovulations in zebu cows in
the "El Macho" experimental station, INIFAP, where the variables of time, FSH dose and
age were considered, concluded that the initial response of a zebu cow to superovulation
cannot be said to be a good predictor of subsequent responses by the same cow(138).
To date, there have been considerable advances in the study of ovarian physiology, as well
as factors inherent to the donor; however, there remain some aspects to be understood in
order to generate more efficient ovarian stimulation protocols(139).
In its beginnings, superovulation was induced with eCG; however, a few years later it was
discovered that crude pituitary extract (FSH with 20% LH) generated a better superovulatory
response than eCG(140). Pituitary extracts are now widely used; there is a high variability in
the amount of LH present in crude extracts, while purified extracts have less variation in the
amount of LH. Multiple studies have been conducted to evaluate in vivo embryo production
using crude and purified extracts(131). In a 1995 study conducted at CEMEGEN in Mexico,
the crude extract was found to produce more embryos than the purified extract in dairy
cattle(141). Conversely, in a study conducted in 2014 at INIFAP with beef cattle, the purified
extract generated more embryos than the crude extract(142); this may be due to the fact that
the hepatic metabolism of dairy cattle is more accelerated compared to that of beef cattle(143).
Despite many efforts to increase embryo production per cow per year by increasing ovarian
response to superovulatory treatment, little progress has been made(131). The use of PIDR in
combination with BE and prostaglandins has allowed the development of a protocol called
Rapid Donor Recycling. This protocol reduces the interval between superovulations by
almost half (33 to 35 d) with no decline in response, either in the number of embryos
produced or in their quality, in successive superovulations for up to one and a half
years(131,142). Thus, the production of transferable embryos per donor per year is nearly
doubled.
The first successful cryopreservation of embryos was reported in murines in 1972(144). One
year later, the first calf was born from a previously cryopreserved blastocyst using a 2M
dimethyl sulfoxide solution with a freezing and thawing rate of 0.2 °C/min and 36 °C/min,
respectively(145). The first calves born from cryopreserved embryos in Mexico came from
embryos frozen in Colorado, USA, and transferred to Nayarit, Mexico, into an experimental
station of INIFAP(146).
For more than 10 yr, glycerol was the cryoprotectant of choice for bovine embryo
cryopreservation. However, in 1992, a direct transfer cryopreservation system using ethylene
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glycol as cryoprotectant was announced. This had a rapid and positive effect worldwide on
the embryo transfer industry to the present day(131).
According to data from the American Embryo Transfer Association, in 2009, approximately
99 % of the beef bovine embryos and 94 % of the dairy bovine embryos were frozen in
ethylene glycol for direct transfer(131).
IVP biotechnology has a variety of applications in basic and applied science; in the first
instance, it has supported the production of embryos used for a wide variety of research,
including the treatment of infertility in humans. It is certainly a tool to increase the
productivity of farm animals by increasing the reproductive potential of animals of higher
genetic merit; in addition, it plays a relevant role in the conservation of the genetic resources
of animals, especially endangered ones(147).
Generically known as IVF (in vitro fertilization) or IVP (in vitro production), it is a
reproductive biotechnology, which, like MOET, is composed of several biotechnologies such
as: in vitro maturation of eggs, sperm capacitation, in vitro fertilization, and the culture of
zygotes and embryos up to pre-eclosion stages (7 to 8 d post-fertilization)(148). IVP consists
of retrieving eggs or oocytes from ovarian follicles to be matured and fertilized under
laboratory conditions; the resulting zygotes are cultured until post-compaction stages (morula
or blastocyst), at which time they are transferred to a recipient cow or cryopreserved for
subsequent transfer. Oocytes can be drawn from trace ovaries or live animals, by means of
ultrasound-guided transvaginal aspiration (TVA)(148).
