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and Heat Shock Protein 90 Messenger Ribonucleic Acid in the Gravid Horn and Nongravid Horn in Sheep during Betamethasone-Induced Labor1
Laboratory for Pregnancy and Newborn Research, Cornell University College of Veterinary Medicine, Ithaca, New York 14853
Address all correspondence and requests for reprints to: Dr. Peter W. Nathanielsz, Laboratory for Pregnancy and Newborn Research, Department of Biomedical Sciences, Cornell University College of Veterinary Medicine, Ithaca, New York 14853-6401. E-mail: pwn1{at}cornell.edu
In the present study, we characterized four myometrial
contraction-associated proteins (mCAPs): oxytocin receptor (OTR),
prostaglandin H synthase 2 (PGHS2), estrogen receptor
(ER
), and
heat shock protein 90 (Hsp90) messenger RNA (mRNA) expression in the
nongravid horn of pregnant sheep and compared them with their
expression in the gravid horn that is exposed to a greater degree of
stretch. We also examined the regulatory effects of estrogen and
progesterone on OTR mRNA expression in ovariectomized nonpregnant
sheep. In addition, we determined the ontogeny of mCAP expression in
the gravid horn throughout late pregnancy and during spontaneous term
labor. Gravid horn and nongravid horn myometria were removed under
general anesthesia from control ewes not in labor at 130140 days
gestational age (dGA; n = 3) and during betamethasone-induced
labor (n = 6) at the same gestational age. Gravid horn myometrium
was also collected from ewes not in labor at 95 dGA (n = 3),
101110 dGA (n = 3), 111120 dGA (n = 3), 121130 dGA
(n = 3), 131140 dGA (n = 3), and 141145 dGA (n = 4)
and from ewes in spontaneous term labor (n = 4). All ewes were
carrying single fetuses. Myometrium was also collected from
ovariectomized nonpregnant ewes treated with saline (n = 5),
estradiol (50 µg/day; n = 5), progesterone (0.3 g,
intravaginally; n = 5), and estradiol plus progesterone (n =
5). Myometrial RNA was extracted and analyzed by Northern blot for OTR,
PGHS2, ER
, and Hsp90 mRNA, normalized for 18S ribosomal RNA or
ß-actin. ER
, Hsp90, OTR, and PGHS2 mRNA were all significantly
up-regulated during betamethasone-induced labor (P
< 0.01) in gravid and nongravid horn myometrium. The level of gravid
horn OTR mRNA during labor was 3 times the level of nongravid horn OTR
mRNA (P < 0.0001). Gravid horn PGHS2 mRNA was also
higher than nongravid horn PGHS2 (P < 0.02). In
contrast, in spontaneous term labor nongravid horn, ER
and Hsp90
mRNA were similar to gravid horn. Myometrial ER
and Hsp90 mRNA
remained unchanged throughout late pregnancy and increased at
spontaneous term labor (P < 0.05). In contrast,
myometrial OTR increased around 130 dGA (P < 0.01)
and further increased at spontaneous term labor (P
< 0.02). Progesterone significantly inhibited myometrial OTR mRNA
expression in nonpregnant sheep and estradiol antagonized
progesterones inhibitory effect. Mechanical stretch differentially
regulated mCAP mRNA expression in the ovine gravid horn and nongravid
horn. Mechanical stretch appears largely responsible for increased OTR
mRNA and to a lesser degree PGHS2 mRNA. In addition, endocrine factors
may be required for full activation of OTR and PGHS2 mRNA associated
with labor. ER
and Hsp90 mRNA are not under the control of uterine
stretch in keeping with our previous results, indicating that systemic
hormones such as estradiol, are prime regulators for these two mCAP
mRNA expression during labor.
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