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1 Division of Environmental Health Sciences, Graduate School of Medicine, Center for Disease Biology and Integrative Medicine, The University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan2 National Institute for Environmental Studies, Research Center for Environmental Risk, Tsukuba 305-8506, Japan
(Correspondence should be addressed to C Tohyama; Email: ctohyama{at}m.u-tokyo.ac.jp)
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Abstract |
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 Top Abstract IntroductionMaterials and MethodsResultsDiscussionReferences |
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4–7 days earlier than in the offspring born to vehicle-treated animals. The ovarian weight gain was also accelerated following exposure to TCDD in a dose-dependent manner. We next examined the ovarian compensatory hypertrophy (OCH) as an indicator of the maturation of the LH/GnRH-generating system in the pituitary and the hypothalamus. Exposure to TCDD accelerated the onset of OCH in the female offspring in a dose-dependent manner. In particular, in the offspring born to the dams exposed to TCDD at 800 ng/kg b.w., hypertrophy, which is characterized by hyperovulation and a marked increase in the weight of the remaining ovary after hemi-ovariectomy, was observed on postnatal days 27–30, which was 10 days earlier than in the offspring born to the vehicle-treated dams. These results indicate that perinatal exposure to a low dose of TCDD induces precocious puberty, including early maturation of the hypothalamic–pituitary axis, the gonads and genitals, in female Long-Evans hooded rats. |
Introduction |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
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To study the effects of perinatal exposure to TCDD on male and female offspring, the experimental protocol of a single oral administration of TCDD to pregnant rats has been widely used. An in utero and lactational exposure to TCDD, administered on gestational day (GD) 15 at a dose of 50–800 ng/kg b.w. was reported to induce disorders of the male reproductive organs (Mably et al. 1992, Ohsako et al. 2002), a decrease in epididymal sperm count (Gray et al. 1997a), and alteration of reproductive behavior in adulthood (Mably et al. 1992). An in vitro study (Lai et al. 2005) showed that TCDD modulates cAMP signaling in rat Leydig cells and affects the process of steroidogenesis. Female offspring, born to dams to which TCDD was administered at an oral dose of 1 µg/kg on GD15, was reported to show delayed vaginal opening (Gray et al. 1997b, Dienhart et al. 2000). However, in these studies, one cannot rule out the possibility that the delay observed might be attributable to the developmental delay and/or health impairment rather than a direct TCDD effect on sexual maturation, because the suppression of body weight gain and vaginal malformation were also observed. In addition, because sexual maturation is associated with not only the development of the external genitalia and ovaries, but also the luteinizing hormone (LH)/gonadotropin-releasing hormone (GnRH) surge-generating mechanism in the pituitary–hypothalamus, the possible effects of perinatal exposure to TCDD on the onset of puberty should be studied from a teratological aspect of the genitalia as well as from the entire aspect of sexual maturation. To clarify the effects of TCDD exposure on female sexual development and maturation, we studied the onset of vaginal opening (referred to as vaginal opening test hereafter), the development of the ovaries (referred to as ovarian development test hereafter), the onset of estrus cyclicity (referred to as estrus cyclicity test hereafter), and maturation of the hypothalamus–pituitary axis (referred also as first ovulation test and ovarian compensatory hypertrophy (OCH) test hereafter) in offspring born to rats that were exposed to a low dose of TCDD, the level of which did not induce body weight loss of the offspring.
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Materials and Methods |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
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Long–Evans hooded rats were purchased and imported directly from Charles River Laboratories in Chicago, IL, USA. The administration of TCDD to animals and autopsies were performed in the specific hazardous chemicals controlled area of the National Institute for Environmental Studies (NIES). TCDD was purchased from Cambridge Isotope Laboratory (Andover, MA, USA). The rats were perinatally exposed to TCDD, as described previously (Ohsako et al. 2002). Briefly, on GD15, pregnant female rats were administered TCDD by gavage (2.5 ml/kg) at 0 (0.1% nonane in corn oil as vehicle), 200, and 800 ng/kg b.w.; each group consisted of 16, 16, and 18 animals respectively. One day after birth, the number of male and female pups was adjusted, if possible, to five each per litter by culling, to minimize the variation in TCDD intake from dams' milk. Pups were weaned on postnatal day (PND) 21 and group-housed unisexually (four to five pups) thereafter (78, 80, and 88 females in groups exposed to TCDD at 0, 200, and 800 ng/kg b.w.; hereafter referred to as 0-, 200-, and 800-TCDD-exposed groups respectively, as shown in Fig. 1). The body weights of the dams and pups were monitored daily throughout the experiment. Animals were handled with humane care according to the guidelines for animal experiments of the NIES. All data except for body weight gain were adjusted for litter membership to minimize maternal effects, and calculated using the average per litter as each representative value.
