The overall oxidative state of the cell, with the main ROS and the system of enzymatic antioxidants, are summarized in Figure 2.
The importance of studying OS for the assessment of animal welfare and health has led researchers to focus on studying the imbalance between oxidants and antioxidants in animal cells.
2. Oxidative Stress in Erythrocytes
Hematopoietic stem cells (HSCs) of bone marrow are multipotential cells that give rise to mature cellular elements of the blood (e.g., red blood cells (RBCs), neutrophils, monocytes, platelets, etc.) [
51]. Erythropoiesis is the process of proliferation and progressive differentiation of HSCs into RBCs. Precursor cells undergo a series of division and differentiation steps until the nucleus is extruded (in mammals) [
52]. Mature RBCs have no nuclei and organelles, and thus are not able to synthesize proteins. Therefore, the entire complement of functional proteins must be already present in mature erythrocytes. The RBCs membrane, essential for microcirculation and gas exchange [
53], consists of a phospholipid bilayer with integral proteins associated. Between them, the glycoprotein membrane Band 3 protein (B3p) makes up to 50% of erythrocytes membrane proteins [
41].
Several studies report that oxidative damage in erythrocytes leads to irreversible clustering of B3p [
54,
55]. In physiological conditions, this is an essential step of RBCs senescence and eryptosis processes, that result in cellular removal [
42,
43]. Such structural alteration, linked to oxidative damage, implies the removal of senescent erythrocytes [
55]. Baralla et al. [
18] reported that the sheep erythrocytes, damaged by the treatment with prooxidant molecules, cannot be eliminated in in vitro conditions, because they are not provided in in vivo blood circle, and then, they undergo hemolysis due to membrane damage.
Oxidative damage has been demonstrated to decrease the survival and rheological properties of erythrocytes, affecting their homeostasis, which is tightly linked to B3p functions, particularly vulnerable to redox balance variations [
55]. Alterations in erythrocyte deformability, caused by OS, underline the problems in the microcirculatory profile [
56].
OS can damage membrane PUFAs, such as RBCs hemoglobin and several enzymes (particularly their sulfhydryl groups) [
57]. Oxidation of hemoglobin alpha leads to the formation of hemichromes, which are proportional to hemolysis [
58,
59]. Interaction of oxidized hemoglobin with the membrane might lead to removal of RBCs through the increase in membrane rigidity, decrease in deformability and/or stimulation of membrane proteolysis [
60]. These processes might be a cause of the increase in morphological changes and osmotic fragility of RBCs, making erythrocytes susceptible to phagocytosis [
18,
61].
After being release from bone marrow, RBCs circulate throughout the vascular system thousands of times before being removed, disassembled, and scavenged by macrophages. The RBC lifespan varies characteristically with species and the differences are at least partially explained by different metabolic rates. Comparative studies reveal that RBCs’ lifespan is positively correlated with species longevity and body mass. As a result, bigger mammals tend to live longer and have longer RBC lifespan than smaller species [
60,
62].
Several experimental studies reported that RBC lifespan in healthy animals may be influenced by RBCs’ antioxidant status. Kurata et al. [
60,
63] found that RBCs’ potential lifespan in several mammalian species is significantly correlated with the RBCs’ levels of SOD, GPX, and GSH.
Aged RBCs have shown compromised antioxidant capacity, including decreases in reduced glutathione, GSR activity and increased lipid peroxidation [
60].
For all these reasons, the RBCs represent an ideal model to investigate oxidative damage in bio-membranes [
64].
3. Oxidative Stress in Spermatozoa
The spermatozoon, a gamete generated in the male reproductive tract, moves to the female reproductive tract in order to fertilize an egg [
65]. In mammals, sperm of the post testicular epididymal tract turns into spermatozoa capable of fertilization [
50]. ROS have proven to be fundamental in sperm maturation and capacitation processes. However, until fertilization, oxidative damage is a threat to spermatozoa [
50]. Membrane integrity, and in particular acrosome integrity, are essential for spermatozoa fertilizing capacity and for sperm penetration into the egg [
66]. PUFA presence gives the membrane the fluidity and flexibility needed to engage in membrane fusion events associated with fertilization [
27].
As a transcriptionally silent cell, spermatozoa largely depend on post-translational modifications of proteins to regulate their functions. Among these regulatory mechanisms, redox regulation plays a significant role, and the deregulation of redox homeostasis is a cause of male infertility [
65].
Several technologies have been experimented to improve animal reproductive performances. Among them, the cryopreservation of semen, widely used in animals, is an energy-demanding activity, which generates ROS during the metabolic processes [
67].
OS represents a major factor in sub lethal cryodamage of sperm in animal species, because, after semen dilution and cryopreservation, there is a significant reduction in the level of spermatozoa antioxidants, thus leading to enhanced susceptibility of these cells to peroxidative injuries [
27,
68].
In mammalian spermatozoa, ROS can attack important substrates, such as DNA, PUFA, and proteins [
69]. Experimental studies revealed that OS breaks the DNA strand in spermatozoa, as detected via the comet assay [
27,
69].
