Acupuncture and HPO Axis
Acupuncture
Normalizes Dysfunction of Hypothalamic-Pituitary-Ovarian Axis By
Bo-Ying Chen M.D.
Professor of Neurobiology
Institute of Acupuncture and Department of Neurobiology
Shanghai Medical University, Shanghai 200032, P.R. China
(Received June 3, 1997; Accepted with revisions June 30,1997)
ABSTRACT
This article summarizes the studies of the mechanism of
electroacupuncture (EA) in the regulation of the abnormal function
of hypothalamic pituitary-ovarian axis (HPOA) in our laboratory.
Clinical observation showed that EA with the effective acupoints
could cure some anovulatory patients in a highly effective rate and
the experimental results suggested that EA might regulate the
dysfunction of HPOA in several ways, which rneans EA could influence
some gene expression of brain, thereby, normalizing secretion of
some hormones, such as GnRH, LH and E2. The effects of EA might
possess a relative specificity on acupoints.
KEY WORDS:
Electroacupuncture, ß-Endorphin, GnRH, LH, Estradiol, Estrogen
receptor, Ovariectomized rat, Hypothalamic-pituitary-ovarian axis
INTRODUCTON
Acupuncture is a
treasure of Chinese traditional medicine, which is employed in the
treatment of different diseases, especially in relief of all kinds
of pain [1, 2] over the world. Since 1960s we have used acupuncture
with appropriate electro-stimulation to cure patients with
anovulation disorder (sterility), the rate of EA induction of
ovulation was increased from 50% initially to 80% presently. Other
authors in China also reported that acupuncture was successfully to
treat patients with sterility [3] and the lying-in woman with
subnormal contraction of uterus [4]. All the above research
demonstrates that acupuncture may be an effective curative method of
some woman's diseases. However, many questions, such as "why", "how
to" and "which" about the mechanism of EA effect are unknown. To
address these problems we supposed that EA might influence the
production and secretion of hormones, neurotransmitters or neuro-modulators
of HPOA leading to the normalization of hormone status. We also
noticed certain artides reported that EA might affect the blood
levels of LH, FSH, estradiol (E2) and prolactin in the female
patients [4, 5, 6] and EA may be related to long term changes in
gene expression [7, 8]. These results are all significant, yet
insufficient to explain the mechanism of EA in the regulation of the
function of HPOA. To obtain more data, a series of experimental
studies in human and animal models has been performed in our
laboratory.
MATERIALS AND
METHODS
Selection and treatment of cases
Ten cases of chronically anovulatatory patients including eight
cases of polycystic ovarian disease (POCA), one case of
hypogonadotropic amenorrhoea and one case of oligomenorrhea were
treated with EA in 13 menstruation cycles. They were all of
productive age and the courses of disease were 3 to 12 years. On the
10th day of each menstruation cycle, the patients accepted the EA
treatment. "Guanyuan(RN4)," "Zhongji(RN3)," "Sanyinjiao(SP6)," and
bilateral "Zigong(EXCA1)" points were stimulated for 30 min at 8:00
AM, Q.D. for 3 days. The stimulation parameters were 7-8mA and 4-5
Hz with G6805 model generator. The electric current of EA was
bearable well for every patient. The blood samples were collected
from forearm of the patients one time per 15 min for detection of
FSH.LH and ß-endorphin (ß-E).
Five health volunteers of a productive age with normal menstruation
cycle were selected as controls, which were undergone the same
treatment as above mentioned.
Animals and treatments
Wistar female rats weighting 200-250g were used. The half of animals
were undergone ovariectomy and fed in the same environment with the
intact rats at least for 15 days and vaginal smears were examined
per day for 3 times. No exfoliative epithelium cell was found in the
smears as an index for successfill ovariectomy. The ovariectomized
rats and intact rats were randomly divided into two groups
respectively: ovariectomized rat group (OVX), ovariectomized rat
accepted EA treatment group (OVX+EA), intact rat group (INT) and
intact rat accepted EA treatment group (INT+EA). The animals in
OVX+EA and INT+EA received EA at the experimental acupoints of
Guanyuan (RN4), Zhongji (RN3), Sanyinjiao (SP6) and bilateral Zigong
(EXCA1) by EA apparatus (Model G6805-2, SMIF, Shanghai, China) with
the frequency of 3 Hz and an intensity to produce a slight twitch of
the limbs. After 3 days' treatment animals were given EA at Waiguan
(SJ5) and Huatuojiaji (EXTRA21) as the control acupoints in the same
way (Fig 1). By the end of last experiment, animals were sacrificed
and their adrenals, brains and pituitaries were taken out for
detection of nucleolar oganizer regions (AgNORs) and hormones.
