| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
|
|
|
|||||||
|
|||||||||
J. Biol. Chem., Vol. 277, Issue 24, 21468-21473, June 14, 2002
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
From the Departments of Biological Chemistry and
Obstetrics/Gynecology, University of Michigan Medical School, Ann
Arbor, Michigan 48109-0617
Received for publication, December 6, 2001, and in revised form, February 26, 2002
Luteinizing hormone (LH) receptor mRNA is
post-transcriptionally regulated. An ovarian cytosolic LH receptor
mRNA-binding protein (LRBP) identified in our laboratory binds to a
polypyrimidine-rich bipartite sequence in the coding region of LH
receptor mRNA. The present studies show a role for LRBP in the
regulation of LH receptor mRNA. We demonstrated that increased LH
receptor mRNA degradation occurs during hormone-induced LH receptor
down-regulation. Furthermore, increased degradation of LH receptor
mRNA was seen when partially purified LRBP was included in an
in vitro mRNA decay reaction. The LH receptor mRNA
binding activity of LRBP measured by RNA electrophoretic mobility shift
analysis showed an inverse relationship to LH receptor mRNA levels
during different physiological states. These results suggest that LRBP
is a physiological regulator of LHR mRNA expression in the ovary
and provides a novel mechanism for the regulation of LH receptor
expression in the ovary.
The expression of luteinizing hormone receptors
(LHR)1 on the rat ovarian
granulosa cells and luteal cells is decreased by an endogenous
preovulatory luteinizing hormone (LH) surge or by the administration of
a pharmacological dose of human chorionic gonadotropin (hCG), a
placental counterpart of LH (1-4). Studies from our laboratory have
demonstrated that the decline in cell surface LHR number seen after hCG
administration is paralleled by a specific loss of LHR mRNA (2, 3).
Following the injection of a bolus of hCG in female rat, a rapid
decline in the steady-state levels of all four LHR mRNA transcripts
(6.7, 4.4, 2.6, and 1.8 kb) is seen in luteal cells within 12 h
with a complete loss occurring by 24 h. This selective loss is
followed by a recovery of receptor mRNA expression between 24 and
48 h (2). We have shown that the loss of LHR mRNA does not
result from decreased transcription but occurs post-transcriptionally
with an approximate 3-fold decrease in half-life (4). Additional
studies led to the identification of a 50-kDa LHR mRNA-binding
protein designated as LRBP in rat and human ovarian cytosolic
fractions. During hormone-induced down-regulation of the LHR, the LHR
mRNA binding activity of LRBP was increased. LRBP specifically
binds to the coding region of LHR mRNA with an apparent
dissociation constant of 10-9 M (5, 6). These
studies were carried out to determine the role of LRBP in LHR mRNA
degradation in vitro as well as to establish a relationship
between LHR mRNA expression and LRBP during ovarian development.
Our results show that LHR mRNA expression inversely correlates with
the LHR mRNA binding activity of LRBP during follicular maturation,
ovulation, and luteinization. Furthermore, a partially purified LRBP
causes accelerated decay of LHR mRNA in an in vitro reconstituted mRNA decay system.
Chemicals--
Pregnant mare serum gonadotropin was purchased
from Calbiochem. Human chorionic gonadotropin was obtained from Sigma.
[ Animals and Tissues--
Pseudopregnancy was induced in
21-day-old Sprague-Dawley female rats by a subcutaneous injection of 50 IU of pregnant mare serum gonadotropin followed by 25 IU of hCG 56 h later. The day of hCG injection is taken as day 0. LH receptor
down-regulation was induced by the injection of 50 IU of hCG on the
fifth day of pseudopregnancy. Ovaries were collected at the indicated
times and were processed immediately.
Preparation of Polysomes--
Ovaries from control
(pseudopregnant) and hormone-treated (12-h post-hCG-injected) animals
were homogenized in solution A (1 mM potassium acetate, 2 mM Mg(Ac)2, 2 mM
dithiothreitol, and 10 mM Tris acetate, pH 7.6) at
4 °C. After centrifugation for 10 min at 10,000 × g, the supernatants were layered over a cushion of solution
B (solution A containing 30% sucrose) and centrifuged at 130,000 × g for 2.5 h. The polyribosome pellets were
resuspended in solution A and stored at In Vitro mRNA Decay Assay--
Half-life of LHR mRNA was
determined by an in vitro decay reaction based on the
protocol developed by Ross (7). An A260 of
0.6-1.0 units of polysomes were mixed gently in 25 µl (final volume) of solution A (as described under polysome isolation) supplemented with 10 mM creatine phosphate, 0.04 mg/ml
creatine kinase, 1 mM ATP, 0.2 mM GTP, 0.1 M potassium acetate, 0.1 mM spermine, 0.8 mM Mg(Ac)2, and placental RNase inhibitor (400 units/ml). The in vitro decay reactions were incubated at
16 °C for 0, 15, 30, 60, and 120 min. Where indicated, total RNA
isolated from control pseudopregnant rat ovaries and partially purified
LRBP were also included in the reaction. After incubation at intervals shown above, the reactions were stopped, RNA in the reaction tubes was
extracted immediately using the acid guanidinium isothiocyanate method
as described by Chomczynski and Sacchi (8), and LHR mRNA was
detected by Northern blot analysis as described below. The 6.7-kb LHR
mRNA (major transcript) was quantitated in densitometric units
using NIH image 1.61 software. The half-life (t1/2) of LHR mRNA was calculated by plotting the corresponding
densitometric units of LHR mRNA versus incubation time.