The lipid peroxidation of PUFA in spermatozoa results in the loss of membrane functionality and integrity, and it varies across sperm regions [
70,
71]. For example, frozen/thawed ruminants spermatozoa showed more intense lipid peroxidation in the sperm flagellum with a greater PUFA content, with respect to the sperm head [
71,
72,
73]. MDA is a cytotoxic aldehyde produced by lipid peroxidation and its assay provides important indications as an OS marker [
27,
74]. Researchers found that the use of antioxidants in the sperm freezing extender can reduce the destructive effects of ROS and can improve the post-thawing quality of goat spermatozoa [
75].
Spermatozoa proteins are involved in key functions, such as sperm motility, capacitation, oocyte binding ability, and the acrosome reaction [
76]. Significant redox-dependent modifications of proteins are thiol oxidation, tyrosine nitration, and S-glutathionylation. O’Flaherty et al. [
77] reported that these reactions were associated with an impairment of sperm function leading to infertility, altering sperm motility in ruminants and equine, and sperm capacitation. Within proteins, the specific ratio of oxidated/reduced thiol groups (SS/SH) is essential to assure protein functions, but it can be affected by ROS [
77]. Thus, the quantification of total thiols and/or GSH in cells is critical for monitoring the level of OS.
In cellular detoxification processes, the SOD-CAT-GPX catalytic triad represents the antioxidant defense against excessive ROS production in spermatozoa (
Figure 2). GPX is the major representative of catalytic triad and its expression failure in the spermatozoa is correlated with infertility [
50].
4. Assays for Measurement of ROS
4.1. ROS Assay in Erythrocytes
Two recent papers for the measurement of ROS in ovine erythrocytes, using the most common ROS assays in RBCs (7 × 10
6 RBCs/mL), with fluorescence detection, were reported [
18,
46]. In both assays, probe 2′,7′-dichlorodihydrofluorescein diacetate (H
2DCF-DA) at the final concentration of 3 µM was used. Within the cell, the esterase cleaves the acetate groups of H
2DCF-DA, resulting in the formation of the probe 2′,7′-dichlorodihydrofluorescein (H
2DCF). Then, intracellular ROS oxidize the H
2DCF, yielding the fluorescent product, 2′,7′-dichlorofluorescein (DCF). Fluorescence was measured using a fluorescent microplate reader at excitation and emission wavelengths of 485 and 535 nm, respectively. All fluorescence measurements (relative fluorescence unit—RFU) were corrected for background fluorescence [
46] and expressed as RFU/10
6 erythrocytes. In the two papers, the values of intracellular ROS for untreated RBCs of sarda sheep were ≈300 RFU/10
6 erythrocytes. Given that H
2DCF-DA is not cell-specific, some authors quantified fluorescence specifically on animal erythrocytes, removing leukocytes and platelets signal, using flow cytometry [
78].
4.2. ROS Assay in Spermatozoa
Different spectrophotometric, fluorometric and chemiluminescent assay methods for intracellular ROS quantification in small domestic ruminant spermatozoa are summarized in Table 3.
Falchi et al. [
79] used 2′,7′-dichlorodihydrofluorescein diacetate probe (H
2DCF-DA, final concentration of 10 µM) for the assessment of intracellular ROS in spermatozoa of rams (Italy). Samples (600 × 10
6 spermatozoa/mL) were analyzed via flow cytometric analysis. Fluorescence emission increased from a basal value of about 2 to a value of about 5 following sperm incubation at 4 °C for 96 h with or without increasing concentrations of cerium dioxide nanoparticles (CeO
2 NPs). ROS concentrations ranged from 1.5 to 6 Rfu (relative fluorescence unit).
Merati et al. [
80] measured, via a flow cytometer at 488 nm, the ROS level in spermatozoa of rams (4–5 years old, Iran). Briefly, 10 mL of 2′,7′-dichlorofluorescein diacetate (DCFH-DA, 25 mM), and 20 mL of dihydroethidium (DHE, 125 mM) were added to 1 × 10
6 sperm suspension and incubated at 25 °C for 40 min for DCFH-DA and for 20 min for DHE. DCFH-DA is considered a general indicator of ROS, reacting with H
2O
2, ONOOֺ°, lipid hydroperoxides, while DHE is used extensively to monitor superoxide production. DHE upon reaction with superoxide anions forms a red fluorescent product (ethidium = HE) which intercalates with DNA. Green fluorescence (DCFH) was evaluated between 500 and 530 nm, and red fluorescence (HE) was assessed between 590 and 700 nm (excitation, 488 nm; emission, 525 and 625 nm). Data were expressed as the percentage of fluorescent spermatozoa. Propidium iodide (PI) has been used as a counter-stain dye for DCFH and Yo-Pro-1 as a counter-stain dye for HE. The results ranged from 22.8% to 56.1% for H
2O
2 and from 0.4% to 3.1% for O
2−.
Reiten et al. [
81] used spermatozoa (5 × 10
6 spermatozoa/mL) of the Norwegian dairy goat breed (age 208–223 days, Hjermstad, Norway) for assaying ROS with flow cytometer. Hoechst 34580 (1.25 µM) and Mitotracker Orange CMTMRos (MO, 0.15 µM) (Invitrogen, ThermoFisher Scientific, Rodano, Italy) were used to eliminate non-spermatozoa events based on DNA and mitochondrial staining, respectively. PI (5 µg/mL) was used to discriminate between plasma membrane-intact and degenerated spermatozoa, while CellROX R Deep Red Reagent was used to assess levels of ROS as a measure of cellular oxidative stress. The results ranged from 10 to 60%.