This biotechnology dates back to the 1970s, thanks to which research and achievements in
the areas of culture media development, oocyte maturation, sperm capacitation and
fertilization (which occurred in that decade and the following one(126)) led to the birth, in
1987, of the first calf produced entirely in vitro(149). Although this biotechnology was initially
oriented primarily to research and was based on tests carried out on ovaries obtained at the
slaughterhouse, with the incorporation of TVA (making it possible to obtain immature
oocytes from living donors), the commercial application was seen as a more promising tool
than MOET for the mass production of offspring from progenitors of high genetic merit. The
above is confirmed by observing that, worldwide, while the number of embryos collected in
vivo and transferred has remained stable in recent years, the number of transferred IVF
embryos has had an average annual growth rate of 12 % and, for the first time, in 2017, the
number of viable embryos produced in vitro, exceeded the number of transferable embryos
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collected in vivo(150); that trend has continued as of the 2019 International Embryo
Technology Society (IETS) report, with data from 2018(151). In this same report, it is noted
that the vast majority of viable IVF embryos were obtained from oocytes collected through
TVA (98.9 %), in contrast to the few embryos obtained from trace ovaries(151). The reason
for this is the uncertainty of obtaining germplasm suitable for commercial production from
the genetic and sanitary point of view. It is known that there are a significant number of
research laboratories where viable IVP embryos are produced and discarded once they have
fulfilled their function; however, this datum is not recorded by the IETS statistics
committee(152).
Globally, there are two events that have been driving forces in IVP: sexed semen
biotechnology and genomic evaluations. The first is that thanks to IVP it is possible to
maximize the use of sexed semen by fertilizing a large number of oocytes (100+) with a
single dose of semen, and the second is that it makes it possible to intensify the power of
selection by shortening generation intervals (TVA in calves, enabling the use of their
germplasm before the age of service) and increasing the reproductive capacity on the
maternal side. Thus, these three biotechnologies (IVP, sexed semen, genomic evaluations)
play a relevant role in genetic improvement and the cattle industry in general(152).
IVP had a period of great growth at the beginning of this century, especially in Brazil, where,
in 2009, 85 % of the available embryos came from in vitro production; this amount was
equivalent to 50 % of the worldwide production. The success of the Brazilian companies
encouraged their expansion to other Latin American countries, including Mexico, where they
settled, working independently or in partnership with Mexican companies or producer
organizations. It has not been possible to replicate what has been achieved in Brazil in
Mexico because this country does not have the competitive advantages that Brazil has
(breeds, demand, size of production units, availability of receivers)(148). Nevertheless, there
continues to be moderate activity by these and other domestic companies; thus, in 2018, the
transfer of almost 28,000 embryos was reported in Mexico, almost all from IVP, and, in
contrast, only over 4,000 embryos obtained in vivo were transferred(151).
Although a considerable amount of research has been generated regarding the main
components of this biotechnology (development of sequential culture media, control of
potentially toxic agents, exclusion of serum components, inclusion of amino acids, vitamins,
chelating agents and hormones, among others)(153-156), and so has research in oocyte
maturation and in vitro fertilization processes(152-157), the fact is that it has not been possible
to exceed the limit of 40 to 50 % of blastocysts obtained from fertilized oocytes, a value not
very different from the 30 to 40 % that existed 20 yr ago. This has drawn attention to the lack
of homogeneity in the oocyte source as the most likely cause of limited IVP success
rates(155,157,158). It is therefore imperative to continue to promote IVP-IVT (in combination
with other biotechnologies such as the use of sexed semen and genomic evaluations) as a
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valuable productive tool, and also to continue to conduct research for IVP in larger quantities
with respect to the eggs left to mature, which achieve a better post-transfer development and
have greater tolerance to cryopreservation.
Due to the complexity and high requirements of infrastructure and equipment, as well as
personnel trained in this biotechnology, IVP research in Mexico has been incipient. Only a
handful of universities ―namely, Universidad Nacional Autónoma de México, Universidad
Autónoma Metropolitana, Universidad Veracruzana, Universidad Autónoma de Nuevo
León, Universidad Autónoma de Tamaulipas, Colegio de Posgraduados, and Universidad
Autónoma de Chihuahua―, some producer organizations and livestock companies, and
INIFAP have worked on certain IVP research topics. The following are some of the results
obtained in research conducted in Mexico on topics related to bovine IVP: in relation to
agents and culture conditions to reduce the production of reactive oxygen species (ROS) in
the culture medium, in a study conducted at INIFAP, it was found that by reducing the O2
tension to 2 %, the number of cells in the blastocysts increased and the production of ROS
was reduced(159). In another study also carried out at INIFAP, pterostilbene, a phytoalexin,
was used as an antioxidant agent at a concentration of 0.33 μM, and it was found to reduce
the production of ROS and the occurrence of intracytoplasmic lipids in 7-d-old embryos(160).