Pushpull perfusion in hypothalamic preoptic area (POA) and elution
of pituitary and LH and ß-endorphin (ß-EP)
The
technique of brain pushpull perfusion was processed as previously
described by our laboratory [1]. The perfusate from hypothalamic POA
was kept at -70°C for GnRX and ß-EP RIA.
The pituitaries were retrieved and put into 4°C cooled saline.
Afterward, each pituitary was homogenized with 500µl of 70% acetone
aqueous solution at 4°C. The homogenate was centrifugalized (2,000xg
for 15 min at 4°C) and the supernatant was freeze-dried for LH and
ß-EP RIA.
Radioimmunoassay (RIA) of hormones
GnRH IRA: GnRH content in the perfusate from rat hypothalamus
was determined by RIA method developed by Nett in 1973 [9]. GnRH was
iodinated by the modified chlomine-T technique[10]. Na125 I was
manufactured by Radiochemical Center, Amersham.
ß-EP RIA: The sensitive radioimmunoassay was a routine in our
laboratory [1]. The standards of human and rat ß-EP was synthesized
by Peninsula Laboratories, Inc. and the rabbit antiserum of both
ß-EP was developed in our laboratory. The cross-reaction from human
ß-EP and camel ß-EP was detected about 20%. The sensitivity of this
method was 10pg/tube.
LH, E2 and corticosterone RIA: LH, E2 and corticosterone RIA
kits were bought from Shanghai Institute of Biologic Products, the
Ministry of Health, P.R. China. All procedures of RIA were performed
as described in the kit manuals.
|
Fig. 1 |
A: |
Sketch of
ventral view (left) and dorsal view (right) of rat shows the
acupoints we used |
|
B: |
Diagram shows
the electroacupuncture procedures in conscious rat |
Staining techniques:
Vaginal smears were fixed by 100% ethyl alcohol, then stained with
HE method. Adrenal sections were cut in 4µm thickness from
paraffin blocks and processed with silver nitrate staining
technique[11]. In each case, one hundred cells in zona fascicula
were examined randomly under 100-fold oil immersion lens. Numbers
and sizes of AgNOR dots were counted and measured.
C-fos protein
immunohistochemistry: The
inmunohistochemical analysis of c-fos expression in rat brain was
perforrned as previously described[11].
Estrogen receptor (ER)
protein immunohistochemistry (ABC method):
Under sodium pentobarbital anesthesia (50 mg/kg, ip), the animals
were perfused via left cardiac ventricle with 100ml of
phosphate-buffered saline (PBS), followed by 300ml ice-cold
fixative containing 4% paraformaldehyde in 0.1 M phosphate buffer
(pH7.4). Afterwards, brain was removed with the same fixative for
one day and immersed in 0. lM phosphate buffer containing 30%
sucrose for another day. The hypothalamus blocks were frozen with
dry ice and cut into 35 µM thick section by cryostat. The brain
sections were washed with 0.01M PBS for 15min x 3 and incubated in
0.01M PBS containing 0.5% Triton 100 and 3% normal goat serum
(NGS) at 37°C-for one hour. Afterwards, the sections incubated in
1:1,000 ER monoclonal antibody (H222, Abott Co.) at 37°C for one
hour, then at 4°C for two days. The sections, washed in PBS three
times, were processed by ABC kit (from Vecot Labs) induding
sequential incubation at 20°C in the following solutions with
washes between them. (1). second antibody (dilution 1:100), 30min.
(2). A+B reagents (dilutionl:100), 60min. (3). 0.05%
diaminobenzidine/ 0.02% hydrogen peroxide in 0.1M Tris- HCI buffer
(pH 7.2) 10min. The sections were washed in tap water, mounted and
examined under light microscope. The certain areas of typical
immunoreactive positive neurons were measured by computer image
analysis system (Vecta PC).