Escobar et al. [
82] assayed ROS, with a spectrofluorimetric method using DCFH-DA, in rams spermatozoa (average age 10 months old, Brazil). The samples were incubated in the dark with 5 mL of DCFH-DA (1 mM). The oxidation of DCFH-DA to DCFH by the ROS was monitored. The fluorescence intensity emitted at 520 nm (488 nm excitation) was monitored 60 min after the addition of the probe. The results ranged from 10 to 100 Rfu.
Gimeno-Martos et al. [
83] assayed ROS in spermatozoa of Raza Aragonesa rams (2–4 years old, Zaragoza, Spain). Briefly, 5 × 10
6 sperm/mL were stained with 5 µL of probes (H
2DCF-DA, 20 µL and PI, 1.5 mM) after 15 min at 37 °C in the dark; the samples were fixed with 5 µL formaldehyde (0.5% in water) and analyzed via flow cytometry (filter 525 and 675 nm). Intracellular ROS levels ranged between 3.9 and 11.2 Rfu.
Liu et al. [
84] assayed ROS in spermatozoa of Guanzhong dairy goats (2–3 years old, Shaanxi, China) using DCFH-DA. Briefly, 1 × 10
6 spermatozoa were washed in PBS and were incubated with 100 mM DCFH-DA at 37 °C for 30 min. The fluorescence of DCF was measured on a flow cytometer at a wavelength of 485/535 nm. The results ranged from 8.36 to 53.83% for DCF-positive cells.
Lv et al. [
85] used goats (2–3 years old, Kunming, China) for the collection of semen. Briefly, 1 × 10
6 spermatozoa/mL was mixed with H
2DCF-DA (20 μM) and 50 μL PI (50 μg/mL). Then, the samples were incubated for 60 min at room temperature in darkness. The spermatozoa suspension was analyzed using flow cytometry. Results are expressed as percentage of viable spermatozoa with less ROS production (identified by H
2DCF-DA negative and no PI staining) and were ranged from 54 to 67%.
Zarepourfard et al. [
86] used male goats (5–6 years old, Isfahan, Iran) to carry out semen collection employing flow cytometer to determine the ROS content. The percentage of ROS positive spermatozoa was measured following incubation of 1 × 10
6 sperm/mL with 5 mM of DCFH-DA for 30 min at room temperature. Live sperm produce a detectable amount of physiological ROS and therefore, the sperm may become DCF-positive. ROS results ranged from 38.7% to 62.0%.
Kumar et al. [
87] measured oxidative status in spermatozoa of sexually mature and healthy goats (2–3 years old). The sperm (10 × 10
8 spermatozoa/mg protein) was mechanically lysed by liquid nitrogen, centrifuged and the supernatant was used for the analysis. OS was assessed by monitoring the concentration of the
N,
N-diethylparaphenylendiamine (DEPPD) radical cation. The formation of this radical cation is not only due to hydroperoxides present in the sample, but also other oxidizing agents. ROS results ranged between 0.16 ± 0.011 and 0.74 ± 0.028 mg H
2O
2/10
8 spermatozoa. [
87].
Anzalone et al. [
88] used a dichloromethyl derivate of H
2DCFDA (5-(and 6-)chloromethyl-2′,7′-dichlorodihydrofuorescein diacetate (CM-H
2DCFDA, final concentration of 3 µM) as a probe for ROS determination in intact ram spermatozoa. CM-H
2DCFDA is sensitive to a wide range of ROS (H
2O
2, ONOO-, superoxide anion, and hydroxyl). Fluorescence measurements (excitation and emission wavelengths were 490 nm and 520 nm, respectively) were carried out in a multimode plate reader during overnight incubation (38 °C). The kinetic of the probe oxidation rate was evaluated from the slope of the fluorescence emission intensity in the initial 10 min of the total recording time. The results are expressed as mean and standard deviation of fluorescence intensity slope as a function of time (DF/min) in the linear region (corresponding to the first 10 min of the kinetic measurement) and the authors found ROS equal to ≈ 63 DF/min when spermatozoa were diluted in PBS.
The same CM-H
2DCFDA fluorescent probe for ROS quantification in ovine spermatozoa was also performed using a cytofluorometer detector [
89,
90]. Del Olmo et al. [
89] found that the 3.3% ÷ 4.0% ± 0.2% of live spermatozoa positive to probe in ram spermatozoa (10
8 cells/mL) using flow cytometer. Vašíček et al. [
90] measured ROS levels in ram semen samples (1 × 10
6 spermatozoa in PBS) via flow cytofluorimetry using four different fluorescent probes: a green dye nonspecifically indicating the presence of intracellular ROS (CM- H
2DCFDA, final concentration of 500 nM), a red superoxide indicator (DHE, final concentration of 2 µM), a red mitochondrial superoxide indicator (MitoSOX™, final concentration of 500 nM), and a green lipid peroxidation sensor (BODIPY™, final concentration of 200 nM) [
90]. They reported 25 ÷ 40% positive cells to CM- CM-H
2DCFDA, 15 ÷ 25% positive cells to DHE, 10 ÷ 20% positive cells to MitoSOX and 8 ÷ 20% positive cells to BODIPY. The authors reported that the unspecific CM-H
2DCFDA probe had higher proportion of ROS positive spermatozoa than the specific probes. Thus, CM-H
2DCFDA seems to be a suitable probe for rapid unspecific detection of ROS production in ram semen samples prior to their further processing [
90].