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The female offspring (24, 23, and 25 animals (selected from 8, 8, and 9 litters respectively, to minimize litter effects) of the 0-, 200-, and 800-TCDD-exposed groups respectively) were monitored daily in the morning by the vaginal opening test (Fig. 1). Once vaginal opening was observed, the first estrus and the estrus cyclicity were determined by the daily monitoring of vaginal smear as the first estrus test (Fig. 1). Vaginal estrus was considered to have occurred when cornified epithelial cells became the major component of the smear. When the normal duration of the estrus cycle was found to be repeated at least three times by monitoring the vaginal smear from each group of rats, the estrus cyclicity was determined by the estrus cyclicity test (Fig. 1). From each group, eight rats, each selected from eight litters, were killed under diethyl ether anesthesia in the morning when the first vaginal estrus was observed, and the number of ova in the oviduct was counted as first ovulation test (Fig. 1). All animals were killed at specified times at a maximum of PND 64 to collect ovaries and uteri.
OCH test
A specified number of animals in the TCDD-exposed groups were subjected to hemi-ovariectomy under light diethyl ether anesthesia on PNDs 15, 20, 25, 30, 35, and 40 (6–15 litters per group, see details in Fig. 1). The remaining ovary was harvested on the day when the estrus phase was detected by smear test in the morning of days 7–10 after hemi-ovariectomy. In case the estrus phase was not detected during this 4-day period, the remaining ovary was harvested on day 10. The harvested ovary was weighed and examined histopathologically, as described below, for OCH test. The number of ova in the oviduct was counted at P25 (hemi-ovariectomy on PND 15 and OCH test on PNDs 23–25), P30 (hemi-ovariectomy on PND 20 and OCH test on PNDs 27–30), P35 (hemi-ovariectomy on PND 25 and OCH test on PNDs 33–35), P40 (hemi-ovariectomy on PND 30 and OCH test on PNDs 37–40), P45 (hemi-ovariectomy on PND 35 and OCH test on PNDs 42–45), and P50 (hemi-ovariectomy on PND 40 and OCH test on PNDs 47–50). The OCH in this experiment indicates the estimated percentage of OCH (estimated OCH%) that was derived from the following equation: (remaining ovarian weight/expected ovarian weight)x100. The expected ovarian weight of each animal was determined using a regression curve of ovarian development in each exposed group (Fig. 3). The equations for regression curve for the 0 ng TCDD/kg group, 200 ng TCDD/kg group, and 800 ng TCDD/kg group are Y=483e0•0457X with R2=0.937, Y=6.18e0•042X with R2=0.954, and Y=23.6 ln(X)–51.4 with R2=0.931 respectively. X and Y represent the day of OCH% test and the expected ovarian weight respectively, when hemi-ovariectomy was not performed.
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To examine ovarian development, the ovary on the right side was removed from each animal during a specific developmental period. The remaining left ovary enlarged to compensate the ovary function, i.e. OCH as described above. The current experimental design enabled us to collect ovary samples to examine the effect of TCDD exposure on ovarian development on PNDs 15, 20, 25, 30, 35, and 40 (see Fig. 1). All these collected ovary samples were weighed and histopathologically examined as described below.
Histological examination
For histological examinations, the organs were weighed, fixed in Bouin's solution, embedded in paraffin, sectioned at 5 µm thickness throughout the organ and stained with hematoxylin and eosin. Every fifth section, was examined for the presence of follicles and corpora lutea in the ovary by light microscopy.