ER mRNA hybridization:
The total mRNA of brain was eluted by the modified phenol method
[12]. ER cDNA probe (244bp) was labeled by the DlG-labeling kit
(from Bohringman Co., Germany). The dot blot hybridization was
processed as the method described by Sambrook J and his colleagues
[13]. The dot blot images were analyzed with gray density by
computer imaging analysis software (TJTY-300, from Tong -Ji
university, Shanghai, China).
Statistics:
All data in this paper were treated with analysis of variation
(ANOVA), least significant difference (ISD) or student T-test.
RESULTS
Effect of EA
on ovulatary induction and curing sterility in woman
After EA the blood ß-EP level of the patients resulting in
ovulation either declined or maintain at the levels within the
range of the normal levels and the ß-EP levels of those failing to
show ovulation were significantly higher than the normal's' (table
1). On the other hand, the blood LH and FSH levels of the patients
with ovulation after EA treatment tended to be the normal [14].
Table 1. Change of blood ß-EP level before and after EA
(pg/ml)
|
Group of
cases |
N |
Before EA |
After EA |
|
 |
|
Ovulation |
6 |
65.59 ±
24.15 |
*38.86 ±
10.11 |
|
No
ovulation |
7 |
65.59 ±
24.15 |
80.09 ±
22.16 |
|
Control |
5 |
38.84 ±
10.13 |
41.52 ±
6.40 |
The values in this table are mean±SE, *P<0.05
Effect of EA on dysfunction of HPOA in ovariectomized rats
For a further study of the mechanism of EA effect on HPOA a series
of experiments in the animal models was performed.
(1). EA induces maturation and exfoliation of vaginal
epithelium cell and enhances blood level of E2.
After ovariectomy two weeks late, the exfoliated epithelium cell
disappeared from the vaginal smears of the rats, but it reappeared
in the smears following EA treatment. The blood level of E2 in OVX
was increased significantly (table 2). No obvious change was seen
in INT after EA treatment and in OVX following EA treatment with
the control acupoints.
Table 2. The level of blood E2 following EA treatment (pg/ml)
|
Group |
N |
Before EA |
After EA |
|
|
|
OVX |
10 |
*5.47 ±
0.63 |
**11.58 ±
0.98 |
|
INT |
10 |
18.00 ±
3.26 |
18.34 ±
8.77 |
*P < 0.05 compared with INT, **P<0.01 compared with before EA
(2). EA promotes enlargement of adrenals and enhances activity
of adrenal AgNORs as well as blood level of corticosterone
We found the adrenals of OVX+EA were enlarged and the weight of
the adrenals was raised significantly. Using histochemical method,
the AgNORs of the cells in inner adrenal cortex were examined. The
result shows that the activity of AgNORs of OVX was enhanced
(table 3, 4), and the level of blood corticosterone in OVX+EA was
also increased (table 5). There were no similar effects in INT
following EA treatment and in OVX after EA with control acupoints.
Table 3. AgNORs number in OVX and INT
|
Group
N |
INT
4 |
INI+EA
3 |
OVX
4 |
OVX+EA
7 |
F value |
|
|
|
Number
of AgNORs
(mean/100 cells) |
1.55
1.82
1.24
1.30 |
1.19
1.28
1.16 |
1.25
1.61
1.66
1.96 |
2.53
2.05
1.82
2.86
2.86
2.93
3.92 |
9.614*
|
|
|
*P < 0.01 tested with ANOVA
Table 4. Weight of adrenal
|
Group
N |
INT
5 |
INI+EA
3 |
OVX
5 |
OVX+EA
8 |
F value |
|
|
|
Weight
(mg) |
57
56
57
43
57 |
54
57
58 |
45
68
56
50
58 |
67
72
66
71
57
74
74
68 |
5.825*
|
|
|
*P < 0.01 tested
with ANOVA
Table 5. The levels of blood corticosterone in OVX and lNT
(mean ± SE, ng/ml)
|
Group |
N |
Before EA |
After EA |
|
|
|
OVX |
12 |
4.78 ± 0.42 |
*6.06 ± 0.73 |
|
INT |
12 |
3.64 ± 0.15 |
4.76 ± 1.25 |
*P
< 0.001 compared with before EA
(3). EA decreases the level of hypothalamic GnRH, pituitary LH
and increases the contents of hypothalamic and pituitary
ß-endorphin
After EA treatment the levels of GnRH released from hypothalamus
was rnarkedly decreased however, the ß-endorphin (ß-EP) secretion
in hypothalamus was raised. The pituitary content of LH was also
fallen, but the ß-EP of pituitary was increased, as well as
peripheral LH and ß-EP level (Fig.2).
