1 Department of Obstetrics and Gynaecology, and 2 Gynaecology Research Group, Faculty of Medicine and Biological Sciences, Leicester University, Leicester LE2 7LX, UK
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Abstract |
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Key words: endometrium/HSP27/hormone replacement therapy/human ß-lactoglobulin/steroid receptors
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Introduction |
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Many markers have been employed to assess the hormonal influence in the endometrium; these include the level of oestrogen and progesterone receptors (ER and PR respectively), and the expression of heat shock protein 27 (HSP27) and human ß-lactoglobulin [pregnancy-associated endometrial 2-globulin (
2-PEG), placental protein 14 (PP14)]. However, no similar work has addressed this in relation to HRT. In the endometrium, both the concentration and the distribution of ER change during the normal menstrual cycle. These changes are predominantly under the influence of oestrogen and progesterone. There remains some disagreement on the exact pattern of expression, this particularly relates to whether the decline noted in the luteal phase commences at the beginning (Lessey et al., 1988
; Amso et al., 1994
) or the end (Garcia et al., 1988
) of the early luteal phase. Stromal staining may either plateau (Amso et al., 1994
) or decline (Lessey et al., 1988
) from the time of ovulation into the late luteal phase.
HSP27 (synonymous with p24 and p29), is a 27 kDa oestrogen-regulated phosphoprotein that may be involved in thermotolerance, protein degradation or as a molecular chaperone for other proteins including ER (Ciocca et al., 1993). The concentration of HSP27 is regulated by steroid hormones and cytokines. In the endometrial glandular epithelium, HSP27 appears during the late follicular phase and decreases after ovulation, and slightly rises premenstrually (Ciocca et al., 1983
). This contrasts to the stronger expression in the luminal epithelium during the luteal phase (maximum around day 21). Expression in the glands is higher in conditions of excessive oestrogen stimulation as in hyperplasia (Ciocca et al., 1985
). The stroma remains negative till the late luteal phase when the predecidual cells both around the spiral arterioles and beneath the superficial epithelium become positive (Ciocca et al., 1983
). Stromal but not glandular epithelium expresses HSP27 under the influence of prolonged progestogen stimulation (Padwick et al., 1994
).
Oestrogen, through an intragenic oestrogen-responsive element (ERE), is the main stimulator of PR gene expression. Progesterone down-regulates PR through a proteinprotein interaction between PR, ER and the same ERE (Savouret et al., 1991). In the mid-follicular phase (days 78), 25% of stromal and glandular cells are PR-positive. During the late follicular phase and the early luteal phase (days 919), the majority (75%) of glandular cells and half the stromal cells are positive. During the late luteal phase (days 2127), PR disappears from the glands but remains faintly positive in the stroma (Garcia et al., 1988
).
Quantitatively, human glycosylated ß-lactoglobulin (2-PEG, PP14) is the major secretory protein product of the decidua and the major soluble product of the endometrium during the late luteal phase (Bell, 1990
). Its function remains unknown, but it may have a role in maternal immune tolerance possibly through suppressing thymus-derived (T) and natural killer (NK) cells, and inhibiting interleukin-2 (IL-2)-mediated T cell proliferation (Seppala et al., 1994
). Human ß-lactoglobulin production is initiated on days 67 after the luteinizing hormone surge (LH+6 to LH+7) and rises thereafter to a maximum in the functionalis zone during the late luteal phase (Waites et al., 1988
). Its concentration is related to the type of progesterone (levonorgestrel>medroxyprogesterone acetate), and is dependent on oestrogen pre-priming (Li et al., 1992
).
Despite a similar bleeding pattern, we have demonstrated significant histological differences between the late progestogenic phase endometrium from women on HRT and the endometrium of the late luteal phase, and whilst some of the observed features were shared with the early or mid-luteal phase others were not noted during the physiological luteal phase (Habiba et al., 1998). In this study, we aimed to investigate the discrepancy by measuring the level of ER, PR, HSP27, and human ß-lactoglobulin as markers of hormone balance.