Zarei et al. [
91] evaluated the intracellular H
2O
2 concentration as an index of ROS, using DCFH-DA as a fluorescent probe (final concentration of 25 µM). DCFH-DA probe was added to ram sperm (Zandi sheeps 3 ÷ 5 × 10
6 spermatozoa/mL 200 cells/slide) and the fluorescence intensity was evaluated using a fluorescent microscope (490 nm/520 nm, excitation/emission wavelengths, respectively). ROS concentration was expressed as the percentage of probe-positive cells out of the total spermatozoa counted. The authors [
91] found 10% of ROS in fresh semen and 24 ÷ 30% in frozen–thawed semen.
O’Brien et al. [
92] detected ROS in sperm (25 × 10
6 sperm/mL 200 sperm cells/slide) of four different ovine species (ram (
Ovis aries), mouflon (
Ovis musimon), buck (
Capra hircus), and Iberian ibex (
Capra pyrenaica) from Madrid (40°25′ N), Spain) using a CellROX R green probe (final concentration of 5 µM) by an epifluorescence microscope with a triple band-pass filter (450 nm/490 nm, excitation/emission, respectively). This fluorescent probe penetrates the cell and when oxidized by intracellular free radicals, binds to DNA, emitting a more intense green fluorescence. The response to the stress of each species was illustrated by calculating a stress resistance ratio (SR) for the sperm variables: SR = (value after stress/value before stress) × 100 [
92]. The ROS in sperm were evaluated before the stress condition, after refrigeration at 15 °C for 20 h, and subsequent incubation at 38.5 °C for 2 h. ROS increases significantly in three of the four sheep species after incubation at 15 °C and also after subsequent incubation at 38 °C, increasing from SR basal values of 100 to SR maximum values of 350.
Jiménez et al. [
93] detected intracellular superoxide (O
2−•) levels in ram semen (5 × 10
6 cells/mL) from Raza Aragonesa rams (2–4 years old) located in Zaragoza, Spain, using DHE (final concentration of 4 µM) and Yo-Pro-1 (final concentration of 40 nM) fluorochromes. DHE is permeable to cells, and it is oxidized by O
2−• to the red fluorescent compound ethidium (E) and detected using flow cytometer. Yo-Pro-1 labels non-viable cells with green fluorescence. A percentage of 10% of viable spermatozoa with high superoxide levels (Yo-Pro-1
−/E
+) was found, although the values increased (35%) with in vitro addition of calcium ionophore, and then returned to lower values (20%), with the concomitant presence of melatonin and its antioxidant action.
Wang et al. [
94] used a commercial kit (Beyotime Institute of Biotechnology, Shanghai, China) to determine ROS content in ram semen (2.0 × 10
9/mL), using DCFH-DC as a probe. The fluorescence intensity was monitored using a multifunctional microplate reader (PerkinElmer Inc., NYSE: PKI, Waltham, MA, USA) at Ex/Em = 488/525 nm). The results found ranged from 2500 to 3500 rfu.
Yu Gao et al. [
95] studied old Suffolk White rams (age of 1–2 years Beijing, China) and the in vitro effect of leptin on their sperm quality. Intracellular ROS of sperm was assessed with a ROS Assay Kit (SAS, Beijing, China) containing H
2DCFDA according to the manufacturer’s instruction. Briefly, 1 µL of H
2DCFDA and 5 µL of PI were added into the sperm suspension and mixed well, following incubation at 37 °C for 30 min in the dark. The samples were centrifuged and suspended with PBS. Then, the samples were detected using a flow cytometer. ROS levels determined were 0.25 ÷ 0.8%.
Shahat et al. [
40] studied the effects of melatonin or L-arginine on the quality of frozen-thawed sperm from heat-stressed Dorset rams (3–4 years old, Canada). For total ROS, ~3 × 10
6 sperm were centrifuged at 400×
g for 5 min, yielding a working concentration of 1 × 10
5 sperm/sample. Then, total ROS was analyzed using a total ROS Assay Kit 520 nm (Invitrogen Life Technologies, Carlsbad, CA, USA) on BD™ LSR II flow cytometer (BD Biosciences, Oxford, UK) at 520 nm using the FITC channel. The flow rate was set to 200 events/s, with 10,000 events counted per sample and all samples tested in duplicate. The ROS detection solution contains a fluorescent probe that stains ROS in sperm, with results expressed as a percentage of sperm that had high ROS activity. The values found ranged from 62.1 ± 1.0 to 79.4 ± 1.4 ROS%.
Liang et al. [
96] studied the effects of four extenders for semen cryopreservation (Andromed
® (Andr
®), Optidyl
® (Opt
®), P3644 Sigma l-phosphatidylcholine (l-α SL), and skim milk-based (milk) extenders) on the post-thaw quality and fertility of goat semen (Yunshang black bucks, weight 80–100 kg, aged between 2 and 3 years). The intracellular concentrations of ROS in frozen–thawed sperm were determined by staining with 2′, 7′-dichlorodihydrofluorescein diacetates (H
2DCFDA) with flow cytometry analysis. Briefly, 500 μL of semen sample was diluted in the TALP buffer to obtain a final concentration of 1 × 10
6 sperm/mL and mixed with 0.5 μL H
2DCFDA (final concentration of 20 μM) and 50 μL PI (50 μg/mL). Then, the samples were incubated for 60 min at room temperature in the darkness. The sperm suspension was analyzed using flow cytometry. The percentage of viable sperm with low ROS was identified by H
2DCFDA negative and no PI staining. The green fluorescence from FITC-PSA, Annexin-V-FITC, and H
2DCFDA was detected on a FacStar-plus flow cytometer (FAC-SCalibur) on the FL1 photodetector (530/30 BP filter). The values found ranged from 45 to 60 ROS%.