|
Fig. 2 |
Change of
hypothalarnic GnRH and ß-EP, pituitary LH and ß-EP, blood LH
and ß-EP before and after EA |
Effect of EA on brain c-fos expression in ovariectomized rats
The area occupied by FOS protein labeled neuron was detected in
medial preoptic nucleus (MPN), lateral preoptic nucleus (LPN),
suprachiasmatic nucleus (SCN), paraventricular nucleus of the
hypothalamus (PAVN), medial amygdala nucleus (MAN),
periventricular nucleus of the hypothaLsmus (PVN), ventromedial
nucleus of the hypothalamus (VNH) and arcuate nucleus (AR) 4 hours
after ovariectomy (fig. 3a). The C-fos immunoreactive labeled
neurons disappeared two weeks later following ovariectomy. The
rats recovering for more than two weeks after ovariectomy, were
received EA treatment. Many specific FOS labeled cells were
observed in LPN, VNH, SCN and especially in POA, ARN, and PVN, but
not any labeled neuron could be found in MAN. No obvious C-fos
expression was shown in those nuclei in INT and INT+EA (fig. 3b).
|
Fig. 3a |
C-fos
immunocytochemistry neurons distribution after ovariectomy |
|
Fig. 3b |
C-fos
expression labeled neurons following electroacupuncture |
Effect of EA on expression of ER protein and ER mRNA in rat
brain
Estrogen receptor (ER) immunoreactive neurons were observed widely
in rat brain with immunohistochemical technique, especially in MPN,
ARN and VNH. The above nuclei were measured by computer image
analysis system, and the results show that the mean gray density
in OVX+EA was decreased apparently compared with that in OVX.
Whereas there were no obvious changes of gray density levels in
INT and INT+EA (fig, 4).
|
Fig. 4 |
Effect of EA
on expression of ER protein in rat brain (Immunohistochernistry
of monoclonal antibody) *p < 0.01 compared with OVX |
The dot blot indicated that ER mRNA expression was increased about
48.11% in OVX compared with INT. The gray density of OVX was
129.75 ± l2.l3 and that in OVX+EA was 199.25 ± 5.75 attenuated
significantly (Fig. 5). The gray density level in INT was 87.60 ±
5.91, and the level in INT+EA was 83.60 ± 4.83. There was no
significant difference between INT and INT+EA
|
Fig. 5 |
Effect of EA
on expression of ER mRNA in rat brain (dot blot) *** p < 0.01
compared with OVX
|
DlSCUSSION
Since 1985 we have observed that the effect of EA ovulatary
induction might relate to the hand skin temperature (HST) and the
blood level of ß-EP [14]. On the other hand, after EA the blood
FSH and LH levels of the patients who successfully ovulated either
declined or maintained at normal. In general, provided that body
temperature was normal and the environmental temperature was
constant round 25°C, the HST may reflect the state of sympathetic
system of a patient. These results suggest that in anovulatary
cases the hyperactive sympathetic system can be depressed by EA
and the function of HPOA can be regulated by EA through central
sympathetic system. Moreover, EA may mediate the abnormal function
via the influence on the secretion of the hormones in the
different Level of HPOA.
To gain more evidences, we designed some animal experiments to
explain the mechanism of EA effects on HPOA at the whole, cellular
and molecular levels. We found that EA can induce maturation and
exfoliation of vaginal epithelium cell in OVX rat. It is known
that maturation and exfoliation of vaginal epithelium cells are a
reaction dependent on estrogen level. So we determined the level
of blood E2 in OVX and OVX+EA. The result shows the level of blood
E2 in OVX was lower than that in normal, but it was increased
significantly after OVX accepted EA treatment with the
experimental acupoints. This result suggests EA might promote the
activity of the compensative mechanism to elevate the subnormal
level of E2 induced by ovariectomy in rats.
What is this compensative mechanism? To resolve this question, we
considered that adrenal is the main organ to secrete sexual
hormones except ovarian in females and observed the adrenals of
the animals in four groups. The results show that the mean weight
of the adrenal in OVX+EA was higher than that in OVX, INT and
INT+EA, suggesting the adrenal function might be activated by EA.
