Department of Obstetrics and Gynaecology, Hamamatsu University School of Medicine, 3600 Handa Cho, Hamamatsu City 431-3192, Shizuoka Prefecture, Japan
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Abstract |
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Key words: interleukin-1/interleukin-8/neutrophil influx/prostaglandin E2/uterine contraction
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Introduction |
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IL-1 is a hormone-like polypeptide that apparently performs many roles in inflammation and immunity. This peptide is synthesized and secreted by choriodecidual macrophages during parturition (Romero et al., 1989d), and has been implicated as a signal for the onset of labour (Romero et al., 1989a
, 1990
, 1991
; Mitchell et al., 1990
). IL-1 has numerous biological effects on various target cells (Dinarello, 1988
). IL-1 induces IL-8 production (Uchiyama et al., 1992
), activates neutrophils (El Maradny et al., 1995
), regulates prostaglandin (PG) biosynthesis (Casey and MacDonald, 1988
; Romero et al., 1989b
; Mitchell et al., 1990
) and increases the production of other cytokines which are capable of stimulating prostaglandin production by intrauterine tissues (Romero et al., 1989c
; Mitchell et al., 1991b
). PGE2 is an inflammatory mediator known to be involved in myometrial contraction during labour (Barclay et al., 1993
). Additionally, IL-8 and PGE2 have been found to act synergistically, PGE2 reducing the concentration of IL-8 required to cause neutrophil invasion of rabbit skin (Colditz, 1990
). Previously, we reported that exogenous IL-8 or IL-1 induces cervical dilatation in rabbit (El Maradny et al., 1994
1995
). However, there have been no reports about the effect of IL-8 to IL-1 on uterine muscle contraction. We postulated that the changes in IL-8 concentrations in the endometrial tissue may potentiate the effect of IL-1-induced uterine contraction. The purpose of this study was to determine the effect of exogenous IL-8 on IL-1-induced uterine contraction in rabbits.
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Materials and methods |
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Experimental design
The animals were divided equally into four groups. The first group (IL-8 group), was treated by suppository containing 200 ng recombinant human IL-8 (Oncogen Science Inc., MA, USA) for 3 days. IL-1 (200 ng; Oncogen Science) was applied to each rabbit for 1 day in the second group (IL-1 group). Human recombinant IL-8 and IL-1 cross-react easily in rabbits. Three day treatment with IL-8 is essential to obtain the desired effect and 1 day treatment with IL-1 was found to be sufficient to produce optimal uterine contraction. Rabbits in the third group (IL-8 + IL-1 group) received suppositories containing IL-8, 200 ng for 3 days followed by IL-1, 200 ng. The fourth group (vehicle group) was treated with 500 µl of Witepsol base (Adeps solidus: Mitsuba Co., Tokyo, Japan). This vehicle group was considered the sham control. The uterine contraction in rabbits was also measured without any treatment, and the effect was found to be quite similar to that of the vehicle group.
Plasma collection
Peripheral blood (1 ml) was gently drawn from the middle ear artery into tubes (containing EDTA + 2Na, indomethacin and aprotinin) 3 h after the last dose of suppository treatment. The blood was centrifuged at room temperature for 10 min at 2000 g within 1 h. Aliquots were frozen immediately at 70°C until analysis. Plasma concentrations of PGE2 were detected by enzyme-linked immunosorbent assay (BIOTRA; Amersham Life Science, London, UK) according to the manufacturer's directions. The concentration of PGE2 was determined from a standard curve derived from PGE2 standard, which was run with each assay. All determinations of plasma PGE2 were carried out in duplicate.