Longobardi et al. [
97] studied the effect of crocin before cryopreservation in the extender for bucks/breed (2–4 years age, Italy) semen. ROS levels were measured as fluorescence emission of DHE. This probe is a cell-permeable compound oxidized by superoxide anion (O
2−•) to ethidium bromide that binds to DNA and emits red fluorescence. DHE (2 µM) was added to frozen–thawed sperm samples and incubated in the dark, at room temperature, for 20 min. Emission was monitored at 570 nm, using a plate reader (GloMax
®-Multi Detection System-Promega, Milano, Italy). ROS levels were evaluated as arbitrary units of fluorescent signal. ROS values ranged between 437.8 ± 4.9 and 347.6 ± 2.8 fluorescence intensity.
Monteiro et al. [
98] evaluated the effect of antifreeze protein type III (AFP III) on the freezing of epididymal spermatozoa of goat (Brejo da Madre de Deus-PE, Brazil). For intracellular ROS levels analysis, performed with the Amnis ImageStream Mark II flow cytometer (EMD Millipore Corp., Lausanne, Switzerland), 5 μL of CM-H
2DCFDA (50 μM in PBS) were added to the samples at 37 °C for 30 min. These were subsequently diluted with 1 mL of PBS and centrifuged (100×
g/5 min) to remove unbound fluorochrome, and the sediment was resuspended with 40 μL of PBS. Then, 5 μL of PI was added to the sample, incubated at room temperature (5 min) and analyzed. The results were expressed as a percentage of viable cells with high levels of ROS (DCFDA+/PI). Values ranged from 79.02 ± 35.51 to 88.67 ± 23.13 ROS %.
Esmaeilkhanian et al. [
99] assessed the efficacy of Mito-TEMPO on post-thawed goat sperm quality using Saanen goats in breeding season for sperm collection. Dichlorofluorescein diacetate (DCFH-DA) evaluated the intracellular H
2O
2 concentrations as an index of ROS. Semen samples were rinsed with PBS to a concentration of 3–5 × 10
6 spermatozoa/mL. DCFH-DA (25 μM) was added to the sperm suspension and incubated for 40 min at 25 °C. After washing, 2 μL of PI were added to the semen, and samples were analyzed via flow cytometry. Obtained values were ranged from 20 to 25 ROS %.
Nazari et al. [
100] studied the effect of trehalose and pentoxifylline in diluents on cooled and frozen–thawed Markhoz goat sperm (3–4 years old of age and weighing 60–65 kg, Sanandaj, Iran). ROS flow cytometry (excitation: 488 nm; emission: 525–625 nm) was carried out using two specific dyes, DCFH-DA and DHE, to detect the intracellular H
2O
2 and O
2−• in 1 × 10
6 spermatozoa. Data were expressed as the percentage of fluorescent sperm and PI was used as a counterstain dye for DCFH. ROS % values ranged from 19.24 to 52.78 and from 1.73 to 2.61 for H
2O
2 and O
2−•, respectively.
Lv et al. [
101] studied the effects of antifreeze protein (AFP) on frozen spermatozoa of black goats (2–3 years old Kunming, Yunnan province, China). The ROS ratios were measured with a flow cytometer by incubating spermatozoa with H
2DCFDA. In brief, a 500 µL semen sample was first mixed with the TALP buffer to a final concentration of 1 × 10
6 spermatozoa/mL. Then, H
2DCFDA (final concentration of 20 mM) and PI (50 mg/mL) were added to the above solution. Finally, mixed samples were incubated in darkness for 60 min at room temperature. Flow cytometry was used to examine the spermatozoa suspension. The percentage of viable spermatozoa with low ROS was identified by negative H
2DCFDA and no PI staining. Values ranged from 60 to 65 ROS %.
Sun et al. [
102] measured the levels of ROS in goat semen from Chongming White goats (3–5 years old) located in Shanghai, China, during spring to early summer, by a chemiluminescence assay using luminol (5-amino-2,3-dihydro-1,4-phthalazinedione). ROS levels were higher in the post-thawed spermatozoa containing soybean lecithin (SL) added to the extender at different concentrations, than in the control (egg yolk (EY) present in the extender). Only SL at 2% brought the ROS values equal to the control (5.5 IU/mL = intensity light units/mL).
Mehdipour et al. [
103] investigated the effects of rosiglitazone on rams semen after cryopreservation on the quality of thawed sperm. Sperm from sexually mature Ghezel rams (3 to 4 years of age, Tabriz, Iran.) were sampled. After washing spermatozoa with PBS and their centrifugation at 300×
g for 7 min, the supernatant was removed and luminol was added to measure ROS production. The results were expressed as 10
3 counted photons per minute (cpm) per 10
6 spermatozoa and ranged from 2 to 4.5 × 10
3 cpm/10
6 spermatozoa.
