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From the Department of Medicine and Animal Surgery, Faculty of Veterinary Medicine, University of Murcia, Murcia, Spain.
| Correspondence to: Dr Jordi Roca, Department of Medicine and Animal Surgery, Faculty of Veterinary Medicine, Campus de Espinardo, University of Murcia, E-30071 Murcia, Spain (e-mail: roca{at}um.es). |
| Received for publication November 10, 2003; accepted for publication January 6, 2004. |
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Abstract |
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Key words: Antioxidants, cryopreservation, sperm, porcine
Various circumstances are associated with the low fertility of frozen-thawed boar spermatozoa after AI (for recent reviews, see Holt, 2000; Watson, 2000), which include the damage that the spermatozoa undergo during the freeze-thaw process, which lowers their fertilizing capacity. The success of preservation by freezing depends on the susceptibility of sperm cells to low temperature, since boar spermatozoa are especially susceptible to cold shock (White, 1993). This problem is related to the lipid composition of the membrane, because membranes of boar spermatozoa have a relatively high proportion of polyunsaturated fatty acids, which decreases significantly during the cryopreservation process, indicating lipid peroxidation (Cerolini et al, 2001). Lipid peroxidation has been correlated to exposure of spermatozoa to reactive oxygen species (ROS). It has been demonstrated that spermatozoa that undergo freeze-thaw cycles produce ROS (Alvarez and Storey, 1992). Moreover, excessive ROS formation by spermatozoa during the cryopreservation process has been associated with a decrease in the function of thawed spermatozoa (Chatterjee and Gagnon, 2001). One way to overcome the detrimental effects of ROS on subsequent sperm performance after thawing could be to add antioxidant compounds to the freezing extender to block or prevent oxidative stress.
A variety of antioxidants have been tested to either scavenge ROS directly or counter the effects of ROS toxicity in the semen of a variety of mammalian and avian species. Among them, butylated hydroxytoluene (BHT), a synthetic phenolic antioxidant, has been widely used as a food additive (Williams et al, 1999). BHT has been tested with varying degrees of success to either preserve liquid spermatozoa in the turkey tom (Donoghue and Donoghue, 1997) and stallion (Ball et al, 2001) or minimize cold shock damage in bull (Hammerstedt et al, 1976) and ram spermatozoa (Watson and Anderson, 1983). BHT has also been successfully tested to minimize cold shock damage in boar spermatozoa (Pursell, 1979; Bamba and Cran, 1992). In spite of these promising results, the use of BHT in freezing extenders is not commonplace, and no results are available that evaluate the potential effect of BHT on frozen-thawed boar spermatozoa. The goal of the present study was to evaluate the potential protective effect of BHT on cryopreservation injuries to boar spermatozoa. Postthaw sperm survival and their ability to produce embryos in vitro that develop to the blastocyst stage were the criteria used to assess the potential protective effect of BHT.
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Materials and Methods |
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-cm, Elgastat UHQPS; Elga Ltd, Wycombe United Kingdom). The basic medium used for sperm dilution was Beltsville thawing solution (BTS) composed of 205 mM glucose, 20.39 mM NaCl, 5.4 mM KCl, 15.01 mM NaHCO3, and 3.35 mM EDTA (Johnson et al, 1988) containing kanamycin sulfate (50 µg/mL). The basic medium used for sperm cryopreservation was a lactose-egg yolk (LEY) extender composed of 80% (vol/vol) ß-lactose solution (310 mM in water), 20% (vol/vol) egg yolk, and 100 µg/mL kanamycin sulfate. The medium used for the collection and washing of oocyte–cumulus complexes was Dulbecco Phosphate-Buffered Saline (DPBS) medium composed of 136.89 mM NaCl, 2.68 mM KCl, 8.1 mM Na2HPO4, and 1.46 mM CaCl2-2H2O. The oocyte maturation medium was the bovine serum albumin (BSA)-free North Carolina State University-23 composed of 108.73 mM NaCl, 4.78 mM KCl, 1.7 mM CaCl2-2H2O, 1.19 mM KH2PO4, 1.19 mM MgSO4-7H2O, 25.07 mM NaHCO3, 5.55 mM D-glucose, 1 mM L-glutamine, 7 mM taurine, 5 mM hypotaurine, 75 µg/mL potassium penicillin G, and 50 µg/mL streptomycin sulfate (NCSU-23) (Petters and Wells, 1993) that was supplemented with 10% (vol/vol) porcine follicular fluid, 0.1 mg/mL cysteine, 10 ng/mL epidermal growth factor, 10 IU/mL equine chorionic gonadotropin (Folligon, Intervet International B.V., Boxmeer, the Netherlands), and 10 IU/mL human chorionic gonadotropin (Chorulon, Intervet). The fertilization medium was a modified Tris-buffered medium composed of 20 mM Tris (Trizma base), 113.1 mM NaCl, 3 mM KCl, 7.5 mM CaCl2-2H2O, 11 mM D-glucose, and 5 mM sodium pyruvate (TBM) (Abeydeera and Day, 1997) that was supplemented with 2 mM caffeine and 0.2% BSA (fraction V; A-7888, initial fractionation by cold alcohol precipitation). The embryo culture medium was NCSU-23 with 0.4% BSA.
