Background
Prostaglandin F
2α (PGF) from the uterus or from the ovary is responsible for the regression of the corpus luteum (CL) in mammals [
1,
2]. In vivo studies in cows demonstrated that intramuscular injections of PGF analogues given in the mid-luteal stage induce an acute decrease in progesterone (P
4) production (functional luteolysis) followed by tissue degradation and a decrease in size of the CL (structural luteolysis) [
2]. On the other hand, in vitro studies showed that direct treatment of pure populations of luteal steroidogenic cells (LSCs) with PGF does not inhibit basal P
4 production by the large LSCs, and stimulates P
4 production by the small LSCs and by a mixture of large and small LSCs [
3,
4] suggesting that PGF action differs in each type of luteal cells. The exact mechanism involved in the luteolytic cascade initiated by PGF remains unclear. Interestingly, several studies reported the presence of PGF receptors in luteal endothelial cells (LECs) and that LECs respond to PGF stimulation [
5,
6], suggesting that LECs are a target for PGF, and that LECs play roles in the local mechanism of CL regression induced by PGF.
Reactive oxygen species (ROS) including hydrogen peroxide (H
2O
2), superoxide anion (O
2-) and hydroxyl radical (OH
-) have been implicated in the luteolytic process [
7]. In rats, PGF induces a decrease in serum concentrations of P
4 in association with increasing generation of superoxide anion and H
2O
2 in the luteal tissue [
8]. Treatment of LSCs with PGF induces ROS production and apoptosis [
9]. Moreover, H
2O
2 was found to stimulate PGF production in human endometrial stromal cells [
10]. We recently observed that an injection of PGF induces a transient (1–2 h) increase in the partial pressure of oxygen (pO
2) in ovarian venous blood [
11], and that the pO
2 of venous blood is higher in the ovarian vein than in the jugular vein in cow. Therefore, the luteal microenvironment seems to be exposed to high O
2 condition, especially during the short period of time (1–2 h) following PGF treatment.
Superoxide dismutase (SOD) acts as an antioxidant enzyme in nearly all cells exposed to oxygen. SOD catalyzes the dismutation of superoxide into oxygen and H
2O
2. Mammalian cells have three forms of SOD. Copper/Zinc (SOD1) is present in the cytosol, nucleus and the inter-membrane space of mitochondria; Manganese SOD (SOD2) is a manganese-containing enzyme that is present in the mitochondrial matrix; Extracellular SOD (SOD3) is a secreted copper-containing protein that is found in the extracellular matrix of tissues [
12]. SOD1 dismutates superoxide radicals resulting from cellular oxidative metabolism into H
2O
2[
13] represents 80% of the total SOD found in the rat CL [
14]. In addition, a decrease in intracellular SOD activity was accompanied by a decrease of P
4 production by rat CL [
15]. However, the local mechanisms controlling the luteolytic actions of PGF in LECs remain unknown. We hypothesized that SOD, the main enzyme involved in the control of intraluteal ROS, is differently regulated at the time of functional (2 h) and structural (24 h) luteolysis.
To test the above hypothesis, we determined the time-dependent changes of SOD in CL tissues after PGF treatment in vivo and the influence of PGF and H2O2 on SOD1 expression and SOD activity in bovine LECs in vitro.
Methods
Collection of CL tissue during PGF-induced luteolysis
The animal procedures were approved by the local institutional animal care and use committee of Polish Academy of Sciences in Olsztyn, Poland (Agreement No. 5/2007, 6/2007 and 88/2007). Healthy normally cycling Polish Holstein Black and White cows were used for collection of CL. Estrus was synchronized in the cows by two injections of an analogue PGF (Dinoprost, Dinolytic; Pharmacia & Upjohn, Belgium) with an 11-days interval. Ovulation was determined by a veterinarian via transrectal ultrasonography examination. Then, CLs were collected by Colpotomy technique using a Hauptner’s effeninator (Hauptner and Herberholz, Solingen, Germany) on day 10 post-ovulation, i.e., just before administration of a luteolytic dose of analogue PGF (Dinoprost, Dinolytic; Pharmacia & Upjohn, Belgium) (0 h), and at 0.5, 2, 12 and 24 h post-treatment (n=4 per time-point). CL tissues were dissected from the ovary and then stored at −80°C until the SOD1 mRNA, protein and total SOD activity analysis.
