Expression localisation and functional activity of pituitary adenylate cyclase-activating polypeptide, vasoactive intestinal polypeptide and their receptors in mouse ovary

Animals

Immature CD1 mice (Charles River, Como, Italy) were housed under controlled temperature (25 °C) and light (12 h light/day) conditions with ad libitum access to food and water. Animals were maintained in accordance with the Italian Department of Health Guide for Care and Use of Laboratory Animals. Experimental protocols were approved by the ‘La Sapienza’ University Committee for Animal Care and Use. Mice were killed by cervical dislocation. Twenty-two-day-old immature mice were either killed or injected i.p. with 7 i.u. equine chorionic gonadotrophin (eCG, Intervet, Milan, Italy) to enhance multiple follicular development. After 46–48 h, the animals were killed, or injected with 5 i.u. human chorionic gonadotrophin (hCG, Intervet) and killed at different times after injection.

Tissue and cell isolation

Ovaries were removed aseptically and freed from adherent tissues in Hank’s balanced salt solution (HBSS, Gibco, Invitrogen). Whole ovaries were processed immediately for RNA or protein isolation.

Granulosa cells (GC) were obtained as described previously (Vaccari et al. 2006). Briefly, the largest follicles from each ovary were punctured with a 25-gauge needle and gently pressed to release GC. Cells were centrifuged at 250 g for 5 min and either resuspended in lysis buffer for RNA extraction or cultured at a density of 1.5 × 10⁵/200 μl in Dulbecco’s modified Eagle medium (DMEM, Gibco, Invitrogen) supplemented with 1 mg/ml BSA, 2 mM glutamine and antibiotics (100 mM penicillin, 100 μg/ml streptomycin). The residual ovarian tissue, mainly theca/interstitial cells and granulosa cells from small preantral follicles, was homogenised in lysis buffer for RNA extraction.

Preovulatory follicles were isolated from ovaries collected 46–48 h after eCG injection in HBSS supplemented with 1 mg/ml BSA and cultured as described previously (Lee et al. 1999). Briefly, four follicles were cultured in polypropylene culture tubes containing 500 μl DMEM supplemented with 2 mM glutamine and antibiotics (penicillin, streptomycin) and 1 mg/ml BSA in the absence or presence of 100 ng/ml luteinising hormone (LH), or increasing concentrations of PACAP or VIP (10⁻⁹–10⁻⁷ M; Calbiochem/Merck Darmstadt).

In additional experiments, follicles were incubated with 10⁻⁷ M PACAP or VIP in the presence of 5 × 10⁻⁷ M PACAP and VIP antagonists, which were PACAP-38 (6–38) trifluoroacetate salt, the hybrid of neurotensin (6–11) and VIP (7–28; Bachem AG, Bubendorf, Switzerland), and the VIP receptor antagonist (d-P-chloro-Phe6,Leu17)-VIP (Sigma–Aldrich).

Morphological analysis of granulosa cell apoptosis

To evaluate the effect of PACAP and VIP on granulosa cell apoptosis, follicles were mechanically dissected from eCG-treated mice and GCs were released in the medium immediately before or after 24 h of follicle culture. Cells from single follicles were fixed for 15 min in 3% (w/v) paraformaldehyde/PBS and cytocentrifuged onto a glass slide at 200 g for 10 min. The samples were washed thrice with PBS and the chromatin was stained using the TUNEL (TdT-mediated dUTP-X nick end labelling) method according to the manufacturer’s instructions (Mebstain Apoptosis Kit Direct, MBL International, Woburn, MA, USA). Apoptotic cells were identified and counted in three or more randomly selected fields with at least 100 cells each.

RNA extraction and RT

Total RNA from whole ovaries, GC and residual ovarian tissue was isolated by a silica gel-based membrane spin column (RNeasy Kit, Qiagen S.p.A.). The purity and integrity of the RNA was checked spectroscopically and by gel electrophoresis. Total RNA (1 μg) was reverse-transcribed in a final volume of 20 μl, using the M-MLV Reverse Transcriptase kit (Invitrogen) according to the manufacturer’s instructions.