Stock solutions of BHT were prepared in absolute ethanol and dried down under air in tubes before the addition of the medium. When medium was added to each tube, the content was mixed on a Vortex mixer (VELP Scientifica, Milano, Italy). The BHT stock solution was made up fresh each experimental day.
Semen Processing and Sperm Cryopreservation
Ejaculate sperm samples were collected from 3 Pietrain boars on a weekly
basis. Sperm-rich ejaculate fractions were obtained using the gloved-hand
method and extended (1:1 [vol/vol]) in BTS. After collection, semen
characteristics (total sperm numbers per ejaculate, subjective sperm motility,
acrosome integrity, and normal morphology) were microscopically evaluated,
using standard laboratory techniques
(Martin Rillo et al, 1996),
and only ejaculate sperm samples with more than 75% motile spermatozoa and
more than 80% normal acrosomes were used.
Spermatozoa were cryopreserved using the straw-freezing procedure described by Westendorf et al (1975) as modified by Thurston et al (1999). Briefly, diluted semen samples (1:1 [vol/vol] in BTS) were cooled to 17°C for 3 hours. After centrifugation at 800 x g for 10 minutes (Megafuge 1.0 R; Heraeus, Germany), the pellets were diluted in LEY (pH 6.2 and 330 ± 5 mOsm/kg) to a concentration of 1500 x 106 cells/mL. After further cooling to 5°C in 90 minutes, diluted spermatozoa were resuspended with LEY-glycerol-Orvus ES Paste (LEYGO) extender (92.5% LEY + 1.5% Equex STM [Nova Chemical Sales Inc, Scituate, Mass] and 6% glycerol [vol/vol]; pH 6.2 and 1650 ± 15 mOsm/kg) to a final concentration of 1000 x 106/mL. The resuspended and cooled spermatozoa were packed into 0.5 polyvinyl chloride-French straws (Minitüb, Tiefenbach, Germany), which were frozen using a controlled-rate freezer (IceCube 1810, Minitüb) as follows: cooled to –5°C at 6°C/min, from –5°C to –80°C at 40°C/min, held for 30 seconds at –80°C, and then cooled at 70°C/min to –150°C and plunged into liquid nitrogen.
Thawing and Postthaw Sperm Survival Evaluation
Thawing was carried out in a circulating water bath at 37°C for 20
seconds. Thawed spermatozoa from 2 straws were extended at 37°C with BTS
(1:2 [vol/vol]) and incubated in a water bath for 150 minutes. Sperm were
assessed for motility and motion characteristics, plasma membrane integrity,
acrosome integrity, and early apoptosis.
