Temporal expression and signalling of prostacyclin receptor in the human endometrium across the menstrual cycle

doi:10.1530/rep.1.00038

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Temporal expression and signalling of prostacyclin receptor in the human endometrium across the menstrual cycle

S Battersby, H O D Critchley¹, A J de Brum-Fernandes² and H N Jabbour

MRC Human Reproductive Sciences Unit and ¹ Department of Reproductive and Developmental Sciences, Centre for Reproductive Biology, University of Edinburgh Chancellor’s Building, 49 Little France Crescent, Old Dalkeith Road, Edinburgh EH16 4SB, UK and ² Rheumatic Diseases Unit, Centre Universitaire de Santé de l’Estrie, 3001-12 Avenue Nord, Fleurimont, PQ, Canada J1H 5N4

Correspondence should be addressed to H N Jabbour; Email: h.jabbour{at}hrsu.mrc.ac.uk

Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

Prostacyclin (PGI₂) synthesis and function in the human uterushas been implicated in the regulation of the process of normaland dysfunctional menstruation. PGI₂ synthesis is elevated duringnormal menstruation and is also associated with blood loss inwomen who suffer from heavy menses. This study was designedto outline further the role of PGI₂ in menstruation by investigatingthe temporal pattern and site of expression of prostaglandinI synthase (PGIS) and the prostacyclin receptor (IP receptor)in the non-pregnant human endometrium across the menstrual cycle.Quantitative RT-PCR demonstrated increased expression of PGISand IP receptor during the menstrual phase of the cycle comparedwith all other phases (P < 0.05). Furthermore, PGIS and IPreceptor were localised to the glandular epithelium, stromaland endothelial cells in the basal and functional layers ofthe endometrium. Functionality of the IP receptor in the humanendometrium was assessed by measuring cAMP generation followingtreatment with 100 nmol l^-1 of the PGI₂ analogue, iloprost.cAMP generation was significantly higher in endometrial tissuecollected during the proliferative compared with the secretoryphase of the menstrual cycle (P < 0.05).

In conclusion, this study has confirmed increased expressionand signalling of PGIS and IP receptor during the menstrualphase and outlines a potential autocrine/paracrine role forPGI₂ on several cellular compartments in the endometrium includingthe endothelium. This may underscore a pivotal role for PGI₂receptor signalling in normal and dysfunctional menstruation.

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

Prostacyclin (PGI₂) is a member of the prostanoid family oflipid mediators and is the main prostanoid synthesised by vascularendothelium (Smyth & FitzGerald 2002). Cyclooxygenase (COX)enzyme is the key enzyme in the synthesis of PGI₂ from arachidonicacid via the common intermediate in prostaglandin (PG) synthesis,PGH₂. In turn, PGH₂ is rapidly converted to PGI₂ by the actionof prostaglandin I synthase (PGIS) (Kniss 1999). There are twopredominant isoforms of COX enzymes, COX-1, which is constitutivelyexpressed in many cell types and COX-2, which is induced byfactors including cytokines and tumour promoters (Kniss 1999).PGI₂ elicits its effects on target cells by interaction withits G protein-coupled receptor (IP receptor), which has a typicalseven-trans-membrane structure (Narumiya et al. 1999). The IPreceptor can stimulate both G_s and G_q species of G proteinscausing an increase in cAMP generation and in phosphatidylinositolresponse (Narumiya et al. 1999).

Temporal expression of other prostaglandins such as PGE₂ andPGF₂and their receptors (EP2/EP4 and FP receptors) has beendemonstrated in the human endometrium and has been shown tovary with the phase of the menstrual cycle (Lumsden et al. 1986,Smith & Kelly 1988, Milne et al. 2001, Milne & Jabbour 2003).Maximal expression and signalling of these receptorsare detected during the mid-late proliferative phase of themenstrual cycle. Recent data implicate a role for PGE₂ and PGF₂inthe proliferation of glandular epithelial cells via diversesignalling pathways (Jabbour & Boddy 2003, Milne & Jabbour 2003).In contrast, little is known of the expression patternand function of the IP receptor in human endometrium, althoughPGIS and IP receptor expression have been demonstrated in pregnantand non-pregnant myometrium (Moonen et al. 1986, Chegini & Rao 1988,Giannoulias et al. 2002).