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Materials and methods |
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The LH-dated natural cycle endometrial biopsies were obtained by dilatation and curettage from healthy women with regular cycles at the time of scheduled tubal sterilization. They were all given a urine ovulation detection kit (Clearplan; Unipath, Basingstoke, Hampshire, UK) and instructed in its use. Sterilization and dilatation and curettage were performed in the early luteal phase (days 26 after the LH peak, n = 10), the mid-luteal phase (days 711 after the LH peak, n = 10), or the late luteal phase (days 1214 after the LH peak, n = 10), with the day of LH peak being day 0. All endometrial samples were fixed in formalin and routinely processed and stained with haematoxylin and eosin to confirm normality and the LH dating.
Quantifying ER and PR using image analysis was shown to have a high degree of agreement when compared to the dextran charcoal-coated (DCC) method (86.7 and 91.1% respectively) (Esteban et al., 1993). Percentage of positive area (PA = positive nuclei/total nuclei) measurement was used in this study as it was demonstrated to have a high degree of correlation with the more complicated percentage of positive stain (PS = summation of optical density of the positive nuclear area divided by the summation of the optical density of all the nuclei studied). Furthermore, the latter was shown not to improve the correlation between PA and DCC (Esteban et al., 1993
). Thus image analysis, although semi-quantitative, combines an acceptable correlation with receptor content (correlation between the PA and DCC for ER, r = 0.71 (Esteban et al., 1993
), with the added advantage of enabling antigen localization.
Immunohistochemistry (IHC)
IHC was performed using the avidinbiotin complex immunolabelling method (Jackson and Blythe, 1993) with modifications. Briefly, sections were dewaxed in xylene, and rehydrated in grades of ethyl alcohol and distilled water. Sections were pretreated using enzyme digestion or microwave according to the antibody to be used (Table I
). Endogenous peroxidase was blocked by freshly prepared 6% v/v hydrogen peroxide for 10 min. Sections were washed in tap water and Tris-buffered saline (TBS)bovine serum albumin (BSA) buffer, and then covered in 100 µl of normal rabbit serum (NRS; Dako, Ely, Cambridgeshire, UK) at 1:10 in TBS (for anti-CD3 antibody, this was replaced with swine serum), and incubated for 20 min, these were then incubated with the primary antibody at the required dilution and time (Table I
). Slides were washed in TBSBSA and incubated for 30 min with the secondary antibody (100 µl of biotinylated antibody from a heterologous species) diluted at 1:150 in TBSBSA. They were then washed in TBSBSA and incubated with a freshly prepared solution Vectastain ABC peroxidase® (Vector Laboratories, Bretton, Peterborough, UK) for 30 min. Sections were washed and incubated with peroxidase substrate (DAB substrate, Vector Laboratories, UK) for 10 min. Slides were washed in running tap water, dried, dehydrated, cleared and mounted using XAM neutral medium (BDH, Poole, Dorset, UK). IHC for each of HSP27 and ß-lactoglobulin were carried out in one batch, IHC for ER and PR were each divided into two batches with two sections duplicated for quality control. The inter-assay variation was 6%. Negative controls were used where the primary or the secondary antibody were missed.
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HSP27 or human ß-lactoglobulin staining in the glands was measured by calculating the percentage of glands that stained positive in 17 low power fields (x100). Staining was evaluated by determining the proportion of tissue stained (P), multiplied by the intensity of staining (i), which was assigned scores, 0 = none, 1 = weak, 2 = distinct, and 3 = strong. The total score (T/score) was calculated using the equation: T/score = Pi (i + 1) (Lessey et al., 1988
; Budwit-Novotny, 1986). This equation reduces the influence of a change in intensity on the overall score. Scoring was carried out by one of the investigators (M.A.H.) who had been blinded to the exact cycle phase. Stromal staining for HSP27 was expressed as the number of cases that were either negative, weak or positive. In order to measure the total secretory gland activity within the glandular unit, including luminal secretions, the total glandular area expressing ß-lactoglobulin was measured in 17 high power fields (x200) per section (equivalent area of 1.59 mm2) and expressed in mm2 and as a percentage.