Sperm motility and motion characteristics were objectively evaluated using a computer-aided sperm analysis (CASA) system (Sperm Class Analyzer [SCA], Microptic, Barcelona, Spain) and a Makler counting chamber (Sefi Medical Instruments, Haifa, Israel). Diluted, thawed spermatozoa were rediluted in BTS to a concentration of 20 x 106/mL. For each evaluation, a 4-µL sperm sample was placed in a Makler counting chamber at 39°C, and 3 fields were analyzed to assess a minimum of 100 spermatozoa. The proportion of total motile spermatozoa (% TMS) and rapid progressive motility spermatozoa (% RPMS, >50 µm/s), straightline velocity (VSL, µm/s), curvilinear velocity (VCL, µm/s), average path velocity (VAP, µm/s), linearity (% LIN, ratio of VSL/VCL), straightness of the average path (% STR, ratio of VSL/VAP), amplitude of lateral head displacement (ALH, µm), and dance (DNC, VCL x ALHmed, µm2/s) were determined.
Plasma membrane integrity was evaluated using the fluorescent probes SYBR-14 (SY) and propidium iodide (PI) according to the manufacturer's instructions (L-7011, Live/Dead Sperm Viability Kit; Molecular Probes Europe, Leiden, the Netherlands). Briefly, 100 µL of thawed spermatozoa (30 x 106 cells/mL in HEPES buffer) was diluted with 25 nM SYBR-14 solution and 12 µM of PI solution. Samples were incubated at room temperature in the dark for 10 minutes before flow cytometric analysis (Garner and Johnson, 1995). Spermatozoa were allocated to "intact membrane," "dying," and "dead" classifications if they exhibited SY+/PI–, SY+/PI+, and SY–/PI+ staining, respectively.
Acrosome status was assessed by fluorescein isothiocyanate conjugated with peanut agglutinin (FITC-PNA) and PI staining as described by Nagy et al (2003), with slight modifications. Briefly, 100 µL of thawed spermatozoa (30 x 106 cells/mL in HEPES buffer) was diluted with 10 µL of FITC-PNA solution (1 µg/mL in bidistilled water) and 12 µM of PI solution. Samples were incubated at room temperature in the dark for 5 minutes before flow cytometric analysis. Spermatozoa were allocated to "live with intact acrosome," "live with damaged acrosome," "dead with intact acrosome," and "dead with damaged acrosome" classifications if they exhibited PNA–/PI–, PNA+/PI–, PNA–/PI+, and PNA+/PI+ staining, respectively.
Early apoptosis was detected using Annexin V conjugated with FITC (A-FITC; Annexin V-FITC Apoptosis Detection Kit) as described by Peña et al (2003a). Briefly, 100 µL of thawed spermatozoa (30 x 106 cells/mL in HEPES buffer) was diluted with 5 µL of Annexin V-FITC solution and 10 µM of PI solution. Samples were incubated at room temperature in the dark for 15 minutes before flow cytometric analysis. Spermatozoa were allocated to "live," "early apoptotic," "late apoptotic," and "dead" classifications if they exhibited A–/PI–, A+/PI–, A+/PI+, and A–/PI+ staining, respectively.
Immediately prior to analysis by flow cytometry, stained sperm samples from the 3 fluorescent probes were rediluted to 6 x 106 cells/mL in HEPES buffer. Analyses were carried out on a Becton Dickinson FACSort flow cytometer (San Jose, Calif) equipped with an argon-ion laser (488 nm, 15 mW). The green fluorescence (FITC) was measured using a 530/30-nm bandpass filter, and the red fluorescence (PI) was measured using a 650-nm LP filter, except in the plasma membrane integrity assessment, where a 585/30-bandpass filter was used. Debris was gated out on the basis of the forward scatter and side scatter dot plot by drawing a region enclosing the cell population of interest. In addition, events with scatter characteristics similar to sperm cells but without reasonable DNA content (very weak SYBR-14 or PI staining) were gated out. Subpopulations were divided by quadrants, and the frequency of each subpopulation was quantified. A minimum of 10 000 spermatozoa were collected and analyzed at a flow rate of approximately 800 cells/s.
Measurement of Membrane Lipid Peroxidation
Membrane lipid peroxidation was estimated by the end point generation of
malondialdehyde (MDA) determined by the thiobarbituric acid (TBA) test
(Esterbauer and Cheeseman,
1990). Briefly, diluted spermatozoa (250 x 106
cells in 1 mL) were mixed with 1 mL of cold 20% (wt/vol) trichloroacetic acid
to precipitate protein. The precipitate was pelleted by centrifugation (1500
x g for 10 minutes), and 1 mL of the supernatant was incubated
with 1 mL of 0.67% (wt/vol) TBA in a boiling water bath at 100°C for 10
minutes. After cooling, the absorbance was determined by a spectrophotometer
(UNICAM PU 8610 Kinetics spectrophotometer; Philips, Eindhoven, Holland) at
534 nm. The results were expressed as a simple concentration of MDA
(pmol/108 cells).