PGI₂ is the main prostanoid synthesised by the vascular endotheliumand it causes blood vessel dilatation and inhibition of plateletaggregation (Smyth & FitzGerald 2002). Moreover, PGI₂ isknown to act as a smooth muscle relaxant (Wilhelmsson et al. 1981,Lumsden & Baird 1986, Dyal & Crankshaw 1988).The effects of PGI₂ on platelet aggregation and vascular tonehave outlined its potential role in menstruation (Baird et al. 1996).This is supported by observations of elevated PGI₂ levelsin uterine venous blood during menstruation as compared withother phases of the menstrual cycle (Goodfellow et al. 1982).Moreover, PGI₂ synthesis is increased in women suffering fromheavy menses compared with those who show normal blood loss(Smith et al. 1981b, Makarainen & Ylikorkala 1986, Cameron et al. 1987).It has also been suggested that menstrual disorderscan be the result of a shift in the ratio of different prostaglandins.Heavy menses has been associated with increased synthesis ofPGI₂ relative to thromboxane A₂ and PGE₂ relative to PGF₂(Smith et al. 1981a,Makarainen & Ylikorkala 1986). Heavy menseswith no known uterine pathology affects 10% of women of childbearing age and is defined as blood loss in excess of 80 mlper menstrual cycle (Prentice 2000).

The objectives of the present study were to investigate theexpression of PGIS (the terminal enzyme responsible for thegeneration of PGI₂) and IP receptor in non-pregnant human endometriumand myometrium across the menstrual cycle. Furthermore, therole of PGI₂ in endometrial cell signalling has been assessedby investigating the effect of the PGI₂ analogue, iloprost,on cAMP generation. A better understanding of IP receptor signallingand function in the human endometrium may ultimately lead tothe development of novel therapies in the treatment of menstrualdisorders that may be associated with elevated PGI₂ synthesis.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

Patients and tissue collection
Endometrial biopsies at different stages of the menstrual cyclewere obtained from women with regular menstrual cycles (25–35days), who had not received a hormonal preparation in the 3months preceding biopsy collection. Samples were collected eitherwith an endometrial suction curette (Pipelle, Laboratoire CCD,Paris, France) or as full thickness endometrial biopsies (includingthe functional layer and basal-myometrial junction) from womenundergoing hysterectomy for benign gynaecological indications.Shortly after collection, tissue was either snap frozen in dryice and stored at -70 °C (for RNA extraction), fixed inneutral buffered formalin (NBF) and wax embedded (for immunohistochemicalanalyses), or placed in RPMI 1640 (containing 2 mmol l^-1 L-glutamine,100 U penicillin and 100 µg ml^-1 streptomycin) and transportedto the laboratory for in vitro culture.

Biopsies were classified within a 28-day cycle range using statedlast menstrual period (LMP) and histological assessment accordingto the criteria of Noyes and co-workers (1975). Furthermore,circulating oestradiol and progesterone concentrations at thetime of biopsy were consistent for both stated LMP and histologicalassignment of menstrual cycle stage. Samples were divided accordingto the phase of the menstrual cycle as: menstrual (days 1–4),early to mid proliferative (EP-MP; days 5–10), late proliferativeto ovulatory (LP-Ov; days 11–14), early secretory (ES;days 15–18) and mid to late secretory (MS-LS; days 19–28).Ethical approval was obtained from the Lothian Research EthicsCommittee and written informed consent was obtained from allsubjects before tissue collection.