Bovine LEC isolation and cell culture
LECs were isolated from five CLs at the mid-luteal phase (days 8–12 of the estrous cycle) [
16] using magnetic beads as previously described [
17] and recently validated in our laboratory [
6,
18]. Briefly, magnetic tosylactivated beads (Dynabeads M-450, 140.04; Dynal ASA, Oslo, Norway) were coated with 0.15 mg/ml lectin from
Bandeiraea simplicifolia (BS-1; L2380; Sigma-Aldrich, St. Louis, MO, USA), which specifically binds the glycoproteins expressed by bovine LECs [
17]. Luteal cell (LC) suspension was mixed with beads at a concentration of 4 × 10
8 beads/ml, and incubated for 20 min at 4°C on a rocking platform. The cells were pooled and cultured in endothelial cell (EC) growth medium (MV 2; C22121; Promo Cell, Heidelberg, Germany) at 37°C in a humidified atmosphere of 5% CO
2 in air. Only colonies with a homogeneous cell population were removed with a pipette and cultured in collagen-coated 25 cm
2 culture flasks (690175; Greiner Bio-One, Frickenhausen, Germany). The cultures and passages were repeated until a homogeneous population of pure LECs was obtained. The LECs used in the present study were previously confirmed to be positively stained with rabbit anti-human von Willebrand factor (vWF, F3520; Sigma-Aldrich), isolated LECs expresses CD31 but not
3β-hydroxysteroid dehydrogenase (
3β-HSD) mRNA as reported previously [
6,
17,
18]. Experiments were performed on confluent cultures and the cells (LECs) were from passage 2–5.
The LECs were seeded at a concentration of 1 × 105 viable cells/ml into 24-well plates (662160; Greiner Bio-One) for determination of SOD1 mRNA or PGF production, and 1 × 106 viable cells/ml into 75-cm2 culture flasks (658175; Greiner Bio-One) for determination of SOD1 protein expression and total SOD activity in culture cells. LECs were cultured in DMEM/F-12 (D/F; D8900; Sigma-Aldrich) supplemented with 10% calf serum (v/v, 16170–078; Life Technologies Inc., Grand Island, NY, USA), 20 μM gentamicin (G1397; Sigma-Aldrich) and 2 μM amphotericin B (A9528; Sigma-Aldrich). The cells reached confluence on 5th day of culture. After the cells reached confluence, the medium was replaced with fresh D/F supplemented with 5 μg/ml holo-transferrin (T3400; Sigma-Aldrich), 500 μM ascorbic acid (013–12061; Wako Pure Chemical Industries, Ltd., Osaka, Japan), 5 nM sodium selenite (S5261; Sigma-Aldrich), and 0.1% (w/v) BSA (10 735 078 001; Roche Diagnostics, Mannheim, Germany).
Cell viability test
LECs cultured in 96-well plates were exposed to H2O2 (0.1 – 1000 μM) for the final 24 h of culture. The cell viability was determined by Dojindo Cell Counting Kit including WST-1 (Dojindo, Kumamoto, Japan; No. 345–06463). Briefly, WST-1, a kind of MTT [3-(4,5-dimethyl-2 thiazolyl)-2,5-diphenyl-2 H-tetrazolium bromide], is a yellow tetrazolium salt that is reduced to formazan by live cells containing active mitochondria. The culture medium was replaced with 100 μl D/F without phenol red medium-BSA, and a 10-μl aliquot (0.3% WST-1, 0.2 mM 1-methoxy PMS in PBS, pH 7.4) was added to each well. The cells were then incubated for 4 h at 38°C. The absorbance (A) was read at 450 nm using a microplate reader (Bio-Rad, Hercules, CA; Model 450). Percentage of cytotoxicity was determined by subtracting the mean A of H2O2-treated wells (Atest) from the mean A of untreated wells (Acontrol) and then dividing by the mean A of untreated wells (Acontrol). The mean A of wells in the absence of the cells was subtracted from the mean A of all experimental wells. The percent cytotoxicity was calculated as 100 × (Acontrol – Atest)/(Acontrol).
Dose-dependent effect of PGF and H2O2 on SOD1mRNA expression at 2 h in vitro
To determine whether LECs were responsive to increased concentrations of PGF and H2O2 in the present culture system, LECs cultured in 24-well plates were incubated for 2 h with or without 0.1-10 μM PGF or 1–100 μM H2O2 (n=4 experiments). The cells were then collected and stored at −80° C for the analysis of SOD1 mRNA expression.