In Vitro Oocyte Maturation, Fertilization, and Embryo Culture
Ovaries were obtained from prepubertal gilts at a local slaughterhouse and
transported to the laboratory in 0.9% NaCl containing 75 µg/mL potassium
penicillin G and 50 µg/mL streptomycin sulfate maintained at
25°C–30°C. Oocytes were aspirated from medium-sized follicles
(3–6 mm in diameter) with an 18-gauge needle fixed to a 10-mL disposable
syringe. Oocytes surrounded by a compact cumulus mass and having evenly
granulated cytoplasm were washed 3 times in maturation medium, and 45–50
oocytes were transferred into each well of a Nunc 4-well multidish containing
500 µL of preequilibrated maturation medium previously covered with warm
mineral oil and cultured for 22 hours with added hormones and then for another
22 hours without hormones in 5% CO2 in air at 39°C. After the
completion of in vitro maturation, cumulus cells were removed with 0.1%
hyaluronidase in NCSU-23 and washed 3 times with fertilization medium. After
washing, batches of 30 oocytes were placed in 50-µL drops of the same
medium in a 35-x 10-mm petri dish. The dishes were kept in the incubator
for about 30 minutes until spermatozoa were added for fertilization. One
hundred microliters of diluted, thawed spermatozoa from 1 pool of 3 straws was
washed 3 times by centrifugation at 1900 x g for 3 minutes in
DPBS medium supplemented with 0.1% BSA, 75 µg/mL potassium penicillin G,
and 50 µg/mL streptomycin sulfate (pH 7.2). At the end of the washing
procedure, the sperm pellet was resuspended in fertilization medium; then, 50
µL of this sperm suspension was added to the medium that contained oocytes
so that each oocyte was exposed to 2000 sperm cells
(Gil et al, 2003). Six hours
after insemination, the oocytes were washed and transferred (30 oocytes per
well) to a Nunc 4-well multidish containing 500 µL of embryo culture
medium; they were then covered with mineral oil and cultured at 39°C, 5%
CO2 in air, for 7 days. At 48 and 168 hours of culture, cleavage
rate and blastocyst formation, respectively, were evaluated under a
stereomicroscope.
Experimental Design
Experiment 1: Determination of the Lowest Effective BHT Concentration to Reduce Lipid Peroxidation—
The goal of this experiment was to determine the lowest BHT concentrations
able to reduce lipid peroxidation in boar spermatozoa. Sperm-rich ejaculate
fractions from 3 boars were pooled immediately after collection. The pooled
semen samples were split into 10 aliquots and diluted in phosphate buffer to
250 x 106 spermatozoa/mL. One aliquot was used as a negative
control, and 9 aliquots were subjected to incubation for 30 minutes at
37°C with the following final concentrations of BHT (B-1378): 0 (as a
positive control), 0.025, 0.05, 0.1, 0.2, 0.4, 0.8, 1.6, and 3.2 mM. After
incubation, these 9 aliquots were subjected to in vitro–induced lipid
peroxidation. To induce lipid peroxidation, diluted spermatozoa were incubated
for 60 minutes at 37°C with 0.5 mM sodium ascorbate and 0.05 mM ferrous
sulfate (Brzezinska-Slebodzinska et al,
1995). After incubation, MDA concentration was evaluated.
Experiment 2: Effect of BHT Supplementation on Postthaw Sperm Function— In this experiment, the effect that BHT had on sperm function was evaluated by adding various ion concentrations of BHT to the freezing extender. After the centrifugation step during the cryopreservation process, the supernatant was removed, and the sperm pellet was split into 5 aliquots. Each aliquot was extended with LEY and LEYGO supplemented with BHT at the final concentrations of 0 (as control), 0.2, 0.4, 0.8, and 1.6 mM. Extended aliquots were cryopreserved according the protocol described above.