Taqman quantitative RT-PCR
RNA was extracted from endometrial biopsies obtained from acrossthe menstrual cycle (n = 35) using Tri Reagent (Sigma, Poole,Dorset, UK) following the manufacturer’s instructions.RNA samples were quantified and were reverse transcribed using5.5 mmol l^-1 MgCl₂, 0.5 mmol l^-1 of each deoxynucleotide triphosphate(dNTP), 2.5 µmol l^-1 random hexamers, ribonuclease inhibitor(0.4 U µl^-1) and 1.25 U µl^-1 Multiscribe reversetranscriptase (all from Applied Biosystems, Warrington, Cheshire,UK). RNA (400 ng) was added to each reverse transcription reactionand samples were incubated for 90 min at 25 °C, 45 min at48 °C and 5 min at 95 °C. The reaction mix for the PCRconsisted of 1 x mastermix, ribosomal 18S forward and reverseprimers, ribosomal 18S probe (50 nmol l^-1; all from AppliedBiosystems), forward and reverse primers for PGIS or IP receptor(300 nmol l^-1) and PGIS or IP receptor probe (200 nmol l^-1)(all from Biosource UK, Nivelles, Belgium). The reaction mix(48 µl) was aliquoted into tubes and 2 µl cDNA wereadded. Duplicate 24 µl samples plus positive and negativecontrols were placed in a PCR plate and wells were sealed withoptical caps. The PCR reactions were carried out using an ABIPrism 7700 (Applied Biosystems). All primers and probes weredesigned using the PRIMER express program (Applied Bio-systems).The sequences of PGIS primers and probe were: PGIS forward primer,5'-ACGCAGATGTGGAGATCCCT-3'; reverse, 5'-GTCGTGTTCCGGCTGCA-3';and probe (6-carboxy fluoroscein labelled) 5'-CCTCAGCAGGTACGGCTT-CGGTCTG-3'.The sequences of the IP receptor primers and probe were: IPreceptor forward primer, 5'-GCCCTC-CCCCTCTACCAA-3'; reverse,5'-TTTTCCAATAACTGTGG-TTTTTGTG-3'; and probe (6-carboxy fluorosceinlabelled) 5'-CCAAGAGCCAGCCCCCTTTCTGC-3'. The sequences of 18Sprimers and probe have been described previously (Milne et al. 2001).Data were analysed and processed using Sequence Detectorversion 1.6.3 (Applied Biosystems) according to the manufacturer’sinstructions. Results were expressed relative to an internalpositive standard (cDNA obtained from a single sample of endometrialtissue) included in all reactions.

In situ hybridisation
A custom synthesised oligonucleotide double fluoroscein isothiocyanate(FITC)-labelled cDNA probe for IP receptor was obtained fromBiognostik (Göttingen, Germany). Sections (5 µm)from full thickness human endometrial biopsies collected acrossthe menstrual cycle (n = 12) were cut onto gelatin-coated slides.Sections were dewaxed and rehydrated and then treated with proteinaseK (50 µg ml^-1 in 100 mmol l^-1 Tris–HCl pH 7.6, containing50 mmol l^-1 EDTA) for 15 min at 37 °C to enhance cDNA probeaccess. Sections were washed in diethylpyrocarbonate-treatedwater and prehybridised for 4 h at 30 °C with 25 µlof the hybridisation buffer supplied with the probe, which hadpreviously been heated to 95 °C. The sections were thenhybridised overnight at 30 °C with the cDNA probe at 6 Uµl^-1 in hybridisation buffer. Following hybridisation,sections were washed for 2 x 5 min in 1 x SSC at room temperatureand 2 x 15 min in 0.1 x SSC at 39 °C. After rinsing in trisbuffered saline (TBS), endogenous peroxidase activity was quenchedwith 10% (v/v) H₂O₂ in methanol at room temperature. The FITC-labelledprobe was detected using standard immunohistochemical reagentswith an additional amplification step (TSA Biotin System, NENLife Science Products, Hounslow, Middlesex, UK). Sections wereincubated with blocking buffer for 30 min. Conjugated anti-FITC-horseradishperoxidase (Roche, Diagnostics Ltd, Lewes, E Sussex, UK) wasadded at a dilution of 1 in 200 in blocking buffer and the sectionswere incubated for 30 min. After washing, biotinyl tyramideamplification reagent (1 in 50) was applied to each slide andincubated for 15 min. Strep-tavidin-horseradish peroxidase (1in 100) was applied after washing and incubated for 30 min;probe localisation was visualised with 3,3'-diaminobenzidine(DAB) substrate. Control sections were treated with a doubleFITC-labelled oligonucleotide probe containing the same proportionof cysteine (C) and guanine (G) bases as the IP receptor probeto assess background hybridisation. All treatments were carriedout at room temperature unless otherwise specified.