SOD1 protein and total SOD activity at 2 h and at 24 h in vitro
To examine whether SOD is differently regulated by PGF and H2O2 at the time of functional and structural luteolysis, LECs cultured in 75-cm2 culture flasks were incubated for 2 h (mimicking functional luteolysis) and 24 h (mimicking structural luteolysis) with or without PGF (1 μM) or H2O2 (10 μM). The samples were then used for analysis of SOD1 protein expression and total SOD activity (n=4 experiments). The concentrations of PGF and H2O2 were chosen based on the result of SOD1 mRNA expression in vitro, and the effect of H2O2 on cell viability
PGF production in vitro
To determine the dose-dependent effects of H2O2 on PGF production, LECs cultured in 24-well plates were exposed to H2O2 (1–100 μM) for 2 h or 24 h. After incubation, the conditioned media were collected in 1.5 ml tubes containing 5 μl of a stabilizer solution (0.3 M EDTA, 1% (w/v) acid acetyl salicylic, pH 7.3) and frozen at −30°C until the PGF assay (n=4 experiments).
Reverse transcript-PCR
Total RNA was prepared from the CL tissue or cultured bovine LECs using TRI reagent according to the manufacturer’s direction (TRI Reagent RNA isolation protocol, © 2008 Ambion, Inc). One microgram of total RNA of each sample was reverse transcribed using a SuperScript First-Strand Synthesis System for RT-PCR (11904–018; Invitrogen), and the reaction mixture was used in each PCR together with the appropriate oligonucleotide primer pairs. The primer for SOD and beta-actin (ACTB) were designed and characterized as described previously [
19]. Primer for SOD1 was: forward: AAGGCCGTCTGCGTGCTGAA; reverse: CAGGTCTCCAACATGCCTCT (accession No: M81129; product: 240 bp). Primer for ACTB was: Forward: CGGCATTCACGAAACTACC; Reverse: ATCAAGTCCTCGGCCACAC (accession No: AY141970; product: 536).
The RT-PCRs were conducted with the house-keeping gene ACTB as an internal standard. ACTB primer was added at the appropriate cycle number by the “primmer-dropping method” as described by Wong et al. [
20] with modification [
21]. The PCRs were carried out using TaKaRa Taq (R001A; Takara Bio Inc., Shiga, Japan) and a thermal cycler (iCycler; Bio-rad Laboratories, Hercules, CA, USA). The PCR conditions were as follow: activation of DNA polymerase for 20 sec at 95°C, annealing for 1 min at 60°C, and extension for 1 min at 70°C, follow by final extension for 5 min at 72°C. The number of cycles was 27 for SOD and 23 for ACTB. Two-fifths aliquot of each reaction mixture was electrophoresed on a 1.5% agarose gel containing ethidium bromide with a known standard (100-bp ladder, New England Biolabs Inc., Beverely, MA, USA; #N3231S) and photographed under ultraviolet illumination. The integrated density was determined by ImageJ software (Windows version of NIH Image,
http://rsb.info.nih.gov/nih-image/, National Institutes of Health). Relative density was quantified by normalization of the integrated density of each corresponding β-actin.