Subsequently, we detected that the number of AgNORs in zona
fasciculata of OVX+EA was significantly increased. Nucleolar
organizer regions (NORs) are loops of DNA, which possess ribosomal
RNA (rRNA) genes. They are of vital significance in the ultimate
synthesis of protein. Thus, the number and configuration of AgNORs
(NORs stained by silver staining method) may reflect the activity
of cell differentiation and transcription of nucleolar rDNA [15].
In the same time we found the content of blood corticosterone in
OVX+EA was raised markedly, but there was no change of blood
corticosterone in OVX, INT and INT+EA. This result provided a
further evidence that the adrenal cortex cells were initiated in
OVX+EA.
The results including the changes of GnRH releasing from
hypothalamus and of the pituitary and blood LH contents suggest
that the effects of acupuncture in the regulation of HPOA may be
exerted via to promote the function of hypothalamic
pituitary-adrenal axis (HPAA), increasing the synthesis and
secretion of adrenal steroid horrnones, the androgen of which then
be transformed into estrogen in other tissues and thereby reset
the negative feedback of estrogen to HPOA. Moreover, EA may
accelerate the release of brain and pituitary ß-EP to inhibit the
overnormal secretion of GnRH and LH that may be normalized.
Recently immunohistochemical analysis of the expression of
oncogene c-fos ABl was induced by variety of stimuli [16, 17].
This represents a new method for mapping neuronal activity at the
cellular level [18] and thus functionally and systematically
tracing neuronal pathway in the nervous system (C NS) [19]. We
used this method to examine the distribution of FOS labeled neuron
in CNS for recovery of more evidences that EA may alter the
neuroendocrine function of HPOA in ovariectomized rats in cellular
and gene level. The results show that the specific FOS labeled
neurons were observed especially in POA, ARN and PVN in OVX
following EA treatment. In above nuclei there were a high
concentration of GnRH and ß-EP neuron [20]. These results suggest
this fact that the expression of FOS labeled neurons reappeared in
above mentioned areas following EA treatment in ovariectomized
rats may be related to the changes of GnRH and ß-EP from rat
hypothalamus after EA treatment.
The level of estrogen in the body may regulate the expression of
ER, which may by down-regulated following increase of estrogen
level and up-regulated after decrease of estrogen [22]. Our
finding that after decline of blood E2 induced by ovariectomy the
expression of ER was increased and the expression of ER was
inhibited by EA inducing the elevation of blood E2 are in
accordance with these reported results. ER existing in the brain,
especially in POA, ARN and VHN may mediate the function of
neuroendocrine system [22, 23]. Thus, our observations suggest
that the influence of EA on the change of ER expression in brain
may be one of further mechanisms of EA normalizing the dysfunction
of HPOA.
INT rats as experimental control we adopted were all of in the
stage of preestrus and estrus because the animal sexual hormes and
brain ER expressions were changed with the sexual cycle [24]. All
INT rats were selected to fix in the two stages there may be a
relative constant comparability.
Our results show no same effects were seen after EA treatment in
INT and following EA with control acupoints in OVX, suggesting
that EA may possess a relative specificity on acupoint and the
effect of EA may be a kind of normalization.
CONCLUSION
Our observations reveal that acupuncture may regulate the abnormal
function of HPOA in many ways, which means that acupuncture may
activate C-fos expression of brain, then a long term changes at
molecular level would start, following the regulation of gene
expression in FOS relative gene, such as ER mRNA and GnRH mRNA
involved. On the other hand, EA may promote the activity of the
body compensative mechanisms, then the levels of hormones, such as
GnRH, LH, estrogen and so on would be normalized. The effect of
acupuncture on regulating the function of HPOA may possess a
relative specificity of acupoint. Moreover, our clinical and
animal experimental results suggest that it is necessary for
obtaining a satisfactory effect that proper stimulation should be
about thirty minutes Q.D. for three days. This suggestion provides
a successful consideration for clinical practice in curing the
woman patients with dysfunction of sexual endocrine, such as
primary ovarian dysfunction, climacteric syndrom, after-ovariectomy
and polycystic ovarian disease etc.
ACKNOWLEDGMENT
The work was supported by National Natural Foundation of China
(3880910 and 392708340) and a grant from the State Key Laboratory
of Medical Neurobiology of China (92003).
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