Immunohistochemistry
Endometrial sections (5 µm) from across the menstrualcycle (n = 12) were dewaxed in xylene and rehydrated using decreasinggrades of ethanol. Antigen retrieval was performed by treatingsections for 5 min in a pressure cooker in boiling 0.1% citratebuffer, pH 3.0. Endogenous peroxidase activity was quenchedwith 10% (v/v) H₂O₂ in methanol at room temperature. Non-immuneswine serum (20% serum in TBS) was applied for 1 h before overnightincubation at 4 °C with rabbit anti-human IP receptor ata dilution of 1 in 500 or rabbit anti-bovine PGIS (shown tocross-react with human PGIS) (Alexis Corporation, Nottingham,UK) at the same concentration. An avidin-biotin peroxidase detectionsystem was then applied (DAKO Ltd, Cambridge, UK) with DAB asthe chromagen. The antibody to IP receptor has been describedpreviously (Fortier et al. 2001). Non-immune rabbit serum andantibody pre-absorbed with IP receptor peptide were used ascontrols for IP receptor, and non-immune rabbit serum was usedas a control for PGIS. Immunoreactivity was negligible withpre-absorbed antibody, and with non-immune rabbit serum therewas occasional generalised pale brown cross reactivity overthe epithelial glands and the endothelium.

Cyclic AMP assay
Endometrial biopsies from the proliferative and secretory phasesof the menstrual cycle (n = 8) were minced finely with scissorsand divided into three portions. The tissue was incubated overnightat 37 °C in a humidified 5% CO₂ incubator in 2 ml RPMI medium(Sigma) containing 2 mmol l^-1 L-glutamine, 100 IU penicillinand 100 µg streptomycin, and 3 µg ml^-1 indomethacin(Sigma). Following overnight treatment, the tissue was incubatedin the same medium containing 1-methyl-3-iso-butylxanthine (Sigma)at 37 °C for 30 min. It was then treated with control mediumor 100 nmol l^-1 iloprost (a gift from Schering Health Care,Burgess Hill, W Sussex, UK) for 10 min at 37 °C and lysedin 0.1 mol l^-1 HCl and frozen until assayed. Cyclic AMP concentrationwas measured by ELISA (Biomol, Affiniti, Exeter, Devon, UK)according to the manufacturer’s instructions and normalisedto the protein concentration determined by a modification ofthe method of Lowry (Bio-Rad, Hemel Hempstead, Herts, UK). Dataare presented as the fold induction of cAMP after treatmentwith iloprost, where fold induction was calculated relativeto the control samples.