Northern Blot Analysis--
Total RNA was extracted using a
previously described procedure (8). Ovaries were homogenized in a
solution of guanidine isothiocyanate, acidified with 2 M
sodium acetate, pH 4.0, and extracted with water-saturated phenol and
chloroform-isoamyl alcohol (49:1). RNA was precipitated at Partial Purification of LRBP--
Purification of LRBP from rat
ovary was performed as described previously (6). Ovaries were
homogenized in buffer A (10 mM HEPES, pH 7.9, 0.5 mM MgCl2, 50 µM EDTA, 5 mM dithiothreitol, and 10% glycerol) containing 50 mM KCl and EDTA-free protease inhibitor mixture at 4 °C.
The homogenate was centrifuged at 105,000 × g for 90 min at 4 °C. The supernatant (S-100) was applied to a Macro-Prep
High S Support (strong cation exchange support) column equilibrated
with Buffer A containing 50 mM KCl. The column was washed
with Buffer A containing 50 mM KCl until the absorbance at
280 nm was <0.02. The proteins were then eluted with Buffer A
containing 150 mM KCl. The column eluates were desalted to
50 mM KCl in buffer A containing EDTA-free complete
protease inhibitor mixture using Centricon YM-10 microconcentrators,
and protein concentrations were determined by BCA (Pierce).
Preparation of Full-length LHR mRNA--
The 2.1-kb LHR
cDNA containing the full-length LHR coding region was ligated into
pBluescript II between XbaI and BamHI sites and
was used to generate full-length LHR mRNA. Radiolabeled RNA was
prepared from linearized template using mMessage mMachine kit in the
presence of 100 µCi of [32P]UTP. Following
transcription, RNA was extracted with nuclease-free water-saturated
phenol-chloroform-isoamyl alcohol (50:49:1). Unincorporated nucleotides
were removed from the labeled RNA using Quik spin columns
(G-50-Sephadex). RNA was precipitated with equal volume of isopropyl
alcohol at -20 °C. Precipitated RNA was then washed with 75%
ethanol air-dried and was dissolved in nuclease-free water.
RNA Gel Shift Analysis--
Unless otherwise indicated, RNA gel
shift analysis was performed as described previously (6). Protein
samples were incubated with 1 × 105 cpm of
radiolabeled gel-purified RNA in homogenization buffer A described
above in the presence of 5 µg of tRNA and 40 units of RNasin at
30 °C for 10 min. Unprotected radiolabeled RNA was then degraded by
the addition of 2 units of RNase T1 at 37 °C for 30 min. Samples
were then incubated with heparin at a final concentration of 5 mg/ml
for 10 min on ice to decrease nonspecific binding. The RNA-protein
complexes were resolved by 8% native polyacrylamide gel
electrophoresis at 4 °C. The gel was then dried and exposed to Kodak
X-Omat AR film and visualized by autoradiography. Radiolabeled
bands were quantitated in densitometric units using NIH image 1.61 software.
Statistical Analysis--
Each experiment was repeated at least
three times, and the results presented represent a single experiment.
Error bar represents the mean ± S.E. of three separate
densitometric scans.
In Vitro Decay of Endogenous and Exogenous LHR mRNA--
The
decay of endogenous and exogenously provided LHR mRNA was examined
in a cell-free system. The polysomes were isolated from day 5 pseudopregnant rat ovaries when LHR mRNA expression was abundant.
The decay of endogenous LHR mRNA associated with polysomes was
determined by incubating polysomes in in vitro decay reactions as described under "Materials and Methods." The
incubations were carried out at 16 °C for 0, 15, 30, 60, and 120 min. At the end of this incubation period, total RNA was extracted from
each fraction, and LHR mRNA was determined by Northern blot using a LHR cDNA probe. The results presented in Fig.