Multiplex PCR

To determine the presence of PACAP and its receptor transcripts, a duplex-touchdown-PCR was performed. The reactions were carried out using a Multiplex PCR Kit (Qiagen) according to the manufacturer’s instruction, with the housekeeping gene β-actin as internal control. To increase the specificity and the quality of target products, a touchdown PCR was performed. The initially high annealing temperature (T_a, 67 °C for PACAP and all the receptors, and 62 °C for VIP) was lowered by 1 °C per cycle to a ‘touchdown’ temperature of 59 °C for PACAP and all the receptors and 55 °C for VIP. This ‘touchdown’ temperature remained the same for the remaining 22 cycles. The primer sequences chosen are shown in Table 1. Each primer pair was previously tested alone for specific amplification. Primers for PAC1-R were chosen in a region that allowed the detection of all splice variants. For each sample, 10 μl PCR product was then subjected to electrophoresis on 2% (w/v) agarose gel and stained with ethidium bromide. The densitometric evaluation of the bands was performed with AIDA software (Advanced Image Data Analyzer 2.11 raytest GmbH, Straubenhartd, Germany). The relative mRNA levels were normalised against the expression of the housekeeping gene. The β-actin primer set 1 was used for the normalisation of PACAP, VIP, PAC1-R and VPAC2-R mRNA levels, while the β-actin primer set 2 was used for VPAC1-R. DNA contamination controls were performed using gene-specific primers on RNA without reverse transcriptase treatment. PCR products were sequenced to verify the specificity of amplified DNA.

Analysis of PAC1-R isoforms

To identify the PAC1-R splice variants present in the ovary, specific primer pairs (Table 1) were designed on the basis of the analysis of the PAC1-R mouse mRNA sequence obtained from NCBI GenBank. The forward (Fw) and reverse (Rv) hip/hop primers, which flanked the site of insertion of the hip/hop cassette region, were used to amplify all the isoforms in this region, whereas the hop-Rv-specific primer was located inside the hop cassette (Fig. 1). RT-PCR was performed with a T_a of 57 °C for 30 cycles. Following amplification, PCR products were purified with the SureClean Kit (Bioline GmbH, Luckenwalde, Germany). Twenty microlitres of each purified cDNA were digested with PvuII and/or AvaI restriction enzymes (Promega) for 4 h at 37 °C and the products of digestion were visualised by electrophoresis on 2% (w/v) agarose gel.

Immunofluorescence

Freshly isolated ovaries from eCG- and hCG-stimulated mice were embedded in optimal tissue freezing medium (TBS, Duram, NC, USA), snap-frozen in liquid nitrogen and stored at 380 °C until being sectioned with a Leitz cryostat. Sections (7 μm) were fixed in 4% paraformaldehyde and permeabilised with 0.1% (v/v) Triton X-100. The sections were blocked for 3 h in 10% (v/v) normal goat serum (Sigma–Aldrich) to minimise non-specific binding, and incubated overnight at 4 °C with 1:1000 rabbit polyclonal anti-PACAP antiserum (kindly provided by Dr A Arimura; Koves et al. 1990). The sections were then incubated for 1 h at RT with 1:1000 Alexa Fluor 488-conjugated mouse anti-rabbit secondary antibody (Molecular Probes, Invitrogen) and observed under a fluorescence microscope. In control samples, the primary antibody was substituted with rabbit pre-immune serum.