Statistics
Where appropriate, data were subjected to statistical analysiswith ANOVA and Fisher’s protected least significant differencetests (Statview 4.0; Abacus Concepts Inc., Piscataway, NJ, USA)and statistical significance was accepted when P < 0.05.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

The temporal pattern of PGIS mRNA expression in the human endometriumacross the menstrual cycle was studied by quantitative RT-PCR.PGIS mRNA was detected in all samples of human endometrium examined(Fig. 1a). Relative expression was significantly higher in themenstrual phase of the cycle compared with all other phases(14.49 ± 5.92 vs 2.28 ± 0.74 for EP-MP; 1.25 ±0.33 for LP-Ov; 1.75 ± 0.67 for ES and 4.7 ± 3.15for MS-LS; P < 0.05 for all comparisons). Similarly, thetemporal pattern of IP receptor mRNA expression across the menstrualcycle was assessed by quantitative RT-PCR and IP receptor mRNAwas detected in all samples of human endometrium examined (Fig.1b). Relative expression was significantly higher in the menstrualphase of the cycle compared with all other phases (33.94 ±17.2 vs 2.62 ± 0.7 for EP-MP; 1.36 ± 0.25 forLP-Ov; 2.95 ± 0.76 for ES and 2.87 ± 0.53 forMS-LS; P < 0.001 for all comparisons).

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Figure 1 Quantitative RT-PCR of (a) PGIS and (b) IP receptor in the human endometrium across the menstrual cycle. Results are expressed as the mean ± S.E.M. of relative mRNA expression levels. *P < 0.05.

Immunohistochemical staining for PGIS was performed in fullthickness human endometrial biopsies collected from across themenstrual cycle. A similar pattern of staining was observedin tissue sections from proliferative and secretory phases (Fig.2

is a representative sample of endometrial tissue collectedduring the proliferative phase). Cytoplasmic and nuclear immunoreactivitywas detected in glandular epithelial cells in the basal (Fig.2b

) and functional (Fig. 2c

) layers. Stromal cell reactivitywas also present in both layers, but with greater reactivityin the functional than in the basal layer (Fig. 2a

). Endothelialcell staining was detected in the microvasculature in both endometriallayers and reactivity was also present in myometrial smoothmuscle cells (enlarged area in Fig. 2a

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Figure 2 Immunohistochemical localisation of PGIS in human endometrial tissue (functional layer and basal-myometrial junction) collected in the proliferative phase of the menstrual cycle. Strong staining was detected in the glandular epithelial cells (G) in basal (B) and functional (F) layers (a–c) and in smooth muscle cells in the myometrium (M) (enlarged area in inset to a). Stromal staining was detected in the basal (b) and the functional layer (c) and endothelial cell reactivity was present in blood vessels (indicated by arrows) in all layers. NEG, negative control; scale bars = 50 µm.

The site of expression of the IP receptor was studied by insitu hybridisation and immunohistochemistry. IP receptor mRNAexpression was detected in endometrial samples collected duringthe menstrual and proliferative phases of the menstrual cycle.IP receptor expression was localised to glandular epithelialand stromal cells in the basal and functional layers of theendometrium (Fig. 3b–d

). In addition, expression was presentin myometrial smooth muscle cells (Fig. 3a

) and in endothelialcells lining vessels in the functional and basal layers of theendometrium and at the basal-myometrial junction (Fig. 3a andc

). Immunohistochemical staining for IP receptor protein wasdetected throughout the menstrual cycle in the cytoplasm andnuclei of glandular epithelial cells in both basal and functionallayers (Fig. 4a–c

). Similar to PGIS immunoreactivity,IP receptor stromal cell staining was stronger and more widespreadin the functional layer (Fig. 4c

) compared with the basal layer(Fig. 4b

). IP receptor protein expression was also localisedto endothelial cells throughout the microvasculature and waspresent in myometrial smooth muscle cells.

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Figure 3 In situ hybridisation of IP receptor in sections of human endometrial tissue collected in the proliferative phase of the menstrual cycle. IP receptor was expressed in smooth muscle cells in the myometrium (a) and reactivity was also present in glandular epithelial cells (G) and in stromal cells in both the basal layer (b) and the functional layer (c and d). IP receptor was also expressed in vascular endothelial cells (indicated by arrows in a and c). NEG, negative control; scale bars = 50 µm.