1A show all four LHR mRNA
transcripts (6.7, 4.4, 2.6, and 1.8 kb) endogenously associated with
the polysomes remaining at different time intervals. The loss of all
four transcripts occurred concomitantly. The 6.7-kb transcript is the
predominant LHR mRNA in rat ovary. Panel C represents the rate of degradation in densitometric units of the 6.7-kb transcript in panel A normalized to 18 S rRNA. The degradation of
endogenous LHR mRNA occurred rapidly (t1/2 = 38 min), and by 120 min, there were minimal detectable levels of LHR
mRNA remaining. Panel B shows 18 S rRNA determined by
Northern blot hybridization for normalizing RNA loading. The level of
18 S rRNA was not altered during the 120-min incubation period. Because the degradation of endogenously associated LHR mRNA occurred
rapidly, in subsequent experiments 15 µg of total RNA extracted from
pseudopregnant rat ovaries were included to ensure that RNA was not
limiting in the in vitro decay reaction.
Because our previous studies have shown that the degradation of LHR
mRNA occurs more rapidly during hormone-induced down-regulation (2-4), attempts were made to examine whether the decay of exogenous LHR mRNA by polysomes from LHR-down-regulated rat ovaries occurred at a rate faster than the degradation of exogenous LHR mRNA by polysomes isolated from control ovaries. For this study, polysomes were
isolated from both LHR-down-regulated and control ovaries. Reactions
containing polysomes from control and LHR-down-regulated ovaries were
then separately incubated with exogenously added total RNA for up to
120 min, and the reactions were terminated at different time intervals
as shown in Fig. 2. RNA was extracted, and Northern blot hybridization was performed using LHR cDNA probe. Panel A shows the 6.7-kb LHR mRNA transcript remaining
at different time intervals in each group. Panel C shows 18 S rRNA in each fraction. Panel D depicts the densitometric
scans of the 6.7-kb transcript (major transcript in rat ovary) in
panel A normalized for 18 S rRNA. The results show that the
decay of exogenously added LHR mRNA occurred with a
t1/2 of 46 min when incubated in decay reactions
using polysomes isolated from control ovaries. The decay of exogenous
LHR mRNA proceeded at a markedly faster rate with a
t1/2 of ~10 min in the decay reactions with
polysomes isolated from hormone-induced LHR-down-regulated rat ovaries.
To determine whether this rapid degradation of LHR mRNA by
polysomes from LHR-down-regulated rat ovaries was selective for LHR
mRNA, we examined the degradation of cholesterol side-chain
cleavage enzyme cytochrome P450scc mRNA by stripping the same blot
and rehybridizing with [32P]cytochrome P450scc cDNA
probe as described under "Materials and Methods." Fig.
2B shows the cytochrome P450scc mRNA remaining at
different time intervals of the in vitro degradation
reaction in each group. Panel D depicts the rate of
degradation in densitometric units of cytochrome P450scc in panel
B normalized to 18 S rRNA (panel C) for the difference,
if any, in RNA loading. There was no discernible difference in the rate
of degradation of cytochrome P450scc between control and
LHR-down-regulated groups. This finding indicates that the LHR mRNA
degradation by polysomes from LH receptor-down-regulated rat ovaries is
selective for LHR mRNA.
LHR mRNA Degradation in Vitro by Partially Purified
LRBP--
To determine whether the partially purified LHR
mRNA-binding protein LRBP induces accelerated decay of LHR mRNA
in vitro, polysomes isolated from control ovaries were
incubated with exogenously added LHR mRNA and partially purified
LRBP. The assays were carried out as described under "Materials and
Methods." Aliquots of decay reactions were incubated for 0, 15, 30, 60, and 120 min at 16 °C, and LHR mRNA content was detected by
Northern hybridization analysis (Fig.
3A). An addition of partially
purified LRBP (70 µg) increased the degradation of LHR mRNA when
compared with incubations with no LRBP. The decay of LHR mRNA was
so rapid that there was an undetectable level of the 6.7-kb transcript
at 120 min. Half-lives of LHR mRNA were calculated from the
densitometric scans of the 6.7-kb transcript in decay reactions
performed in the presence of LRBP or with equal volume of buffer as
shown in Fig. 3B. The t1/2 of exogenously
added LHR mRNA was reduced to 26 min in the presence of partially
purified LRBP. The t1/2 of LHR mRNA in control
reactions was 38 min. To address whether the degradation of LHR
mRNA is dependent on LRBP concentration, in vitro decay
reactions with control polysomes and exogenously added LHR mRNA
were performed with different concentrations (9.6, 19.2, 38.5, and 77 µg) of partially purified LRBP at 16 °C for 60 min. As shown in
Fig. 4, an increased degradation of LHR
mRNA was observed by increasing the LRBP concentration in the decay
reactions when compared with that seen in its absence. These data
indicate that LRBP, which binds to the coding region of LHR mRNA,
causes an accelerated and
concentration-dependent degradation of the
mRNA.