Table 3. Different methods for ROS assay in spermatozoa of small domestic ruminants.
As can be seen in Table 3, in recent years, most researchers employed fluorescent methods using mostly commercial kits, for ROS quantification. Only two papers with luminescent methods and one with spectrophotometric method are reported.
5. Assays for the Measurement of Enzymatic Antioxidants
5.1. SOD
5.1.1. SOD in Erythrocytes
Different methods for the measurement of SOD in erythrocytes of small domestic ruminants are summarized in Table 4.
In 2021, Pasciu et al. [
46] investigated oxidative response under in vitro conditions using high doses of glycerol on the RBC of Sardinian sheep (Sassari, Italy). Blood cells were treated with HBSS containing 0.1% Triton X100. SOD activity in cellular extracts was enzymatically detected at 470 nm using the xanthine and xanthine oxidase methods. The SOD levels ranged from 50 to 80 U/106 erythrocytes.
Mousaie et al. [
106] measured SOD activity in erythrocytes of male lambs (Jiroft, Iran), 28.5 ± 2.6 kg of body weight. RBC hemolysate was prepared according to manufacturer’s protocol (Randox Ransod kit, Randox Laboratories Ltd., Antrim, UK). The mean SOD level in erythrocytes was 1307.2 ± 29.8 unit per gram Hb (U/g Hb).
Tao et al. [
107] evaluated the effect of copper sulphate poisoning on the morphological and functional characteristics of goat RBCs: for this in vitro study, five goats which were 10–14 months old (Xinjiang Uygur Autonomous Region China) were used. Erythrocytes were hemolyzed under hypotonic conditions. SOD activity was measured in terms of inhibition of the decrease in nitro-blue tetrazolium (NBT) by superoxide. One unit of SOD activity was determined as the amount of enzyme that caused a reduction in half the maximum suppression of NBT; this reduction was acquired by measuring the absorbance at 550 nm. The SOD obtained was 200 ÷ 300 U/mg protein.
In 2022, Zheng et al. [
49] measured the antioxidant effect of flavonoids extracted from Chinese herb mulberry leaves in an in vitro study on sheep erythrocytes for analyzing the activity of antioxidative enzymes. Commercial kits (Nanjing Jiancheng Institute of Biotechnology of China) were used to assay SOD, GPX and CAT. Blood cells were collected in tubes with heparin anticoagulant and washed three times with PBS (pH 7.4), lysed by adding approximately 4 times the volume of ultrapure water and centrifuged (1200×
g, 10 min, 4 °C) after 10 min of an ice bath. The obtained cell lysate was stored at −80 °C until analysis. Reported values, were of 2 ÷ 13 U/mg protein, 1 ÷ 5.5 U/mg protein and 10 ÷ 65 U/mg protein for SOD, CAT and GPX, respectively.
Sousa et al. [
108] used a commercial Randox kit (RANSOD) to measure SOD levels in RBCs of non-pregnant Santa Inês crossbred sheep (weighing on an average 52.89 ± 6.7 kg, semi-arid, UFERSA, Brazil). Blood samples were centrifuged and subsequently, RBCs were washed three times with phosphate solution (PBS 10%). Then, a freeze–thaw cycle was performed at −20 °C for 10 min, followed by melting at room temperature for another 10 min, repeating the process for two consecutive times. The obtained hemolysate was stored at −40 °C until analysis. The mean found SOD value was 11.9 ± 4.12 U/g Hg.
Seifalinasab et al. [
109] studied the effect of dietary treatments with chromium supplementation on male lambs (Jiroft, Iran) (8–9 months old, average body weight of 31.9 ± 1.2 kg). Blood sample was taken in heparinized tubes and SOD activity was measured with a commercial kit Ransod (Randox Laboratories Ltd., Antrim, UK). The method employs xanthine and xanthine oxidase to generate superoxide radicals which react with 2-(4-iodophenyl)-3-(4-nitrophenol)-5-phenyltetrazolium chloride to form a red dye (470 nm). The SOD activity is then measured by the degree of inhibition of this reaction. The mean value for SOD was 1127.37 ± 48.75 U/g Hb.
Table 4. Spectrophotometric methods for SOD detection in erythrocytes of small domestic ruminants.
As can be seen in Table 4, all analyzed studies reported spectrophotometric methods, and many of them used commercial kits.
5.1.2. SOD in Spermatozoa
In
Table 5, a summary of SOD assays in spermatozoa of small domestic ruminants is reported. In particular, Hashem et al. [
111] determined the total SOD activity in spermatozoa of Qezel rams (3–4 years of age, Urmia, Iran), assaying the auto oxidation and illumination of pyrogallol at 420 nm for 3.5 min. One-unit total SOD activity was calculated as the amount of protein causing 50% inhibition of pyrogallol autooxidation. A blank without treated sample was used as a control for non-enzymatic oxidation of pyrogallol in Tris–EDTA buffer (50 mM Tris, 10 mM EDTA, pH 8.2). The total SOD activity was expressed as units per milligram of protein (unit/mg protein) in the spermatozoa samples and the authors found 50 ÷ 60 Unit/mg protein for SOD spermatozoa of ram.