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Figure 4 Immunohistochemical localisation of IP receptor in human endometrial tissue (functional layer and basal-myometrial junction) collected in the proliferative phase of the menstrual cycle. Glandular epithelial staining (G) was present in both basal (B) and functional (F) layers and reactivity was detected in smooth muscle cells in the myometrium (M) (a–c). Stromal cell staining was present throughout the endometrium, but was stronger in the functional layer (c) compared with the basal layer (b). Endothelial cells throughout the endometrium and at the basal-myometrial junction also exhibited positive reactivity for the IP receptor (indicated by arrows in b and c). NEG, negative control; scale bars = 50 µm.

To investigate the functionality of the IP receptor, cAMP generationin response to iloprost (a PGI₂ analogue) treatment was assessedin endometrial biopsy tissue collected across the menstrualcycle (Fig. 5

). Cyclic AMP generation in response to 100 nmoll^-1 iloprost was significantly higher in endometrial samplescollected during the proliferative phase compared with the secretoryphase (4.83 ± 0.74 fold increase vs 2.07 ± 0.39fold increase; n = 4 for each group; P < 0.05).

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Figure 5 Fold increase in cAMP generation in endometrial tissue collected from the proliferative (n = 4) and secretory (n = 4) phases of the menstrual cycle in response to 100 nmol l^-1 iloprost. Results are expressed as the mean ± S.E.M. of fold cAMP induction. *P < 0.05.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion Acknowledgements References

This study demonstrates the expression of PGIS and IP receptorgenes in the human endometrium and shows significant up-regulationof both during menstruation. PGIS is the terminal enzyme thatleads to synthesis of PGI₂ in target tissues (Kniss 1999). Thehigher expression level of PGIS during menstruation supportsprevious observations reporting a temporal pattern of PGI₂ secretionby the human endometrium across the menstrual cycle; PGI₂ concentrationsare maximal in uterine venous blood during menstruation (Goodfellow et al. 1982).The elevated expression of IP receptor duringmenstruation suggests that PGI₂ synthesis and IP receptor aretemporally regulated to induce their effects on target cells.This is supported by the maximal iloprost-induced cAMP responseobserved in the endometrium collected during the menstrual/proliferativephases. The IP receptor has been shown to couple to G_s proteinswhich are linked to increases in cAMP generation (Narumiya etal. 1999). Although only the protein kinase A pathway was investigatedin this study, it is predicted that the IP receptor may activateother signalling pathways in the human endometrium, as has beenshown recently for other prostaglandin receptors (Jabbour & Boddy 2003,Milne & Jabbour 2003). Such diverse signallingpathways may lead to differential activation of target genesthat can promote various phenotypic changes on target cells.In addition to the classical G protein-coupled IP receptor,recent evidence suggests that prostacyclin functions via thenuclear peroxi-some proliferator-activated receptor delta (PPAR ${delta}$ )(Lim & Dey 2002). The importance of this mechanism in prostacyclinactivity in non-pregnant endometrium is not known. However,it is unlikely to be the predominant signalling pathway, sinceexpression of PPAR ${delta}$ in the normal human endometrium is minimal(Tong et al. 2000).

The factors that regulate the expression of the PGIS and IPreceptor during menstruation in the human endometrium are notclear. It is likely that this temporal expression is regulatedby steroid hormones as has been postulated for other prostanoidsand their receptors (Milne et al. 2001, Milne & Jabbour 2003).Oestradiol-17ßhas been shown to stimulate thesecretion of PGI₂ in endometrial stromal cells (Levin et al. 1992).Whether this is associated with up-regulation in theexpression of the IP receptor is unclear. Expression of theIP receptor may also be regulated by PGI₂ or other prostaglandins.Expression of PGIS and synthesis of PGI₂ is induced by COX-2(Caughey et al. 2001), which is up-regulated during the timeof menstruation (Jones et al. 1997). It is also plausible thatlocal mediators within the endometrium may play a role in theregulation of PGI₂ synthesis and/or expression of its receptor.For instance, PGI₂ is a mediator of the protective effects ofvascular endothelial growth factor (VEGF) on the vasculature(Zachary 2001) and PGI₂ biosynthesis is up-regulated by VEGFvia ERK-mediated cytosolic phospholipase A₂ activation and arachidonicacid mobilisation (Zachary & Gliki 2001).