SOD1 protein expression
SOD1 protein expression in luteal tissue and in cultured bovine LECs was assessed by Western immunoblotting analysis. Tissues or cells were lysed in 150 μl lysis buffer (20 mM Tris–HCl, 150 mM NaCl, 1% Triton X-100 [Bio-Rad Laboratories], 10% glycerol [G7757; Sigma-Aldrich], Complete [11 697 498 001; Roche Diagnostics, Basel, Switzerland], pH 7.4). Protein concentrations in the lysates were determined by the method of Osnes et al. [
22], using BSA as a standard. The proteins were then solubilized in SDS gel-loading buffer (10% glycerol, 1% β-mercaptoethanol [137–06862; Wako Pure Chemical Industries, Ltd.], pH 6.8) and heated at 95°C for 10 min. Samples (50 μg protein) were electrophoresed on a 15% SDS-PAGE for 1.5 h at 30 mA. The separated proteins were electrophoretically transblotted to a 0.2-μM nitrocellulose membrane (LC2000; Invitrogen) at 300 mA V for 3 h in transfer buffer (25 mM Tris–HCl, 192 mM glycine, 20% methanol, pH 8.3). The membrane was washed in TBS-T (0.1% Tween 20 in TBS [25 mM Tris–HCl, 137 mM NaCl, pH 7.5]), incubated in blocking buffer (5% nonfat dry milk in TBS-T) for 1 h at room temperature, incubated at 4°C with a primary antibody specific to each protein (goat SOD1 polyclonal antibody [23 kDa; 1:500 in TBS-T, overnight; sc-8637; Santa Cruz Biotechnology, Santa Cruz, CA, USA] and mouse ACTB monoclonal antibody [internal standard, 42 kDa; 1:4000 in TBS-T, overnight; A2228; Sigma-Aldrich]). The membrane was washed three times for 5 min in TBS-T at room temperature, incubated with secondary antibody (SOD1 [1:10000 in TBS-T]: anti-goat Ig, HRP-linked whole antibody produced in donkey, sc-2020; Santa Cruz; ACTB [1:40000 in TBS-T]: anti-mouse Ig, HRP-linked whole antibody produced in sheep, NA931; Amersham Biosciences, Buckinghamshire, UK) for 1 h, and washed three times in TBS for 5 min at room temperature. The signal was detected by a ECL Western immunoblotting detection system (RPN2109; Amersham Biosciences). The intensity of the immunological reaction was estimated by measuring the optical density in the defined area by computerized densitometry using NIH Image (National Institutes of Health; Bethesda, MD, USA).
Total SOD activity assay
Total SOD activity was determined in CL tissues collected at 0, 0.5, 2, 12, and 24 h after PGF injection and in the LECs at the end of a 2-h or 24-h incubation period using SOD Assay Kit-WST (S311-08; Dojindo Laboratories, Kumamoto, Japan). Total SOD activity was calculated using a concurrently run SOD standard curve, and expressed as inhibition rate or percentage of control (raw data on total SOD activity was normalized based on protein concentrations, units per mg of cellular protein).
Determination of PGF concentration
The concentration of PGF in the culture medium was determined by enzyme immunoassay (EIA) as described previously [
18]. The PGF standard curve ranged from 15.625 to 4000 pg/ml, and the median effective dose (ED
50) of the assay was 250 pg/ml. The intra- and inter-assay coefficients of variation were 7.4 and 11.6%, respectively. The cross-reactivities of the antibody were 100% for PGF, 3.0% for PGD2, 1.1% for PGI, 0.15% for PGE2, and < 0.03% for PGA2. The DNA content, estimated using the spectrophotometric method by Labarca & Paigen [
23], was used to standardize the PGF concentrations.
Statistical analysis
Data of SOD1 mRNA, protein level and total SOD activity were obtained in four separate experiments. PGF concentration and cell viability were performed in triplicate samples for each experimental group of LECs or CL tissues (in vivo). The statistical significances of differences in the amounts of SOD1 mRNA, protein levels, total SOD activity, cell viability and differences in PGF concentrations were analyzed using two-way analysis of variance (ANOVA) with repeated-measures or one-way ANOVA followed by Fisher’s protected least-significant difference (PLSD) procedure as multiple comparison tests. All values were expressed as the mean ± SEM of four separate experiments. A level of P<0.05 was considered to be statistically significant.
Discussion
The present study demonstrated that administration of a luteolytic dose of PGF increased the expression of SOD1 in the CL tissue between 0.5 and 2 h post-treatment, but decreased at 24 h in vivo. Furthermore, in vitro studies examining the effects of PGF and H2O2 on SOD expression in LECs, showed a similar pattern with increased SOD at 2 h followed by an inhibition at 24 h. These results suggest that SOD is temporally regulated by PGF and ROS during luteolysis in cattle. The dose of H2O2 used in the present study to examine SOD1 protein and total SOD activity did not affect significantly the viability of LECs.