Changes in LHR mRNA Binding Activity of LRBP during
PMSG and hCG-induced Regulation of LHR
mRNA--
Experiments were then conducted to determine
whether LHR mRNA binding activity of the LRBP present in the
ovarian S-100 fractions bears any relationship to the steady-state
levels of LHR mRNA. First, the changes in LHR mRNA binding
activity of the LRBP and LHR mRNA expression were determined after
hormone treatment. 21-day-old rats were treated with 50 IU of
PMSG to induce follicular maturation, and ovaries were collected
56 h later. LHR mRNA expression was examined by Northern blot
analysis and the LHR mRNA binding activity of LRBP by RNA
electrophoretic mobility shift analysis using the S-100 fractions
isolated from the ovaries. The results (Fig.
5, A, C, and
D) show that expression of LHR mRNA increased slightly 56 h after PMSG injection, but LRBP activity in the S-100 fraction showed a decline at this time interval compared with the pretreatment level. The PMSG-treated animals were then treated with 25 IU of hCG to
induce ovulation and corpus luteum formation. Ovaries were collected at
6, 12, 24, 48, and 72 h after hCG injection to determine LHR
mRNA expression and the LHR mRNA binding activity of LRBP. Upon
treatment with hCG, as expected, the levels of LHR mRNA started to
decline by 6 h and reached the lowest level by 12 h. The LHR mRNA expression started to increase by 24 h and further
increased by 72 h (Fig. 5, A and D)
following hCG treatment. RNA electrophoretic mobility shift analysis
was performed in S-100 fractions prepared from ovaries collected at the
same time intervals as those used for determining LHR mRNA levels.
The intensities of the ribonucleoprotein complexes formed (Fig.
5C) were quantitated by densitometric scanning (Fig.
5D). The results show that following hCG injection, the LHR
mRNA binding activity of LRBP showed an increase at 6 and 12 h. The LHR mRNA binding activity of LRBP in the S-100 fractions started to decrease by 24 h after hCG injection. This finding is
in sharp contrast to the pattern of LHR mRNA expression seen at
different time intervals following hCG treatment. The results show that
in all instances the expression of LHR mRNA inversely correlated
with the LHR mRNA binding activity of LRBP.
LHR mRNA Expression and LHR mRNA Binding Activity of LRBP
during Pseudopregnancy--
Because the corpus luteum has a defined
life span and the expression of LHR mRNA shows marked changes
during this period, both LHR mRNA levels and the LHR mRNA
binding activity of LRBP were assayed to examine whether a correlation
exists between the two.
Pseudopregnancy was induced by a subcutaneous injection of 50 IU of
PMSG to 21-day-old rats followed by treatment with 25 IU of hCG 56 h later. The day of hCG injection was taken as day 0 of
pseudopregnancy. Ovaries were collected at 2, 4, 6, 8, 10, 12, and 14 days of pseudopregnancy for LHR mRNA expression and RNA
electrophoretic mobility shift studies as described in earlier experiments and under "Materials and Methods." Fig.
6A represents the Northern
blot showing the expression of LHR mRNA at different days of
pseudopregnancy. Following a steady increase in LHR mRNA expression
culminating in maximum expression on day 8, a sharp decline was seen
after day 8 of pseudopregnancy extending to day 14. The LHR mRNA
binding activity of LRBP in ovarian S-100 fractions at the same time
interval is shown in Fig. 6C, and the intensities of these
ribonucleoprotein complexes were quantitated densitometrically (Fig.
6D). The results show that the LHR mRNA binding activity of LRBP increased from days 4-10 of pseudopregnancy. The maximum binding activity of LRBP was observed on day 10 of pseudopregnancy. The
binding activity of LRBP started decreasing from day 10 but remained
higher than the levels seen on days 6 and 8. Taken together, these
results show that the LHR mRNA binding activity of LRBP is
inversely related to LHR mRNA expression.
Differences in expression of the LH receptor observed during
follicular development, ovulation, and luteinization involve concomitant changes in the steady-state levels of LH receptor mRNA
(1, 2, 11-13). Previous studies have shown that during hCG-induced
down-regulation of the LH receptor, the steady-state levels of LHR
mRNA show a dramatic decline (2). Furthermore, it has been shown
that the selective loss of LH receptor mRNA is because of increased
mRNA degradation rather than decreased transcription (4).
We have recently identified a 50-kDa LHR mRNA-binding protein on
native acrylamide gel designated as LRBP that is induced during
down-regulation of the LH receptor (5). The present studies have
examined the role of LRBP in LHR mRNA degradation during
hCG-induced down-regulation of LH receptor. We have used an in
vitro mRNA decay system to determine the effect of LRBP on the
stability of LHR mRNA. In general, cell-free mRNA turnover systems afford many benefits for studying mRNA degradation.