PGIS and IP receptor expression have been co-localised to multi-cellularcompartments of the human endometrium. These include stromal,glandular epithelial, endothelial and smooth muscle cells. Thissuggests that PGI₂ acts in an autocrine/paracrine manner withinthe human endometrium to induce its cellular effects. PGIS andIP receptor immunoreactivities have been demonstrated previouslyin myocytes, vascular smooth muscle cells and endothelial cellsin pregnant and non-pregnant human myometrium (Moonen et al. 1986,Chegini & Rao 1988, Giannoulias et al. 2002). To ourknowledge, however, this the first report of localisation ofPGIS and IP receptor in glandular epithelial and stromal cellswithin the human endometrium. Previous studies using autoradiographywith [³H]PGI₂ on human uterine tissue failed to demonstratePGI₂ binding sites in epithelial cells (Chegini & Rao 1988),although in that study binding sites were demonstrated in myometrialsmooth muscle. This inconsistency with findings presented hereinmay reflect differences in the sensitivity of the methods used.Interestingly, stromal expression of PGIS and IP receptor washighest in the functional layer of the endometrium. In pre-menopausalwomen, the human endometrium undergoes phases of proliferationand apoptosis during successive menstrual cycles. These phasesare observed predominantly in the functional layer of the endometrium,which is shed at menstruation before regenerating during theproliferative phase of the subsequent menstrual cycle. Hence,this spatio-temporal expression of PGIS and IP receptor maybe crucial for, and in keeping with, its predicted role in menstruation.

Baird et al. (1996) have postulated a role for PGI₂ in menstruationbased on its myometrial smooth muscle and vascular relaxationeffects and inhibition of platelet aggregation. This would counteractthe effects of other prostaglandins such as PGF₂, which causesvasoconstriction and myometrial smooth muscle contraction (Crankshaw & Dyal 1994).It is also likely that PGI₂ is involved inthe repair of the vascular bed, since it has protective effectson the endothelium by inhibiting vascular smooth muscle proliferationand enhancing endothelial cell survival (Zachary 2001). Theincreased expression of PGIS and IP receptor during menstruationis also consistent with a role for PGI₂ in the aetiology ofmenorrhagia. Evidence for this has been provided previouslyby studies of dysfunctional menstrual bleeding, which have demonstratedincreased prostaglandin synthesis including PGI₂ (Smith et al.1981b, Cameron et al. 1987) or increased synthesis of PGI₂ relativeto thromboxane A₂ (Makarainen & Ylikorkala 1986b) in uterinetissue from women with excessive blood loss relative to controls.Whether IP receptor expression and signalling are also elevatedin the endometrium of women with dysfunctional menstruationremains to be established.

In summary, this study has demonstrated temporal expressionof PGIS and IP receptor in the non-pregnant human endometrium.Expression of both genes is highest during the menstrual phaseand is localised to multi-cellular compartments. The functionof PGI₂ in the human endometrium is linked to the protein kinaseA pathway during menstruation. Future studies will elucidatethe exact role of PGI₂ in menstruation and the mechanisms ofits signalling in the human endometrium.

Acknowledgements

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

The authors would like to acknowledge Mrs Sheila Boddy for assistancewith cAMP assays and Mrs Catherine Murray for patient recruitment.This research was funded by the Medical Research Council awardedto H N J (Unit Support) and H O D C (programme grant no. 0000066).

Footnotes

Received 21 July 2003
First decision 11 September 2003
Accepted25 September 2003

References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

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