After thawing, assessments were made of sperm survival, membrane lipid peroxidation, and the ability of spermatozoa to fertilize in vitro–matured oocytes and for embryos to develop to the blastocyst stage using the procedures previously described. Sperm survival was assessed 30 and 150 minutes after thawing, and the MDA concentration (as an indicator of lipid peroxidation) was determined 0, 30, and 150 minutes after thawing.
Statistical Analyses
All of the data editing and statistical analyses were performed by SPSS,
version 11.5 (SPSS Inc, Chicago, Ill). Data from 6 replicates in each
experiment were analyzed by analysis of variance using the MIXED procedure
according to a statistical model, including the fixed effect of concentration
of BHT and the random effect of semen pool. In experiment 2, data of the
postthaw incubation times (30 and 150 minutes for sperm survival and 0, 30,
and 150 minutes for MDA production) were combined and analyzed as a complete
data set. Percentages of postthaw sperm survival were subjected to an arcsine
transformation before analysis. Embryo development data are presented in
accordance with the binomial model of parameters as described by Fisz
(1980) before analysis. When
analysis of variance showed a significant effect, values were compared using
the Bonferroni test and were considered significant when P < .05.
Results are presented as means ± standard error of the mean.
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Results |
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Experiment 2: Effect of BHT Supplementation on Postthaw Sperm Function
The effect of the presence of BHT in the freezing extender on postthaw
sperm motility parameters is shown in Table
1. The percentages of TMS and RPMS were significantly (P
< .05) higher in spermatozoa frozen in the presence of 0.2–0.8 mM BHT
than in the control. However, BHT had no influence on the other motility
parameters (VSL, VCL, VAP, LIN, STR, ALH, and DNC).
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Table 2 shows the results of plasma membrane integrity and acrosome integrity tests carried out in thawed spermatozoa. The percentages of spermatozoa classified as membrane intact (SY+/PI–) and live with intact acrosome (PNA–/PI–) were significantly (P < .05) higher in the samples cryopreserved in the presence of BHT at concentrations ranging from 0.2 to 0.8 mM than in its absence.
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The percentages of thawed spermatozoa in the 4 categories identified using the A/PI tests are presented in Table 3. The percentage of spermatozoa classified as live (A–/PI–) was significantly (P < .05) higher in the samples cryopreserved in the presence of BHT at concentrations ranging from 0.2 to 0.8 mM, than in the control. The percentages of apoptotic sperm (A+/PI– and A+/PI+) were not affected (P > .05) by the presence of BHT in the freezing extender.
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Figure 2 displays the production of MDA by thawed spermatozoa. The presence of BHT in the freezing extender significantly decreased (P < .05) the MDA concentration in thawed semen, irrespective of the concentration of BHT.
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The results of in vitro embryo development are summarized in Figure 3. BHT in the freezing extender did not improve (P > .05) the cleavage rates of oocytes. However, a higher proportion of oocytes reached the blastocyst stage (P < .05) when in vitro–matured oocytes were fertilized with thawed spermatozoa cryopreserved in the presence of 0.4 mM BHT compared to the control (28.8% vs 15.8%).
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Discussion |
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The concept that BHT might be beneficial to mammalian and avian sperm
preservation, when it is added to semen extenders, has been previously tested.