The latter is presented as an alternative for improving IVP embryo cryopreservation. In a
collaborative work between INIFAP and UANL, the effect of the addition of a heat shock
protein (HSP70) on the development of bovine embryos produced in vitro was evaluated,
and the addition of HSP70 to the culture media was found to have favorable effects on the
percentage of blastocysts and cell number(161). A system for individual embryo culture called
"WOW" was also evaluated at INIFAP, and, although it produces a similar number of
embryos compared to group culture in microdroplets, the WOW system was found to produce
a higher percentage of embryos with a better morphological quality(162). In another study
carried out at UNAM, the effectiveness of two vitrification devices for cryopreserving bovine
embryos was compared. Cryotop® was found to be a more effective vitrification support
than Open Pulled Straw®, resulting in higher post-vitrification viability(163). Another study
carried out between the Colegio de Posgraduados and the Universidad Veracruzana tested
the alternative of utilizing the culture media used in the human IVF system to cultivate bovine
embryos and found that it is possible to produce blastocysts with similar results(164). It should
be noted that the culture media used in humans are often more readily available on the
domestic market. Yet another study, carried out at the Autonomous University of Chihuahua,
proved that the addition of IGF-I at different times during the IVP process did not produce a
beneficial effect on the percentage of blastocysts(165).
The future of IVP in cattle faces important challenges that must be resolved in order to ensure
its usefulness as a productive tool, as well as support for research in multiple areas of
knowledge. The evolution of culture media to provide near-physiological conditions for
gametes and embryos has been one of the areas with the greatest progress(152), despite which,
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difficulties are still encountered today in producing similar embryos to those obtained in vivo,
resulting in low pregnancy rates at transfer, low tolerance to cryopreservation and alterations
in fetal and placental development(157). Research efforts have focused on the development of
chemically defined culture media(166), use of oxidation level regulating compounds(167), use
of delipidating compounds or lipid metabolism regulators(160,168), and mechanisms such as
the use of sequential media to remove the presence of molecules that are toxic to the
embryo(169), as well as on the development of cryopreservation methods that are friendlier to
the embryo produced in vitro, such as vitrification(170). On the other hand, with the
development of biotechnologies such as embryonic nuclear transplantation (16-cell stage
blastomers) and somatic transplantation (cumulus cells, fibroblasts, etc.)(171), an important
future was foreseen for the genetic modification of embryos for productive, medical and
research purposes (gene function studies, xenotransplantation, recombinant protein
production, genetic improvement, and food production)(172) and their eventual cloning.
However, despite some encouraging results, the random insertion of the transgenes generated
highly variable and unpredictable results, rendering the use of this technology unviable(173).
Today, with the advent of gene editing technologies (CRISPR - Cas - 9), it is already possible
to perform precise gene editing, including epigenetic reprogramming, which augurs a golden
age in the genetic modification of farm animals for the aforementioned purposes, with the
strong support of IVP biotechnologies(174). There will still be ethical impediments and legal
pitfalls to be resolved.
Conclusions
As a final reflection, it can be said that, although research institutions in Mexico, and
especially INIP-INIFAP, have accompanied the development of reproductive
biotechnologies in the world in the last five decades. With the passage of the years, these
have evolved meteorically, and it has been increasingly difficult to maintain a solid research
base that allows us to be aligned with the technological developments that are taking place.
Although the information generated by Mexican institutions on current topics such as in vitro
embryo production is modest, the national livestock industry is demanding immersion in
these technologies. This should encourage research institutions to generate technological
components that will allow the efficient use of this and other technologies under local
conditions.
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