Although decay rates of mRNA in vitro generally occur at
slower rates than in intact cells, the relative rates of turnover of
different mRNAs are maintained. Moreover, the rates of mRNA
degradation can be measured without the necessity of transcriptional
repressing agents, which are generally nonspecific and cytotoxic. The
in vitro mRNA decay reactions performed with polysomes
isolated from control and hCG-induced LHR-down-regulated ovaries permit
reconstitution of LHR mRNA-degradative activity in a cell-free
system. The accelerated degradation of LHR mRNA in the presence of
partially purified LRBP in vitro presented in this report
indicates that LRBP acts as a trans-acting factor to induce
the decay of LHR mRNA.
Earlier studies from our laboratory have shown that the LHR mRNA
binding activity of LRBP in the ovarian S-100 fraction increases during
hCG-induced down-regulation of LH receptor (5). Hormonal manipulation
of rats has been shown to cause changes in LHR mRNA expression
(1-3, 12, 13). Using this paradigm, we have examined the relationship
between LRBP activity and LHR mRNA expression. The data presented
in this report (Figs. 5 and 6) clearly show that when the expression of
LHR mRNA is low, the ovarian S-100 fractions yields higher levels
of ribonucleoprotein complexes, establishing an inverse relationship
between LHR mRNA expression and LHR mRNA binding activity of
LRBP. This inverse relationship suggests that LRBP might play a role in
the accelerated degradation of LHR mRNA in vivo. This
possibility is supported by the observation that LHR mRNA
degradation is accelerated by the addition of LRBP in the in
vitro decay assay (Figs. 3 and 4). We have found that LRBP binds
to a polypyrimidine-rich bipartite sequence in the coding region of LHR
mRNA (5'-202UCUCX7UC
UUCCU220-3') with an apparent dissociation constant
of 10 A number of cytoplasmic proteins, some of which shuttle between nucleus
and cytoplasm, have been identified as either RNA-stabilizing or
destabilizing trans-acting factors (14-17). Studies in a
variety of systems have demonstrated the presence of binding sites for trans-acting factors in the coding region of mRNA
(18-23) similar to that seen in this study. For example, the
post-transcriptional regulation of tropoelastin mRNA in response to
transforming growth factor *
This work was supported in part by National
Institutes of Health Grant HD-06656 (to K. M. J. M.) and Predoctoral
Fellowship National Institutes of Health Training Grant
PR5-T32-HD-07048 (to J. C. K.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
To whom correspondence should be addressed: Depts. of Biological
Chemistry and Obstetrics and Gynecology, University of Michigan Medical
School, 6428 Medical Sciences Building I, 1301 Catherine, Ann Arbor, MI
48109-0617. Tel.: 734-764-8142; Fax: 734-936-8617.
Published, JBC Papers in Press, April 8, 2002, DOI 10.1074/jbc.M111653200
The abbreviations used are:
LHR, luteinizing
hormone receptors;
LH, luteinizing hormone;
hCG, human chorionic
gonadotropin;
LRBP, LH receptor mRNA-binding protein;
PMSG, pregnant mare serum gonadotropin.
Post-transcriptional Regulation of Luteinizing Hormone Receptor
mRNA in the Ovary by a Novel mRNA-binding Protein*
,
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
MATERIALS AND METHODS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-32P]dCTP was purchased from ICN (Costa Mesa, CA),
and [-32P]UTP was from PerkinElmer Life
Sciences. EDTA-free protease inhibitor mixture tablets, RNase
T1, and Quik spin columns (G-50-Sephadex) for radiolabeled RNA
purification were obtained from Roche Molecular Biochemicals. mMessage
mMachine Kit was a product of Ambion (Austin, TX). RNasin was purchased
from Promega (Madison, WI). Macro-prep High S Support column was
obtained from Bio-Rad. Centriplus YM-10 and Centricon YM-10
microconcentrators were products of Millipore (Bedford, MA).
80 °C. Quantitation of
polysomes was performed by measuring the absorbance at 260 nm.
20 °C
using three volumes of ethanol and was quantified by UV-absorbance
spectroscopy. Northern blot hybridization analysis was performed
essentially as described by Maniatis and colleagues (9). The LHR
cDNA probe used for Northern blot hybridization has been described
earlier (4). A 1.7-kb cDNA for human cytochrome P450scc was used as
probe for Northern blot analysis (10). The intensity of LHR and P450scc mRNA was quantified in densitometric units and normalized to 18 S rRNA.
RESULTS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
View larger version (25K):
[in a new window]
Fig. 1.