In situ hybridisation histochemistry

Freshly isolated ovaries from eCG- and hCG-stimulated mice were fixed in Bouin’s fluid for 48 h at room temperature. Fixed ovarian tissue was embedded in paraffin and sectioned at 7 μm. Paraffin sections were mounted on microscope polylysine slides (Menzel-Glaser, Braunschweig, Germany), deparaffined and rehydrated. Slides were then post-fixed in 4% para-formaldehyde for 10 min at room temperature, and treated with 10 μg/ml proteinase K (Roche Diagnostics S.p.A.). Hybridisation was carried out overnight at 55 °C in a humidified chamber in a mixture containing 50% (v/v) formamide, 1 × standard sodium citrate (SSC), 1 × Denhardt’s solution, 10% (w/v) dextran sulphate, 200 mg/ml salmon sperm DNA and 300 ng/ml digoxigenin-labelled DNA PACAP probe. The probe was labelled by direct incorporation of DIG-dUTP (Roche Diagnostics) during PCR amplification performed with the same primers as those used to amplify PACAP in multiplex RT-PCR (PAC1-R, see Table 1). After hybridisation, washings were performed under stringent conditions to a final concentration of 0.1% (v/v) SSC. Sections were then incubated in blocking solution (100 mM Tris–HCl (pH 7.5), 100 mM NaCl, 2 mM MgCl₂, 1% (w/v) BSA) and in 1:300 alkaline phosphatase-conjugated anti-digoxigenin antibody (Roche Diagnostics) diluted in blocking solution. Colorimetric detection was developed with a chromogen substrate (NBT, BCIP; Roche Diagnostics). The sections were observed by light microscopy and not counterstained.

A digoxigenin-labelled β-actin DNA probe was used as a positive control, whereas an unlabelled PACAP DNA probe, as well as competing hybridisations, with different mixtures (1:5 and 1:10) of digoxigenin-labelled/-unlabelled PACAP DNA probes, were used as negative and specificity control reactions.

Western blot analysis

Ovaries from untreated 22-day-old immature mice or from eCG-treated mice were lysed with RIPA buffer (10 mM Tris (pH 7.2), 150 mM NaCl, 1% (v/v) Triton X-100, 1% (w/v) sodium deoxycholate, 0.1% (w/v) SDS, 5 mM EDTA) containing protease inhibitors (Sigma–Aldrich) and sonicated on ice. The sonicated tissue was centrifuged for 2 min at 15 000 g at 4 °C and the supernatant was stored at −20 °C until use. Protein concentration was measured by BCA protein assay (Pierce Biotechnology, Rockford, IL, USA). ~50 μg proteins were subjected to SDS-PAGE under denaturing conditions on a 12% (w/v) acrylamide gel (Laemmli 1970) and transferred onto a nitrocellulose membrane (Schleicher & Schuell, Whatman GmbH, Dassel, Germany). Non-specific binding was blocked by incubation with 5% (w/v) low-fat dry milk and 0.3% (v/v) tween-20 in PBS calcium-magnesium-free (CMF). The membrane was then incubated overnight at 4 °C with rabbit anti-VPAC1-R polyclonal antibody (1:200, sc-30019; Santa Cruz Biotechnology, Heidelberg, Germany) and with a mouse monoclonal antibody anti-tubulin (1:1000, T5168, Sigma–Aldrich) in CMF added with 5% (w/v) low-fat dry milk. The membrane was washed thrice with CMF for 20 min at room temperature and then incubated with the AP-conjugated secondary anti-rabbit antibody (1:2000, Zymed, San Francisco, CA, USA) for 1 h at room temperature or anti-mouse biotinilated antibody (1:5000; Dako Italia S.p.A. Milano, Italy) followed by incubation with streptavidin–AP complex (1:1000, Dako) at room temperature for 1 h. After washing with washing buffer (0.1 M Tris (pH 9.5), 0.1 M NaCl), immunocomplexes were detected by western blot chemiluminescence reagent (CDP-star; NEN, Boston, MA, USA), following the manufacturer’s instructions. Molecular masses were measured by prestained molecular markers (Gibco).

Statistical analysis

Data are expressed as the mean ± s.e.m. from at least three independent experiments. Statistical analysis was performed using ANOVA followed by the Tukey–Kramer test for comparisons of multiple groups. Values with P<0.05 were considered statistically significant.

Expression of PACAP

To verify the presence of PACAP transcripts and characterise their expression pattern following gonadotrophin stimulation, total RNA was extracted from ovaries obtained from 14- and 22-day-old untreated mice, eCG-primed or eCG/hCG-primed mice. Furthermore, the level of specific mRNAs was assessed by multiplex RT-PCR.

Our data did not show PACAP expression in 14-day-old ovaries (data not shown), in untreated (22d) or eCG-treated whole ovaries from 22-day-old animals; PACAP expression was transiently induced by hCG treatment, when it became detectable after 1 h, reached a maximum level after 3–6 h, and decreased to unstimulated levels after 9 h (Fig. 2A). VIP transcripts were never observed at the time points considered (data not shown).