However, adding BHT to stored semen has shown mixed results with respect to
improving the survival of spermatozoa. Whereas BHT improved sperm survival in
cold-stressed (Graham and Hammerstedt,
1992) or cryopreserved
(Killian et al, 1989) bull
spermatozoa and chilled turkey tom semen
(Donoghue and Donoghue, 1997), it had a detrimental effect on cooled stallion spermatozoa
(Ball et al, 2001). These
results suggest that considerable difficulties still exist with regard to
species differences and technical abilities when using BHT to preserve sperm
motility and viability. In relation to boar semen, our findings, as well as
those previously reported (Pursel,
1979; Bamba and Cran,
1992), demonstrate that the presence of BHT in the extender
protects boar spermatozoa from damage caused by cryopreservation or cold
shock. Moreover, our results indicate that the addition of BHT at
concentrations ranging from 0.2 to 0.8 mM improves the motility, plasma
membrane integrity, and acrosome integrity of thawed spermatozoa. Because BHT
has the ability to incorporate into sperm membranes and prevent the damaging
activities of the lipid peroxyl radical, the resulting effectiveness of BHT
suggests that boar spermatozoa subjected to chilled storage or
cryopreservation are particularly susceptible to oxidative attack of lipid
peroxyl radicals. This explanation is supported by previous studies in which
-tocopherol, another powerful scavenger for lipid peroxyl radicals
(Kotamraju et al, 2001), improved survival of chilled (Cerolini et
al, 2000) and cryopreserved
(Peña et al, 2003b)
boar spermatozoa. Moreover, lipid peroxyl radicals have been shown to initiate
lipid peroxidation specifically in boar sperm membranes
(Comaschi et al, 1989).
The potential effect of BHT to protect spermatozoa from stress induced by cold or frozen storage may also vary widely with the concentration used. The results of experiment 1 indicate that all doses of BHT examined (ranging from 0.025 to 3.2 mM) were effective in the reduction of in vitro–induced lipid peroxidation. This finding is in agreement with those achieved in human spermatozoa by Aitken and Clarkson (1988), who demonstrated the effectiveness of BHT in the suppression of lipid peroxidation at concentrations ranging from 0.1 to 10 mM. However, these researchers reported that the highest concentrations of BHT had a toxic effect on spermatozoa, both inducing loss of motility and affecting their capacity to fuse with oocytes. The controlled generation of ROS in spermatozoa is associated with some normal physiologic functions such as sperm hyperactivation, capacitation, and acrosome reaction (Aitken, 1995). An excessive addition of antioxidant substances to the semen extender can neutralize the oxidative stress induced by an excessive ROS formation, but it can also stop the normal sperm functions associated with ROS. Therefore, it is important to select the appropriate antioxidant concentrations to maintain the natural balance that exists between ROS generation and scavenging activities. At the BHT concentrations tested in the second experiment (ranging from 0.2 to 1.6 mM), there were no deleterious effects on any of the functional parameters of thawed sperm. On the contrary, when the concentrations ranged from 0.2 to 0.8 mM, the postthaw sperm survival improved. Similarly, the improvement of sperm survival observed by Pursel (1979) and Bamba and Cran (1992) in boar spermatozoa undergoing cold shock was achieved at BHT concentrations ranging from 0.05 to 2 mM. Nevertheless, at the highest concentration evaluated (1.6 mM) in the present study, BHT had no protective effect on boar spermatozoa. Likewise, Bamba and Cran (1992) observed a loss of the protective effect of BHT against the cold stress of spermatozoa when the concentrations used were more than 2 mM. It seems, therefore, that the addition of BHT to semen extenders has beneficial or detrimental effects on postthaw sperm survival depending on the concentration used, with the maximum concentration required for effectiveness being between 1 and 2 mM.
The interaction between extender components and antioxidants is another important factor to consider when evaluating the effectiveness of any antioxidant in the protection of spermatozoa from either cold shock or freeze-thaw stress. In this way, it has been reported that catalase supplementation prolongs survival of bull spermatozoa in yolk extenders but not in skim milk extenders (Foote, 1962). For frozen boar spermatozoa in the present study, we used an extender containing 20% egg yolk. The effectiveness of BHT for improving both the survival and fertility of thawed spermatozoa may be related, in part, to the cooperative interaction between BHT and egg yolk. In this respect, Graham and Hammerstedt (1992) reported that BHT analogs in diluents with no egg yolk resulted in reduced sperm motility compared with the presence of egg yolk, suggesting that egg yolk interacted synergistically with BHT analogs to protect spermatozoa from cold shock.