In vitro decay of
polysome-associated LHR mRNA. A, autoradiogram of
Northern blot hybridization analysis of all four endogenous LH receptor
mRNAs associated with polysomes isolated from control ovary and
incubated for 0, 15, 30, 60, and 120 min at 16 °C. Blots were probed
using a labeled cDNA corresponding to the LH receptor carboxyl
terminus and a portion of the 3'-untranslated region (nucleotides
1936-2682). B, the blot was stripped and rehybridized with
cDNA for 18 S rRNA. The rate of degradation of 6.7-kb transcript in
densitometric units is shown in C.
View larger version (29K):
[in a new window]
Fig. 2.
In vitro decay of LH receptor
mRNA and cytochrome P450scc mRNA associated with control and
LHR-down-regulated polysomes. A, autoradiogram of
Northern blot hybridization analysis of 6.7-kb LH receptor mRNA
content in cell-free mRNA decay reactions containing polysomes
isolated from control and 12-h-down-regulated ovaries incubated in the
presence of 15 µg exogenously added total RNA for 0, 15, 30, 60, and
120 min at 16 °C. Blots were probed using a labeled cDNA
corresponding to the LH receptor carboxyl terminus and a portion of the
3'-untranslated region (nucleotides 1936-2682). B,
autoradiogram of Northern blot hybridization analysis of cytochrome
P450scc associated with control and LHR-down-regulated polysomes. The
LH receptor mRNA and cytochrome P450scc mRNA remaining in each
time interval in A and B were quantitated by
densitometric scanning and normalized for 18 S rRNA as shown in
D. The blot was stripped and rehybridized with a cDNA
probe for 18 S rRNA (C).
View larger version (21K):
[in a new window]
Fig. 3.
LHR mRNA degradation in vitro
in the presence of partially purified LRBP. LH receptor
mRNA decay was examined in reactions containing 1 optical density
unit of polysomes isolated from control pseudopregnant rat ovaries and
exogenously added LHR mRNA. Aliquots of decay reactions were
incubated for 0, 15, 30, 60, and 120 min in the absence or in the
presence of LRBP (70 µg). LHR mRNA content was assayed at each
interval by Northern blot analysis (A). Half-lives of the
exogenous LHR mRNA were calculated using densitometric scans of the
6.7-kb transcript (B).
View larger version (77K):
[in a new window]
Fig. 4.
LRBP dose response on LHR mRNA decay
in vitro. In vitro decay reactions
were performed as described under "Materials and Methods." Aliquots
of the decay reactions were incubated for 60 min in the absence of
added protein (C) and in the presence of increasing
concentrations of LRBP (9.6-77 µg). LHR mRNA content was assayed
by Northern blot analysis, quantitated by densitometric scanning, and
normalized for 18 S rRNA.
View larger version (34K):
[in a new window]
Fig. 5.
LHR mRNA expression and RNA binding
activity of LRBP during PMSG and hCG-induced regulation of LHR
expression. Immature rats were injected with PMSG at 0 h. Ovaries were collected at 0 and 56 h later, at which time hCG
was administered. Ovaries were subsequently collected at 6, 12, 24, 48, and 72 h. A, LHR mRNA levels were obtained by
Northern blot analysis. B, the Northern blot was normalized
using 18 S rRNA. C, RNA electrophoretic mobility shift
analysis was performed for these time points using 50 µg of protein
from the isolated ovarian S-100 extracts and radiolabeled LHR mRNA.
D, the 6.7-kb LHR mRNA transcript and RNA
electrophoretic mobility shift analysis bands were quantitated by
densitometric scan and expressed in arbitrary units.
View larger version (36K):
[in a new window]
Fig. 6.
LHR mRNA expression and RNA binding
activity of LRBP during corpus luteum life span. Ovaries were
collected from PMSG/hCG-primed rats on days 2, 4, 6, 8, 10, 12, and 14 of pseudopregnancy. A, LHR mRNA levels were obtained by
Northern blot analysis. B, the Northern blot was normalized
to18 S rRNA. C, the RNA binding activity of LRBP was
measured by RNA electrophoretic mobility shift analysis using 50 µg
of S-100 extract. D, the 6.7-kb LHR mRNA transcript and
RNA electrophoretic mobility shift analysis bands were quantitated by
densitometric scanning and expressed in arbitrary units.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
9 M (5). LRBP could function by
targeting an endonuclease to LHR mRNA either by direct interaction
or by targeting the receptor mRNA to a particular location in the
cytoplasm where mRNA degradation occurs. The increased LHR mRNA
decay activity seen under in vitro conditions in the
presence of LRBP is an indication that LRBP is one of the
trans-acting factors involved in LHR mRNA degradation. It is possible that other proteins associated with the ribosomes might
also participate in the decay process.