The percentage of glands expressing ER and PR was counted in 17 random low power fields (x100)/section and the percentage of luminal epithelium expressing the receptor was also calculated in the same area. Receptor expression was measured assuming two levels of intensity above the preset threshold. The proportions of weakly stained cells were almost identical at 41, 38, 37 and 40% in the early, mid-, and late luteal phases and the late pseudoluteal phase respectively. Comparison thus yielded results that are almost identical to those calculated based on a single scale. We therefore present the results using the percentage and the numerical scores (Tables II and IV).
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Results |
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In the late pseudoluteal phase, smaller glands were predominantly ER positive whilst the larger glands, which exhibited more advanced secretory features, were negative (Figure 1a). Some glands contained positive and negative cells, although the majority were uniformly either positive or negative. Staining in the surrounding stroma followed a similar pattern, with the stroma surrounding positive glands being predominantly positive, and vice versa. The higher expression of ER in the glandular epithelium of the late pseudoluteal phase endometrium is attributable to higher expression in the more prevalent smaller glands. There was, however, a wide patient-to-patient variability. The only statistically significant differences between the late pseudoluteal phase and the early luteal phase were in the number and the proportion of positive stromal cells (P < 0.05) (Table II
).
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The pattern of expression in the luminal epithelium in the late pseudoluteal phase was similar, but the HSP27-negative segments were larger and this accounted for the weaker overall expression. These differences were statistically significant compared with the physiological cycle (P < 0.05). Glandular staining followed the same pattern as in the physiological cycle, although staining was very weak. Expression of HSP27 was lower in glands in the late pseudoluteal phase compared to all stages of the luteal phase, but the difference was statistically significant only in comparison to the early luteal phase (P < 0.05). There was no preferential expression of HSP27 in relation to glandular size or distribution. The late pseudoluteal phase exhibited the highest stromal HSP27 expression (Table III).
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Expression of human ß-lactoglobulin
Glandular and luminal human ß-lactoglobulin was only rarely detected during the early luteal phase. This peaked during the mid- and late-luteal phase where most glands were positive. There was no staining in the stroma. The difference between the early luteal phase and both the mid- and late luteal phase was statistically significant (P < 0.05). During the late pseudoluteal phase the majority of the glands expressed human ß-lactoglobulin (Figure 1c), but a higher proportion (compared with the mid- and late luteal phases), especially of the smaller glands were negative. The glandular area expressing human ß-lactoglobulin during the late pseudoluteal phase was significantly higher compared with the early luteal phase, but lower compared with the mid-luteal phase or the late luteal phase (P < 0.05) (Figure 1c,d
; Table V
).
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Discussion |
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The expression of HSP27 in the endometrial glandular epithelium was found to be lower during the mid-progestogenic phase in women treated with sequential HRT in comparison with the endometrium during the physiological proliferative phase, and to be similar to that observed during the mid-luteal phase of the physiological cycle (Padwick et al., 1994). The expression of HSP27 may be inhibited by progestogens, and this inhibition may be type- or dose-related (Padwick et al., 1994
). Thus, the low values of HSP27 in the glandular epithelium during the late pseudoluteal phase observed in our study suggest, in the absence of other evidence of progestogenic influence, low induction rather than adequate inhibition.
It was argued that the late expression of human ß-lactoglobulin (luteal day 5) suggests that it is not directly dependent on either oestrogen or progesterone (Manners, 1990). Factors known to affect serum levels of human ß-lactoglobulin include the anti-oestrogen tamoxifen, the antiprogestin RU486, clomiphene citrate, HCG and the GnRH analogue buserelin (Seppala et al., 1994
). Glucocorticoid/progesterone regulatory elements (PREs) have been found in the human ß-lactoglobulin gene, and these elements bind purified PR in vitro (Vaisse et al., 1990
). It is therefore possible that factors affecting human ß-lactoglobulin secretion (other than progestogens) may act by modifying PRE response, with human ß-lactoglobulin secretion reflecting the balance of these factors. In sequential HRT specimens human ß-lactoglobulin production was reduced, despite evidence of stromal decidualization (Habiba et al., 1998
), thus emphasizing the dissociation between stromal and gland development, and between gland development and menstrual function.