Statistical analysis
All statistical analyses were performed using SPSS 16.0 software (SAS Japan Inc., Tokyo, Japan). A difference was considered statistically significant at P<0.05. In statistical analyses, data for the incidence of ovulation and the presence of corpora lutea in the ovary were analyzed by the 
2-test. Other data were analyzed by one-way ANOVA followed by Scheffe's post hoc test, while body and ovarian weight gains were analyzed by either two-way or repeated-measures two-way ANOVA. Data were expressed as mean ± S.E.M. unless otherwise stated.
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Results |
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Following the administration of TCDD to the pregnant rats at a single oral dose of 200 and 800 ng/kg b.w., no significant physiological gross alterations were observed in dams and pups: these alterations refer to body weight gain during pregnancy, maternal death, number of live pups, and birth weight of pups (data not shown). A slight decrease in body weight gain was observed on PND 49 in the 800-TCDD-exposed group (P<0.05), whereas there were no difference between groups from PND 0 to 42 (Table 1).
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The day of vaginal opening in each female offspring was monitored to determine the maturation of the external genitalia by the vaginal-opening test. In the female rats of the 0-TCDD-exposed group, vaginal opening was found to occur on PND 36.6±1.9 (Table 2), which was similar to observations in previous studies using Long-Evans hooded rats (Rayner et al. 2004, Salazar et al. 2004). In comparison with the control offspring rats, TCDD accelerated the onset of vaginal opening in the offspring of the 200- and 800-TCDD-exposed groups in a dose-dependent manner, and vaginal opening was observed on PNDs 33.3±1.8 and 29.1±1.8 respectively.
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First estrus test The onset of the first estrus was determined by the daily vaginal smear monitoring. The onset of the first estrus in the female offspring of the 0-TCDD-exposed group was PND 40.6±2.2 (Table 2). By contrast, perinatal exposure to TCDD at 200 and 800 ng/kg b.w. was found to accelerate the onset of the first estrus of the offspring, namely PNDs 35.9±3.4 and 32.7±2.2 respectively, in a dose-dependent manner, with a statistically significant difference for the 800-TCDD-exposed group (P<0.01 versus the 0-TCDD-exposed group, Table 2).
First ovulation test When ovulation at the first estrus was examined, five out of eight female rats born to vehicle-treated dams ovulated at the first estrus on PND 40.0±1.7, ranging from PND 37 to 42. All the rats born to dams treated with TCDD at 200 or 800 ng/kg b.w. ovulated at the first estrus on PNDs 34–38 and PNDs 29–33 respectively. No significant difference in the number of ova was found among the animals ovulated (13.2±2.2, 13.9±2.1, and 14.2±2.4, in the 0-, 200-, and 800-TCDD-exposed groups respectively).
Estrus cyclicity test When we examined whether perinatal exposure to TCDD affected the estrus cycle of these offspring (8, 8, and 9 litters in the vehicle group, 200-TCDD-exposed group and 800-TCDD-exposed group respectively), all the rats showed an estrus cycle of 4 or 5 days, and no abnormal estrus cyclicity was observed since they had the first estrus.
OCH test
In the control offspring born to vehicle-treated dams, OCH was not observed until P40 (hemi-ovariectomy was performed on PND 30 and the OCH was examined on PNDs 37–40, as described in the Materials and Methods). No ovulation was observed on P25 (data not shown) and P30 (Fig. 4A), and the OCH% values were only 102.0±15.6% and 102.5±12.1% respectively (Fig. 4B). Only one out of seven litters (2 out of 12 offspring) born to vehicle-treated dams ovulated, and the average number of ova in the ovulating animals were 5.5 (five and six each) on P35. On P40, seven out of the nine control litters, which comprises 10 out of 12 offspring respectively, hyperovulated (10.9±2.4 ova from the remaining ovary, P<0.001 versus the 0-TCDD-exposed group without hemi-ovariectomy of P40, 6.6±2.0 ova per ovary), and the OCH% values were 212±15% (Fig. 4A and B).