1 is very similar to the LHR mRNA
regulation that we describe in this report. Similar to our system,
tropoelastin mRNA contains an 18-nucleotide cis-acting
motif near the 5' end of the coding region, and a 50-kDa cytosolic
protein interacts with this cis-acting motif causing
destabilization of the mRNA (24). c-Fos and c-Myc mRNAs
are some of the other well characterized mRNAs that contain binding
sites in the coding region for trans-acting factors (19, 21,
22, 25, 26). The present studies clearly show that the LHR
mRNA-binding protein LRBP, which binds to a region between nucleotides 188 and 228 in the open reading frame of LHR mRNA, plays a crucial role in the hormonal control of LHR mRNA stability. The mechanisms, which regulate the degradation of LHR mRNAs, are not clearly understood, although several mechanisms that involve deadenylation, decapping, and exonucleolytic and endonucleolytic degradation of eukaryotic mRNAs have been proposed (18, 27, 28).
Regulated degradation of mRNA allows rapid cessation of protein
synthesis without the need to alter transcription rates. The ability to
regulate receptor protein expression at the level of mRNA
degradation not involving changes in rate of transcription as
demonstrated here provides a novel strategy for the control of gene
expression under selective physiological or pharmacological states. The
present study provides for the first time a novel mechanism by which
LHR mRNA is regulated by altering the rate of mRNA degradation.
FOOTNOTES
Present address: Dept. of Microbiology, University of Washington
Medical School, Seattle, WA 98195.
ABBREVIATIONS
REFERENCES
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
1.
LaPolt, P. S.,
Oikawa, M.,
Jia, X. C.,
Dargan, C.,
and Hsueh, A. J.
(1990)
Endocrinology
126,
3277-3279[Abstract]
2.
Hoffman, Y. M.,
Peegel, H.,
Sprock, M. J.,
Zhang, Q. Y.,
and Menon, K. M. J.
(1991)
Endocrinology
128,
388-393[Abstract]
3.
Peegel, H.,
Randolph, J. J.,
Midgley, A. R.,
and Menon, K. M. J.
(1994)
Endocrinology
135,
1044-1051[Abstract]
4.
Lu, D. L.,
Peegel, H.,
Mosier, S. M.,
and Menon, K. M. J.
(1993)
Endocrinology
132,
235-240[Abstract]
5.
Kash, J. C.,
and Menon, K. M. J.
(1998)
J. Biol. Chem.
273,
10658-10664 6.
Kash, J. C.,
and Menon, K. M. J.
(1999)
Biochemistry
38,
16889-16897[CrossRef][Medline]
[Order article via Infotrieve]
7.
Ross, J.
(1993)
in
RNA-Protein Interaction Protocols
(Haynes, S. R., ed)
, pp. 459-476, Humana Press, Totowa, NJ
8.
Chomczynski, P.,
and Sacchi, N.
(1987)
Anal. Biochem.
162,
156-159[Medline]
[Order article via Infotrieve]
9.
Sambrook, J.,
Fritsch, E. F.,
and Maniatis, T.
(1989)
Molecular Cloning: A Laboratory Manual
, Cold Spring Harbor Laboratory, Cold Spring Harbor, NY
10.
Golos, T. G.,
Miller, W. L.,
and Strauss, J. F., III
(1987)
J. Clin. Invest.
80,
896-899[Medline]
[Order article via Infotrieve]
11.
Segaloff, D. L.,
Wang, H.,
and Richards, J. S.
(1990)
Mol. Endocrinol.
4,
1856-1865[CrossRef][Medline]
[Order article via Infotrieve]
12.
Camp, T. A.,
Rahal, J. O.,
and Mayo, K. E.
(1991)
Mol. Endocrinol.
5,
1405-1417[CrossRef][Medline]
[Order article via Infotrieve]
13.
Nakamura, K.,
Minegishi, T.,
Takakura, Y.,
Miyamoto, K.,
Hasegawa, Y.,
Ibuki, Y.,
and Igarashi, M.
(1990)
Biochem. Biophys. Res. Commun.
172,
786-792[CrossRef][Medline]
[Order article via Infotrieve]
14.
Peng, S. S.-Y.,
Chen, C.-Y. A., Xu, N.,
and Shyu, A.-B.
(1998)
EMBO J.
17,
3461-3470[CrossRef][Medline]
[Order article via Infotrieve]
15.
Klausner, R. D.,
Rouault, T. A.,
and Harford, J. B.
(1993)
Cell
72,
19-28[CrossRef][Medline]
[Order article via Infotrieve]
16.
Fan, X. C.,
and Steitz, J.
(1998)
EMBO J.
17,
3448-3460[CrossRef][Medline]
[Order article via Infotrieve]
17.