There appears to be an inverse relationship between the expression of PR and human ß-lactoglobulin in both the physiological cycle and the late pseudoluteal phase. Semi-quantitative expression of human ß-lactoglobulin demonstrated that the late pseudoluteal phase cannot be compared with either stage of the luteal phase, expression being higher than in the early luteal phase, but lower than in the mid- or late-luteal phases. This may indicate a suboptimal progestogenic response, which may be secondary to a suboptimal oestrogenic induction of PR, or a function of the type or dose of progestogen used, or both. The higher ER expression in the glands and tendency to lower expression in the stroma suggest adequate progestogenic effect in the latter. This is supported by the finding of normal levels of PR during the late pseudoluteal phase. This, however, does not rule out the possibility of low initial levels of PR.
These findings suggest adequate progestogenic response on the stroma. Although the observation that some glands are ER-positive, but PR-negative, suggests that suboptimal PR expression in the glands may have contributed to the low human ß-lactoglobulin expression. A suboptimal progestogenic response may be due to the overall low level of receptor. This is supported by the finding of a difference in the level of PR but not in the PRA/PRB ratio in relation to the differential effect of progesterone and its antagonists on fibroids (Viville et al., 1997). However, an alteration of the PRA/PRB balance cannot be ruled out. This study demonstrates a suboptimal progestogenic response in this particular sequential HRT preparation that incorporates a progestogen with relatively strong androgenic properties and a high affinity to PR, and it is possible that the hypo-oestrogenism is secondary to relatively higher anti-oestrogenic properties. The differences observed in the oestrogenic and progestogenic effects on the endometrium may reflect the non-phasic administration mode of these steroids in this regimen, as is the case with all currently available HRT regimens. Alternatively, it may reflect the serum concentration of the steroids. This study did not address this question and further research is needed.
The value of urinary LH home detection kits in relation to infertility treatment is subject to debate (Robinson et al., 1992; Anderson et al., 1996
), and its accuracy may be reduced in infertile women with a high endogenous LH (Anderson et al., 1996
). It has, however, been shown to be highly sensitive and specific in women with normal cycles and no history of infertility (Schmutzler et al., 1995
; Miller and Soules, 1996
). Furthermore, we used histological assessment in order to confirm LH-dating in our study group. The difference in the level of expression of functional markers between the physiological cycle and women on sequential HRT, despite similar bleeding pattern (Habiba et al., 1996
), demonstrates dissociation between endometrial behaviour and functional markers. This parallels the observed dissociation between ER and PR and the amount of blood loss (Critchley et al., 1994
), and may be a function of the role of second messengers such as cAMP, protein kinase A, protein kinase C, activator protein-1 (AP-1), insulin-like growth factor-I (IGF-I), epidermal growth factor (EGF), and the proto-oncogene erb-2 ligand, glycoprotein 30 (gp30), in controlling or modifying the action of steroids (Katzenellenbogen, 1996
; Saceda, 1996). Nuclear receptor co-regulators and co-repressors modulate ligand-induced transcription (McKenna et al., 1999
). In relation to ER, oestrogen and raloxifene have been shown to induce distinct conformational changes in the transactivation domain of the ligand-binding domain (Brzozowski et al., 1997
; Grese et al., 1997
), which may affect the type of co-activator(s) recruited. This provides a putative mechanism for the differential effect of agonists and antagonists binding to the steroid receptor. Similarly, a differential binding of co-activators is a putative mechanism for the discrepant effect of norethisterone, and it is possible that pregnane and 19-norpregnane derivatives might have different molecular effects. Recently, it was suggested that the 19-nortestosterone derivative, levonorgestrel, may induce its progestational effects through non-receptor-mediated mechanisms (Salmi et al., 1998
). These observations highlight the need for further studies to clarify the molecular pathways of progestogen action.
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Notes |
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References |
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Submitted on June 1, 1999; accepted on October 12, 1999.