To investigate the expression of PACAP in the different ovarian compartments, RNA was extracted from isolated GCs and residual ovarian tissue (TI cells) obtained from ovaries of 22-day-old untreated, eCG- and hCG-treated mice. As shown in Fig. 2B, the expression pattern of PACAP transcripts in isolated GCs mimicked that of whole ovary, with no expression before hCG treatment and transient expression between 1 and 6 h after gonadotrophin stimulation. Residual ovarian tissue displayed very low overall PACAP expression, which slightly, though significantly, increased after hCG injection (Fig. 2C), thus suggesting that, following gonadotrophin stimulation, PACAP was predominantly expressed in GCs.

Localisation of PACAP

To determine the cell type that expresses PACAP mRNA, in situ hybridisation histochemistry was performed on ovarian sections obtained from mice before and 6 h after hCG injection. The PACAP signal was absent in ovaries of eCG-treated mice (Fig. 3B); it was instead detected mainly in GCs of large preovulatory follicles after gonadotrophin stimulation (Fig. 3C). PACAP immuno-reactivity was very low in the ovaries of eCG-treated animals (Fig. 4A), whereas was observed in GCs and cumulus cells of preovulatory follicles 6 h after hCG stimulation (Fig. 4B).

In vitro stimulation of PACAP

Granulosa cells, isolated from preovulatory follicles obtained from eCG-treated mice, were incubated for 6 h in medium alone (C), or in the presence of 100 ng/ml follicle-stimulating hormone (FSH) or LH. At the end of the culture, cells were processed for RNA extraction and the presence of PACAP was assessed by semiquantitative RT-PCR. The expression levels of PACAP were compared with those attained in vivo by granulosa cells 6 h after hCG injection. After gonadotrophin stimulation, we observed a significant increase in PACAP mRNA, which reached levels that were slightly, though not significantly, lower than those obtained after in vivo stimulation (Fig. 5).

Expression of PAC1 receptor

To characterise the expression of PAC1-R in mouse ovary, total RNA was extracted from whole ovaries, isolated granulosa cells and residual ovarian tissues, as described above. Using the primer pair common to all splice variants of the receptor, located at the 5′-end of the PAC1-R mRNA (PAC1R-Fw, PAC1R-Rv; see Fig. 1 and Table 1), we detected two different products. In addition to the expected 317 bp fragment, we observed a fragment of 254 bp generated by the alternative splicing of the exon encoding a 21-aa domain in the N-terminal extracellular region of PAC1-R (Pantaloni et al. 1996; Fig. 6). The expression analysis of PAC1-R mRNA in whole ovaries shows that it is already present before gonadotrophin stimulation and is transiently stimulated between 3 and 6 h after hCG injection (Fig. 6A). When the GC population was analysed separately, we observed a similar pattern of expression, with an induction of PAC1-R-mRNA after hCG stimulation (Fig. 6B). In the residual ovarian tissues obtained from unstimulated animals, we observed a level of expression of PAC1-R mRNA similar to that observed in GCs but no modulation by gonadotrophin (data not shown).

To test whether the aforementioned different splice variants were present in mouse preovulatory ovary, we performed RT-PCR on RNA extracted from whole ovaries 3 h after hCG injection (ov) with primers flanking the site of insertion of the hip/hop cassettes (hip/hop-Fw, hip/hop-Rv; Fig. 1 and Table 1). This primer pair gave rise to two amplification products corresponding to the 181 bp PAC1-R short isoform, with neither hip nor hop exons, and a 265 bp with only one hip or hop cassette, or a mixture of the two isoforms (Fig. 7, lane a). Both isoforms were induced by hCG treatment (data not shown). Mouse brain, used as a positive control, expressed the same splice variants as those detected in ovary (Fig. 7, lane c).