Recently, it was proposed that lipid peroxyl radicals induce an apoptotic signaling cascade in endothelial cells (Kotamraju et al, 2001). Moreover, it is claimed that apoptosis occurs as a result of cryodamage in mammalian cells (Baust, 2002). Likewise, BHT inhibited caspase-3 activation, an enzyme that is considered a committed step in several apoptotic pathways (Kotamraju et al, 2001). In the present study, sperm apoptosis was investigated using the Annexin V assay. The Annexin V and PI stain combinations are able to identify early and late apoptosis in thawed boar spermatozoa (Peña et al, 2003a). As shown in Table 3, the presence of BHT in the freezing extender did not reduce the percentage of either early or late apoptotic cells in thawed spermatozoa. It may be that caspase-3 does not play an important role in sperm apoptotic mechanisms or that there is no relationship between ROS and apoptosis in boar sperm. Further studies are needed to address these questions.
It is well established that cryopreservation induces lipid peroxidation in mammalian spermatozoa. Alvarez and Storey (1992) demonstrated that the freeze-thaw process enhanced peroxidation of human sperm membrane lipids. Likewise, Chantterjee and Gagnon (2001) showed how cooling and thawing processes caused an increase of lipid peroxidation in bovine spermatozoa. Until the present study, no data were available on the effect of cryopreservation on lipid peroxidation in boar spermatozoa. Lipid peroxides, derived from peroxidation of polyunsaturated fatty acids, are unstable and decompose to form a complex series of compounds. These include reactive carbonyl compounds, of which the most abundant is MDA. Therefore, measurement of MDA is widely used as an indicator of lipid peroxidation in a variety of cell types, including spermatozoa (Sikka, 1996). In the present study, MDA production was used to determine the peroxidation levels of thawed spermatozoa. We showed that the presence of BHT in the freezing extender reduced MDA production in thawed spermatozoa. Since it has been demonstrated that lipid peroxyl radicals are one of the most important of the ROS involved in MDA production in boar spermatozoa (Comaschi et al, 1989), our results corroborate the hypothesis that lipid peroxyl radicals could be one of the most important ROS implicated in cryodamage to boar spermatozoa.
The investigation of in vitro fertilization and embryo development demonstrated that BHT at a concentration of 0.4 mM in the freezing extender boosted the ability of embryos derived from thawed boar spermatozoa to develop to the blastocyst stage. A possible explanation for our results is that BHT had an additional protective effect on cryopreserved spermatozoa to prevent the loss of DNA integrity. Besides membrane damage and impairment of motility, lipid peroxidation can damage the DNA in the sperm nucleus, either through oxidation of DNA bases (primarily guanine via lipid peroxyl or alkoxyl radicals) or through covalent binding to MDA, resulting in strand breaks and crosslinking (Sikka, 1996). A reduction in embryonic development after fertilization with DNA-damaged spermatozoa has been described in humans (Ahmadi and Ng, 1999). Possible differences among BHT concentrations in the protective effect on sperm DNA integrity could explain differences in the ability of thawed spermatozoa to develop embryos in vitro. Unfortunately, as DNA damage in thawed spermatozoa was not evaluated in the present study, it was not possible to check the above-mentioned hypothesis. However, if lipid peroxidation promotes sperm DNA damage and oocyte fertilization with DNA-damaged spermatozoa results in a low rate of embryo development, then the reduction of lipid peroxidation should improve development in embryos derived from spermatozoa treated with antioxidants. This hypothesis is supported in the present study where the levels of MDA, as indicators of lipid peroxidation, were lower in spermatozoa that had been freeze-thawed in the presence of BHT than in the control. Moreover, the lowest MDA levels were measured when a BHT concentration of 0.4 mM was used, which was the concentration that achieved the highest rate of embryo development in vitro. However, the implications of lipid peroxidation, as well as the protective role of BHT on sperm DNA integrity and its consequences to postthaw sperm fertility of boar spermatozoa in vitro or in vivo, require considerable further investigation.
To summarize, the data presented in this study demonstrated that the presence of BHT in the freezing extender at concentrations ranging from 0.2 to 0.8 mM improved the survival of boar spermatozoa after thawing. Furthermore, at a concentration of 0.4 mM, BHT enhanced the ability of embryos derived from thawed spermatozoa to develop in vitro. These results also suggest that the protective effect of BHT on cryopreserved spermatozoa is directly related to a reduction in lipid peroxidation. We conclude that adding BHT to the freezing extender improves the overall efficiency of utilization of thawed boar spermatozoa.
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Acknowledgments |
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Footnotes |
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