In-vivo measurement of isometric contraction force
After blood sampling, in-vivo uterine contractions were measured as described previously (Machino et al., 1997). Briefly, surgery was conducted on a servo-controlled heating table to maintain body temperature at a constant 37°C. Anaesthesia was induced with ketamine hydrochloride (30 mg/kg, Ketalar; Parke Davis, Tokyo, Japan), injected through a marginal ear vein. Two PE-50 catheters were placed in the left jugular vein. One catheter was used for continuous infusion of Ketalar (68 mg/kg/h) and another for infusion of saline. The animals were allowed to breathe spontaneously. The uterus was exposed through a lower midline abdominal incision. The force transducer (NEC, Tokyo, Japan) was attached to the anterior surface of the body of the uterus using 30 suture material. These sutures were used to anchor the transducer cable to the uterus. The transducer was connected to a polygraph recorder (RMG 5204, Nihon-Kohden, Tokyo, Japan) via a universal amplifier. The transducer was standardized and 30 min were allowed for stabilization. Measurements were made after reaching stable uterine contraction. Contraction responses were measured isometrically for 30 min and recorded on a polygraph. Since the force transducer cannot give the absolute values of contraction the data were expressed as g weight that equals to 0.026 mV. All procedures were performed with strict aseptic conditions.
Sample preparation
The rabbits were killed with an overdose of Ketalar immediately after the experiments. After careful dissection, the uterus was divided into two parts; one half was placed in oxygenated buffer for the measurement of uterine contraction (in vitro) and another half was placed in 10% formalin for histological sections. The uterine muscles were immediately immersed in chilled, oxygenated KrebsRinger bicarbonate solution. Uterine muscle fibres were cut into 3x7 mm strips under a stereomicroscope. The myometrial strips were suspended in temperature-controlled organ baths containing 15 ml of KrebsRinger bicarbonate-buffered solution of the following composition (mM): NaCl 113, KCl 4.8, CaCl2 2.2, KH2PO4 1.2, MgSO4 1.2, NaHCO3 25, and glucose 5.5. The organ baths were oxygenated with 95% O25% CO2 at 37°C.
In-vitro recording of isometric force development
The isometric contraction of the myometrium was measured with a force-displacement transducer (TB-612T, Nihon-Kohden) connected to a MacLab Dose Response (AD Instruments, Tokyo, Japan) computer-based data acquisition system. Silk ligatures were tied to each end of the strips and one end of each strip was fixed to a Plexiglass rod and mounted in the organ baths irrigated with KrebsRinger buffered solution. The other end of each strip was connected to the force-transducer. A resting tension of 1 g was applied to the strips, and the isometric tension of the myometrial strips was recorded for 6 h.
Immunohistochemistry and quantification of stained cells
Histological sections were stained immunohistochemically for the surface antigen RT2, found in rabbit leukocytes using anti-rabbit RT2 monoclonal antibody (Cedar lane Laboratories, Hornby, Canada) as described previously (Ponsard et al., 1986). Paraffin embedded tissue sections were deparaffinized in xylene baths and rapidly rehydrated through graded 95% alcohol. Excess liquid was removed, and sections were washed in phosphate buffered saline (PBS, pH 7.2). Endogenous peroxidase was blocked by fixation of the sections in methanol and 3% hydrogen peroxide for 20 min at 23°C. To block the tissue sections bovine serum albuminphosphate buffered solution (BSA-PBS, 2%) was used. Anti-rabbit RT2 (1:100) monoclonal antibodies were placed on the sections after 20 min, and kept overnight at 4°C. The sections were incubated with the second antibodies (goat anti-rabbit IgG antibody; DAKO, USA) at 1:100 dilution for 2 h at room temperature, after washing 5 times in PBS. Avidinbiotinperoxidase complex (DAKO) was added at 1:1000 dilution for 1 h and washed with PBS. Bound antibody was detected by incubation with 3,3'-diaminobenzidine-tetrahydrochloride (DAB, 0.5 mg/ml; Sigma, St Louis, MO, USA), in 0.05 M TrisHCl buffer (pH 7.6) containing 1% H2O2. The sections were counter-stained in haematoxylin and dehydrated, then examined by light microscopy at x200 magnification. Negative controls received the same treatment without primary antibody. Neutrophils in the tissue were used as positive control. The number of neutrophils was estimated by counting the number of stained extravascular cells within a line grid (10x10 squares) occupying an area on the section of 0.15 mm2 using a x20 objective and x10 eyepiece and the mean values were calculated.