Burd, C. G.,
and Dreyfuss, G.
(1994)
Science
265,
615-621 18.
Decker, C. J.,
and Parker, R.
(1994)
Trends Biochem. Sci.
19,
336-340[CrossRef][Medline]
[Order article via Infotrieve]
19.
Bernstein, P. L.,
Herrick, D. J.,
Prokipcak, R. D.,
and Ross, J.
(1992)
Genes Dev.
6,
642-654 20.
Herrick, D.,
and Ross, J.
(1994)
Mol. Cell. Biol.
14,
2119-2228 21.
Shyu, A.-B.,
Belasco, J. G.,
and Greenberg, M. E.
(1991)
Genes Dev.
5,
221-231 22.
Shyu, A.-B.,
Greenberg, M. E.,
and Belasco, J. G.
(1989)
Genes Dev.
3,
60-72 23.
Veyrune, J. L.,
Carillo, S.,
Vie, A.,
and Blanchard, J. M.
(1995)
Oncogene
11,
2127-2134[Medline]
[Order article via Infotrieve]
24.
Zang, M.,
Pierce, R. A.,
Wachi, H.,
Mecham, R. P.,
and Parks, W. C.
(1999)
Mol. Cell. Biol.
19,
7314-7326 25.
Chen, C.-Y.,
You, Y.,
and Shyu, A.-B.
(1992)
Mol. Cell. Biol.
12,
5748-5757 26.
Prokipcak, R. D.,
Herrick, D. J.,
and Ross, J.
(1994)
J. Biol. Chem.
269,
9261-9269 27.
Ross, J.
(1995)
Microbiol. Rev.
59,
423 28.
Sachs, A.
(1993)
Cell
74,
413-421[CrossRef][Medline]
[Order article via Infotrieve]
Copyright © 2002 by The American Society for Biochemistry and Molecular Biology, Inc.
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati What's this?
This article has been cited by other articles:
|
|
 |
|
  L. Wang, A. K. Nair, and K. M. J. Menon Ribonucleic Acid Binding Protein-Mediated Regulation of Luteinizing Hormone Receptor Expression in Granulosa Cells: Relationship to Sterol Metabolism Mol. Endocrinol., September 1, 2007; 21(9): 2233 - 2241. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 C. Stocco, C. Telleria, and G. Gibori The Molecular Control of Corpus Luteum Formation, Function, and Regression Endocr. Rev., February 1, 2007; 28(1): 117 - 149. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 A. K. Nair, H. Peegel, and K. M. J. Menon The Role of Luteinizing Hormone/Human Chorionic Gonadotropin Receptor-Specific mRNA Binding Protein in Regulating Receptor Expression in Human Ovarian Granulosa Cells J. Clin. Endocrinol. Metab., June 1, 2006; 91(6): 2239 - 2243. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 A. K. Nair and K. M. J. Menon Regulation of Luteinizing Hormone Receptor Expression: EVIDENCE OF TRANSLATIONAL SUPPRESSION IN VITRO BY A HORMONALLY REGULATED mRNA-BINDING PROTEIN AND ITS ENDOGENOUS ASSOCIATION WITH LUTEINIZING HORMONE RECEPTOR mRNA IN THE OVARY J. Biol. Chem., December 30, 2005; 280(52): 42809 - 42816. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 N. H. Ing Steroid Hormones Regulate Gene Expression Posttranscriptionally by Altering the Stabilities of Messenger RNAs Biol Reprod, June 1, 2005; 72(6): 1290 - 1296. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 L. Wang and K. M. J. Menon Regulation of Luteinizing Hormone/Chorionic Gonadotropin Receptor Messenger Ribonucleic Acid Expression in the Rat Ovary: Relationship to Cholesterol Metabolism Endocrinology, January 1, 2005; 146(1): 423 - 431. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
A. K. Nair and K. M. J. Menon Isolation and Characterization of a Novel trans-Factor for Luteinizing Hormone Receptor mRNA from Ovary J. Biol. Chem., April 9, 2004; 279(15): 14937 - 14944. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
K.M.J. Menon, U. M. Munshi, C. L. Clouser, and A. K. Nair Regulation of Luteinizing Hormone/Human Chorionic Gonadotropin Receptor Expression: A Perspective Biol Reprod, April 1, 2004; 70(4): 861 - 866. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
N. K. Ryan, K. H. Van der Hoek, S. A. Robertson, and R. J. Norman Leptin and Leptin Receptor Expression in the Rat Ovary Endocrinology, November 1, 2003; 144(11): 5006 - 5013. [Abstract] [Full Text] [PDF]
|
|
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
| All ASBMB Journals | Molecular and Cellular Proteomics |
| Journal of Lipid Research | ASBMB Today |