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Discussion |
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TopAbstractIntroductionMaterials and MethodsResultsDiscussionReferences |
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Second, TCDD causes central precocious puberty by affecting the brain and not by the peripheral organs. This hypothesis is supported by the present experimental evidence revealing that TCDD-exposed animals showed early onset of ovulation and estrus cyclicity, which are governed by the GnRH-generating system in the brain (Mitsushima et al. 2003, Odum et al. 2004, Pinyerd & Zipf 2005). On the other hand, peripheral precocious puberty, which is typically observed as early genital and somatic development, occurs independent of brain maturation (Mitsushima et al. 2003), but is not associated with early ovulation and estrus cyclicity. It is widely accepted that peripheral precocious puberty cannot induce the early ovulation and the early onset of estrus cyclicity (Partsch et al. 2002). To verify the TCDD-induced early maturation of the GnRH-generating system in the brain, we examined the onset of OCH during the developmental period as a new index of the maturation of the hypothalamus–pituitary–genital axis, as described in the following paragraph.
Third, the onset of compensatory hypertrophy during the prepubertal period was shown to be a new useful index for the sexual maturation of the brain. The OCH% is calculated on the basis of the removed ovarian weight at the time of hemi-ovariectomy (Fukuda et al. 1984, Baligar & Kaliwal 2004). However, this method could not be directly applied to our present experiment because ovarian weight showed a marked increase during the developmental period, and because we could not preclude the possibility that TCDD itself affected ovarian development. Thus, in this study, we developed a method of obtaining an estimated OCH% using a minimum number of animals, and the expected ovarian weight was determined on an individual animal basis, by calculating from the regression curve of ovarian development for each exposed group (Fig. 3). Thus, the estimated OCH% in this study represents the effects of hemi-ovariectomy on the occurrence of OCH itself. Thus, the data at the time of hemi-ovariectomy in the OCH study allowed us to estimate ovarian development in the present experiment, including the theoretical curve of ovarian weight gain. There has been theoretical and experimental background knowledge on the OCH. Since the concept of the OCH phenomenon was first proposed nearly half a century ago (Mandl et al. 1952), experimental evidence has accumulated. When rats were hemi-ovariectomized, the remaining ovary showed compensatory hypertrophy with a twofold increase in its weight as well as hyperovulation, and this phenomenon was considered to be induced by an increase in the secretion of gonadotropins and/or direct neural regulation via vagus nerves (Chavez et al. 1987). The right side of the medial anterior hypothalamus is considered to be responsible for predominantly regulating OCH, because a unilateral lesion placed in the right side, but not in the left side of this region suppresses OCH (Fukuda et al. 1984). The maturation of the hypothalamus, ovary and pituitary are prerequisites for the onset of OCH, indicating that the negative feedback of estrogen and the GnRH-surge secretion cooperatively functions. Thus, the onset of OCH can be an excellent index for the maturation of the hypothalamus.
Because the aryl hydrocarbon receptor (AhR) is ubiquitously distributed in various brain regions including the hypothalamus (Petersen et al. 2000), and TCDD enters and distributes in the brain tissue from the blood circulation (Kakeyama et al. 2003), it is reasonable to speculate that TCDD affects the GnRH surge-generating mechanism and elicits its toxicity by activating the AhR pathway. Other studies showed that TCDD distributed at the CNS exerts neurotoxicological effects: a high TCDD dose (10 µg/kg) administered to rats was shown to reduce LH secretion and the number of ova at ovulation (Petroff et al. 2001). Exposure to TCDD at 15 µg/kg was reported to decrease the neuropeptide Y level in the arcuate nucleus (Fetissov et al. 2004) that is presumably involved in ovulation (Estrada et al. 2003) and the sexual maturation of the hypothalamus (Kalra & Kalra 2004). We reported in our previous study (Kakeyama et al. 2001) that the in utero and lactational exposure of rat dams to TCDD resulted in the alteration of the N-methyl-D-aspartate (NMDA) receptor subunit mRNA expression in the brain of their offspring. Because NMDA receptors are involved in the maturation of the brain GnRH surge-generating mechanisms (Kanamaru et al. 2001), it is reasonable to speculate that an alteration in the NMDA neural transmission induced by TCDD during development is, at least in part, responsible for the TCDD-induced central precocious puberty. Further studies are required to clarify this point.
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Acknowledgements |
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Received in final form 25 February 2008
Accepted 3 March 2008
Made available online as an Accepted Preprint 3 March 2008
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