Since there is no mouse hip sequence in NCBI GenBank, in order to test the presence of the hip cassette in the mouse ovary, we based our analysis on the high homology (93%) of the mouse PAC1-R with the rat gene. In rat, the hip sequence is cleaved by the AvaI restriction enzyme. When we digested the amplified products obtained with the hip/hop primer pair, we did not observe any cleavage fragments (data not shown). Amplification with the hip/hop-Fw and hop-Rv (within the hop cassette, Fig. 1) primer pair resulted in only one product at 148 bp (Fig. 7, lanes b and d), confirming the presence of the hop1/hop2 isoforms and the absence of the hip isoform in both ovary and brain.

In order to distinguish between the hop1 and 2 isoforms, we exploited the nucleotide triplet insertion at the 5′-end of the hop1 exon, which generates a recognition site for the restriction enzyme PvuII. After complete digestion of the PCR products obtained with the hip/hop primers, the 181 bp band remained unchanged, while we observed digestion of the 265 bp band, accompanied by the appearance of two shorter fragments (Fig. 7, lanes e and g) of 117 and 148 bp, which thus confirmed the presence of the hop1 isoform. The incomplete digestion of the 265 bp band suggested the contemporary presence of the hop2 isoform. Similar conclusions were drawn when the product obtained with the hip/hop-Fw and hop-Rv primers was digested with PvuII. The 148 bp band was partially digested and a 117 bp band appeared (Fig. 7, lanes f and h).

Expression of VIP receptors

Analysis of VPAC1-R mRNA in whole ovary showed that the transcripts were present in untreated 22-day-old immature animals (22d) and were significantly down-regulated after gonadotrophin stimulation. VPAC1-R mRNA decreased after eCG stimulation and almost disappeared after hCG stimulation (Fig. 8). VPAC1-R was predominantly expressed in the residual ovarian tissue, in which it decreased markedly after gonadotrophin stimulation, whereas in GCs it was constantly present at very low levels (Fig. 9).

VPAC2-R expression slightly increased between 1 and 9 h following hCG stimulation in both whole ovary (Fig. 10) and the various cell populations considered separately (data not shown).

Evaluation of receptor activity

To determine the presence of functional receptors and ascertain which receptor is physiologically active in the preovulatory follicle, we studied the effects of PACAP and VIP on GC apoptosis. Follicles obtained from eCG-treated animals were cultured for 24 h in the absence of serum and in the presence of increasing concentrations of PACAP and VIP (from 10⁻⁹ to 10⁻⁷ M). At the end of the culture, GCs were mechanically isolated by puncturing the large antral follicles and were stained with TUNEL to assess the presence of apoptotic cells. GCs obtained from follicles immediately after isolation displayed very weak signs of apoptosis (2 ± 0.5%). In GCs obtained from follicles incubated in serum-free medium for 24 h, apoptosis increased to 61.2 ± 5.2%, with PACAP and VIP proving equally effective in preventing GC apoptosis (Fig. 11). To further determine the contribution of the different receptor subtypes to this inhibitory effect, follicles were incubated with 10⁻⁷ M PACAP or VIP in the presence of 5 × 10⁻⁷ M PACAP/VIP receptor antagonists. The antagonists used were: PACAP (6–38; P1), a PAC1-R and, to a lesser degree, VPAC2-R selective antagonist, (d-P-chloro-Phe6,Leu17)-VIP (V1), a moderately potent VPAC1-R antagonist and a hybrid of neurotensin (6–11), and VIP (7–28; P1/V2), a moderately potent PAC1-R antagonist and a weak VPAC2-R antagonist (Dickinson et al. 1997). All the receptor antagonists significantly reverted PACAP action, with P1 proving the most effective, though only V1 and P1/V2 inhibited VIP action, thereby supporting the presence of all three receptor subtypes in the follicle.

Western blot of VPAC1-R

Although VPAC1-R mRNA significantly decreased after gonadotrophin stimulation, the VPAC1-R antagonist nonetheless inhibited PACAP and VIP action on GC apoptosis (Fig. 12). Therefore, we investigated by western blot the presence of this receptor in whole ovary. As shown in Fig. 13, VPAC1-R was present in untreated 22-day-old immature animals and was still present at similar levels after eCG stimulation. The heterogeneity in molecular mass observed for VPAC1-R was probably due to differences in levels of glycosylation, as demonstrated in other human tissues (Bajo et al. 2000).