Ren et al. [
112] measured SOD, CAT, and GSH-Px activities from spermatozoa of Cashmere goats (aged 3–5 years old, Yulin, Shaanxi, China). The samples from the thawed frozen semen were centrifuged at 1600×
g for 5 min at 25 °C, and the supernatant was discarded. The sperm pellet was re-suspended with Triton X-100 (1%) for 20 min for extracting enzymes, was centrifuged at 4000×
g for 30 min at 25 °C and its supernatant was collected for follow-up determination. The antioxidant enzyme activities of SOD, CAT, and GPX were detected using a commercial enzyme detection kit (Nanjing Jiancheng Bioengineering Institute, Nanjing, China). The results were 200 ÷ 250 U/mL for SOD, 1.8 ÷ 3.10 U/mL for CAT, and 18 ÷ 33 U/mL for GPX.
Liu et al. [
113] evaluated the antioxidant effects of a diet with different zinc levels on spermatozoa of Liaoning Cashmere goats (body weight of 56.2 ± 2.45 kg and age of 3 years, Shenyang, China). Cells were separated from semen fluid and washed by resuspending in PBS. After three centrifugations, 1 mL of Triton X-100 (0.1%) was added to spermatozoa, and the samples were centrifuged again at 8000 rpm for 30 min in a refrigerated centrifuge. The supernatant was analyzed using the Bradford method, and SOD activity was determined using a commercial assay kit (Nanjing Jiancheng Bioengineering Institute, China). The SOD values ranged from 18 to 30 U/mg protein.
Al-Mutary et al. [
114] studied the effect of resveratrol on antioxidant enzyme activities of ram sperm during cooling storage. Ram spermatozoa (50 × 10
6/mL) were grinded using satirized Sigma rods (pestles for 2 mL tubes), and then centrifugated and analyzed for SOD evaluation using a colorimetric method that measured its ability to inhibit the phenazine methosulphate reduction in nitroblue tetrazolium dye. SOD levels, measured at 560 nm, ranged from 112.75 ± 5.80 U/mL to 180.09 ± 12.55 U/mL.
Mortazavi et al. [
115] evaluated SOD activity by determining the extent of inhibition of pyrogallol autoxidation. Ram spermatozoa (25 × 10
6/mL) was electronically homogenized at 5.000 ÷ 6.000 g for 5 min. The assay data were normalized considering the concentration of spermatozoa. The authors found 24.07 ± 1.48 U/mL ÷ 31.45 ± 5.13 U/mL of SOD.
Žaja et al. [
116] investigated the effect of melatonin on antioxidative enzyme activity in the seminal plasma and spermatozoa of French Alpine bucks (with body weight ranging from 40 to 60 kg, aged 1.5 to 4 years, Varazdin, Croatia) during the nonbreeding season. The samples of spermatozoa were prepared as cellular lysates. The frozen samples were thawed and resuspended in cooled distilled water, then stored in a refrigerator at 4 °C for 10 min. The samples were then centrifuged at 2400×
g for 5 min, and the obtained supernatants were used for analyzing the activity of antioxidative enzymes. SOD activity was determined using a commercial kit (Randos, Randox Laboratories) that uses xanthine and xanthine oxidase for generating superoxide radicals which react with 2-(4-iodophenyl)-3-(4-nitrophenol)-5-phenyltetrazolium chloride to form a red formazan dye. SOD activity was spectrophotometrically measured at 505 nm observing the degree of inhibition of this reaction. The activity of SOD in spermatozoa was 100 ÷ 600 U/g of protein.
Saberivand et al. [
117] assayed SOD activity in Romanov ram spermatozoa (Tabriz, Iran), based on the inhibition of nitro blue tetrazolium (NBT) reduction by superoxide radicals to blue-colored formazan. The reaction was followed by reading at 560 nm. Semen hemolysate was prepared by treating cells with ethanol and chloroform, and, after centrifugation, the supernatant was used for the assay. SOD activity is defined as the amount of enzyme required to inhibit the reduction in NBT by 50% detectable via the spectrophotometer at 560 nm and results were reported as U/mg protein (76.20 ÷ 118.60 U/mg prot).
Wang et al. [
94] used a WST-8 kit (Beyotime Institute of Biotechnology, Shanghai, China) for measuring SOD activity in ram. Samples of semen (2.0 × 10
9/mL) were centrifuged at 12,000×
g for 5 min, and after incubation with WST-8/enzyme working solution, the absorbance at 450 nm was determined. SOD activity was 110 ÷ 220 U/mg protein. One unit of total SOD activity was calculated as the amount of protein causing 50% inhibition of pyrogallol autooxidation.
Also, Shayestehyekta et al. [
118] studied the effect of melatonin on fresh epididymal spermatozoa of ram (2–5 years old, Kermanshah, Iran) after post-mortem recovery under normal and oxidative stress conditions under liquid preservation (4 °C) at different times (24, 48 and 72 h). To assess SOD activity, a SOD assay kit (TPR INNOVATIVE) was used after ultrasonic lysis on the ice of spermatozoa pellets and centrifugation at 6000 rpm for 10 min. The activity of SOD was 30 ÷ 70 U/mL.
Zhang et al. [
105] studied the effects of proline supplementation on goat sperm (healthy Laoshan bucks aged between 1.5 and 2 years, Qingdao, China). SOD activity was assayed with a microplate reader at 450 nm, using a commercial kit (A001-3-2, Nanjing Jiancheng Bioengineering Institute) after ultrasonication on ice. The values found were 2.5–3.5 U/µg protein.