Previous in vivo studies in cows demonstrated that injection of a luteolytic dose of PGF induces a transient (1–2 h) increase in the partial pressure of oxygen (pO
2) in the ovarian venous blood [
11]. In addition, it has been shown that a functional PGF receptor (FPr) is present in bovine LECs, and that PGF acutely increased ROS production in these cells [
6]. Moreover, the rat CL produces significant amounts of ROS [
24] and increases ROS (H
2O
2) generating capacity within a few hours after injection of a luteolytic dose of PGF [
8,
9]. In the present study, PGF stimulated the expressions of
SOD1 mRNA, protein, and total SOD activity at 2 h in bovine CL tissue and LECs. The temporal pattern of SOD expression suggests a role for ROS and SOD during the beginning functional luteolysis in cows. On the other hand, SOD acts as an antioxidant enzyme, and together with catalase, protects the endothelium of a variety of tissues against ROS [
25]. Taken together, SOD and ROS seem to be involved in the luteolytic cascade induced by PGF in bovine CL.
ROS have been implicated in luteolysis due to their ability to increase uterine PGF [
10], to decrease P
4 biosynthesis [
15] and to induce apoptosis in LSCs [
26]. The intraluteal production of ROS is regulated by SOD [
15]. SOD catalyzes the dismutation of superoxide into oxygen and H
2O
2[
12]. SOD1 inhibition increases the steady-state levels of superoxide [
27]. On the other hand, the presence of superoxide anions can induce intracellular SOD1. In the present study, H
2O
2 stimulated the expressions and activity of SOD1 at 2 h in bovine LECs. Sander et al. demonstrated an increase in total SOD activity and a decrease in catalase activity during CL regression in mice [
28]. Since H
2O
2 has the capacity to increase PGF production in bovine LSCs [
29] and LECs (the present study), as well as to induce apoptosis in bovine LSCs and human umbilical vein endothelial cells [
29,
30], increased levels of H
2O
2 may be crucial for luteal regression. The above findings also suggest that a local increase of ROS within the bovine CL facilitates the local production of PGF. Moreover, the concomitant increase of SOD and ROS may be due to the strong stimulatory effect of ROS on SOD in response to the increasing levels of PGF within the CL.
Although luteolytic PGF is derived from the uterus in many species, including ewes [
31] and cows [
2], a considerable amount of PGF is also synthesized by the CL [
32] and LECs represent an important source of PGF [
18]. Previous studies have reported that PGF increases the production of ROS in rats [
9,
24] and cow in vivo [
11]. Interestingly, ROS has been demonstrated to stimulate PGF production in the CL of rats [
33], cows [
29] and human [
10]. In the present study, H
2O
2 stimulated PGF production in cultured bovine LECs. The above results suggest the presence of a positive feedback loop between PGF and ROS in the bovine CL during luteolysis. Also, the increase of intraluteal PGF induced by ROS seems to be crucial for promotion of luteal regression in cow.
The present study demonstrates that PGF and H
2O
2 inhibited the expression of SOD1 protein in bovine LECs cultured for 24 h. The inhibitory effects of PGF and H
2O
2 on SOD expression at 24 h contrasted with their stimulatory effects at 2 h. The increase in SOD observed at 2 h seems to be the result of an acute stimulatory effect of PGF on ROS production by LECs. However, the mechanism by which PGF and H
2O
2 inhibit the expression of SOD1 at 24 h of incubation is unclear. SOD catalyzes the dismutation of superoxide into H
2O
2 and oxygen, to maintain low-state levels of superoxide [
12]. Therefore, a reduction of SOD by PGF and H
2O
2 at 24 h may enhance intraluteal ROS or superoxide radical accumulation for the promotion of structural luteolysis [
29,
30]. In support of such an idea, an accumulation of superoxide radicals and a decrease in SOD levels are associated with the inhibition of luteal P
4 secretion [
7] and apoptotic cell death [
34].
Furthermore, SOD1 protein was localized in LECs (Additional file
1: Figure S1) and other types of luteal cells (Additional file
2: Figure S2). A robust SOD1 protein expression was detected in bovine CL tissue after PGF treatment (Additional file
2: Figure S2). These findings suggest that not only SOD1 in LECs but also in other types of luteal cells including LSCs are regulated during PGF induced luteolysis. Further studies are needed to clarify the relative contribution of LSCs in total luteal SOD during luteolysis in cow.
Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
HVV participated in the in vitro experiments and drafted the manuscript. TJA conceived of the study, participated in its design and performed in vivo and in vitro experiments. He also helped to draft the manuscript. ShY participated in data analysis and drafted the manuscript. HA carried out the in vitro experiments. KO participated in experimental design and discussion. All authors read and approved the final manuscript.