Statistical analysis
Results are expressed as mean ± SD of all experiments. Statistical differences were analysed by Student's paired t-test. A value of P < 0.05 was considered statistically significant.
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Results |
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Discussion |
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The present study demonstrates that administration of suppositories containing IL-1 and IL-8 + IL-1 induces a potent contractile effect in rabbit uterus. Only IL-8 produced no contractile effect, but in the presence of IL-1 it promoted uterine contractions with increased frequency and amplitude. We have also shown that treatment with IL-8 + IL-1 increases the neutrophil number as well as PGE2 synthesis. The increase in neutrophil number and PGE2 synthesis were greater in the IL-8 + IL-1 group than the IL-1 only group. Previous findings suggest that the application of TNF- and IL-1ß, but not IL-8, induced pre-term labour and delivery in guinea-pigs, which may be a result of a variable cytokine action on prostaglandin production (Chwalisz et al., 1994
). Both TNF-
and IL-1ß stimulated PGE2 production from cultured amnion, decidual and chorion cells (Mitchell et al., 1991b
), whereas IL-8 did not lead to stimulation of PGE2 production in these cells (Mitchell et al., 1991a
; Dudley et al., 1993
), which is consistent with our observations that administration of IL-8 suppository did not induce uterine contraction in rabbits. However, IL-8 is critically involved in the process of parturition. A synergy between IL-8 and PGE2 may be operational here.
Growing evidence suggests that cytokines are present in the gestational tissue and play a major role in the triggering and perpetuation of labour (Romero et al., 1991; El Maradny et al., 1994
1995
1997
; Kelly, 1994
). Various uterine cells and cervical fibroblasts are capable of producing cytokines such as IL-8 and IL-1 (Uchiyama et al., 1992
; Kelly et al., 1994
). The action of IL-8 and IL-1 suggests that they interact. According to our hypothesis, the mechanism of cross-talk between IL-8 and IL-1 is as follows. Firstly, we found that IL-8 leads to accumulation of neutrophils in rabbit endometrial tissue. The neutrophil influx and activation of neutrophils in the cervix and choriodecidual tissue initiate a cascade of events leading to the loosening of endometrial connective tissues (Wewer et al., 1992; Kuijpers and Harlan, 1993
) as well as increased permeability of the vessels (Wedmore and Williams, 1981
). As a result, inflammatory cells such as macrophages infiltrate to the matrix from vessels, contributing to the synthesis of IL-1 (Kelly, 1994
). Secondly, IL-8 enhances the release of other inflammatory cytokines such as IL-1 (Yu et al., 1994
), which can stimulate the production of PGE2 and enhance uterine contraction. Thirdly, there is evidence that the inflammatory cytokine IL-1 also regulates IL-8 synthesis in endometrial cells (Arici et al., 1993
), which may further modulate the inflammatory reaction (Yu et al., 1994
). Thus the number and existence of neutrophils in the endometrial tissue were more significantly increased in the IL-8 + IL-1-treated group.
To clarify the effect of IL-8 on myometrial contraction, we used animals which are not affected by progesterone. However, a pilot study showed that the effect of IL-8 on myometrial contraction in pregnant rabbits was similar to that in nonpregnant rabbits (data not shown). These findings suggest that IL-8 together with IL-1 enhance PGE2 mediating uterine contraction via neutrophil transmigration at the onset of labour. IL-8 is a locally acting cytokine and possibly a small amount of IL-8 is absorbed into the circulation. However, red blood cells carry multispecific receptors that can bind a wide array of chemokines. IL-8 can be absorbed by red cells and no free IL-8 exists in the circulation (Darbonne et al., 1991). Thus exogenous IL-8 might act on the endometrial tissue by simple diffusion.
In conclusion, at the onset of labour IL-8 and IL-1 concentrations increase, which triggers the production and action of PGE2. The combination of PGE2 and IL-8 would be a powerful stimulus for the invasion of neutrophils and their degranulation. The interaction between IL-8 and IL-1 seems to be essential for forceful uterine contraction.
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Acknowledgments |
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Notes |
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References |
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Submitted on June 19, 1998; accepted on November 3, 1998.