Zou et al. [
104] explored the effect of bovine seminal plasma replacing different doses of dairy goat seminal plasma on semen freezing quality of Guanzhong dairy goat (2.5–3 years old, Lantian, Shaanxi Province, China). Thawed semen was used for SOD, and ROS assay using commercial kits (BC 0175, and CA1410) from Solarbio and the amount was found to be 165.99 ÷ 199.78 U/mL for SOD (
Table 5), and 397.58 ÷ 461.79 U/mL for ROS (
Table 3).
Li et al. [
119] investigated the cryoprotective melatonin effect on the semen of healthy adult Huang-Huai rams (2–4 years of age) (Dingyuan County, Anhui province, China). Semen was diluted using two types of cryopreserved media (with and without melatonin) at a final sperm concentration of about 3 × 10
8/mL. Fresh and cryopreserved semen pellet was sonicated on ice using a high intensity ultrasonic processor (Scientz) in pre-cooled sodium chloride injection (0.9% NaCl) (
m/
v) and 1% Triton X-100, followed by centrifugation at 5000×
g for 10 min at 4 °C. The total SOD concentration, determined using a commercial assay kit (A001–1-2; Nanjing Jiancheng, China), was about 45 ÷ 60 U/mg protein.
Table 5. Spectrophotometric methods for SOD detection in spermatozoa of small domestic ruminants.
As can be seen in Table 5, all analyzed studies reported spectrophotometric methods, with many of them using commercial kits.
5.2. CAT, GPX, and GSR
5.2.1. CAT, GPX, and GSR in Erythrocytes
In the last five years, as reported in
Table 6, only Zheng et al. [
49] measured the antioxidant activity of enzymes GPX and CAT within erythrocytes. They used a commercial kit (Nanjing Jiancheng Institute of Biotechnology of China) to in vitro assay the antioxidant effect of Chinese herb mulberry leaves. Blood cells, collected in tubes with heparin anticoagulant, were washed three times with PBS (pH 7.4), lysed by adding ultrapure water and centrifuged (1200×
g, 10 min, 4 °C) after 10 min of an ice bath. The levels of CAT and GPX ranged from 1 ÷ 5.5 U/mg protein to 10 ÷ 65 U/mg protein, respectively.
Table 6. Analytical methods for CAT, GPX, and GSR detection in erythrocytes and spermatozoa of small domestic ruminants.
5.2.2. CAT, GPX, and GSR in Spermatozoa
In
Table 6, a summary of CAT, GPX, and GSR assays in spermatozoa of small domestic ruminants is reported. In particular, Žaja et al. [
116] investigated the effect of melatonin on the antioxidative activity of enzymes GPX, GSR, and CAT in French Alpine bucks spermatozoa (body weight ranging from 40 to 60 kg, aged 1.5 to 4 years Varazdin, Croatia). The cellular lysates were centrifuged at 2400×
g for 5 min, and the obtained supernatants were used for analyzing the antioxidant activity of GSR, GPX, and CAT, using commercial kits (glutathione reductase kit, Randox Laboratories; Ransel kit, Randox Laboratories, Crumlin, UK; and Cayman Catalase Assay kit, Cayman Chemical Company, Ann Arbor, MI, USA, respectively). The absorbance was measured spectrophotometrically at 340 nm for both GSR and GPX and at 540 nm for CAT, using a Microtiter plate reader (Human, Wiesbaden, Germany). The obtained results were 2000 ÷ 3500 U/g protein for GSR, 3200 ÷ 4000 U/g protein for GPX and 300 ÷ 750 nmol/min/g protein for CAT.
Liu et al. [
113] evaluated the GPX and CAT levels in spermatozoa, following the procedure already reported in the paragraph of SOD. The activities of GPX and CAT were determined using commercial assay kits (Nanjing Jiancheng Bioengineering Institute, Nanjing, China). The obtained results were 20 ÷ 80 U/mg protein for GPX and 2.5 ÷ 3 U/mg protein for CAT.
Li et al. [
119] investigated the antioxidative enzyme activities in spermatozoa of Huang-Huai ram (2–4 years of age, Dingyuan county, Anhui province, China), followed by in freezing medium supplemented with melatonin. Sperm pellet (3 × 10
8/mL) was sonicated on ice using a high intensity ultrasonic processor (Scientz) in pre-cooled sodium chloride injection (0.9% NaCl) (
m/
v) and 1% Triton X-100, followed by centrifugation at 5000×
g for 10 min at 4 °C. GPX and CAT activities were measured using commercial kits (A005–1-1 and A007–1-1, Nanjing Jiancheng, China, respectively) and the absorbance was read at 412 nm (GPX) and 405 nm (CAT). GPX and CAT levels were 10 ÷ 16 U/mg protein, and 0.12 ÷ 0.20 U/mg protein, respectively.
Zou et al. [
104] explored the GPX levels in Guanzhong dairy goats (2.5–3 years old, Lantian, China). GPX activity, assayed with a commercial kit (BC1195 from Solarbio), was 106.30 ÷ 133.55 U/L.
As can be seen in Table 6, all analyzed studies reported spectrophotometric methods with the use of commercial kits. Most used kits are those for CAT and GPX, for both erythrocytes and spermatozoa, while only one manuscript reports the employment of the GSR assay in spermatozoa.