Temporal Patterns of Gonadotropin-Releasing Hormone (GnRH), c-fos, and Galanin Gene Expression in GnRH Neurons Relative to the Luteinizing Hormone Surge in the Rat

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The Journal of Neuroscience, January 15, 1998, 18(2):713-719

Temporal Patterns of Gonadotropin-Releasing Hormone (GnRH), c-fos, and Galanin Gene Expression in GnRH Neurons Relative to the Luteinizing Hormone Surge in the Rat
Patricia D. Finn¹, Robert A. Steiner¹^,²^,³, and Donald K. Clifton²^,³
Departments of ¹ Physiology and Biophysics and ² Obstetrics and Gynecology and ³ The Population Center for Research in Reproduction, University of Washington, Seattle, Washington 98195

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Gonadotropin-releasing hormone (GnRH) neurons increase their expression of Fos and galanin coincident with the luteinizinghormone (LH) surge in the female rat. To define the temporal relationshipsbetween the expression of these genes and the GnRH gene itselfand to gain insight about the possible functional interactionsof these processes, we compared levels of c-fos, galanin, andGnRH mRNA in GnRH neurons and plasma levels of LH in the rat,beginning 6 hr before and continuing for 24 hr after a sex steroid-inducedLH surge. LH levels were increased significantly by 1600 hr. Theyincreased twofold further by 1800 hr and then returned to baselineby 2400 hr. Using in situ hybridization, we determined that levelsof c-fos mRNA in GnRH neurons were elevated significantly at 1600hr only, whereas levels of galanin mRNA in GnRH neurons firstincreased twofold by 1800 hr, increased an additional twofoldby 2400 hr, and remained elevated at all time points sampled thereafter.There were no significant changes in cellular levels of GnRH mRNAover the time points sampled. These results are consistent withthe hypothesis that the induction of c-fos gene expression inGnRH neurons leads to an increase in galanin gene expression,and that the sustained increase in galanin mRNA levels in GnRHneurons reflects either the need to replenish galanin stores thatare depleted at the time of the LH surge or the involvement ofgalanin with physiological events that occur on the day of estrus.

Key words: gonadotropin-releasing hormone; luteinizing hormone-releasing hormone; c-fos; galanin; in situ hybridization; luteinizing hormone; reproduction; neuroendocrine regulation

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

On the afternoon of proestrus in the rat, the combined actions of estrogen (E) and progesterone (P) increase the release ofgonadotropin-releasing hormone (GnRH), which in turn induces apreovulatory surge of luteinizing hormone (LH) (see Freeman, 1994).Although the precise sequence of molecular events mediating thisphenomenon is poorly understood, several key intermediates havebeen identified, and these may provide insights into the overallprocess. The immediate early gene products Fos and Jun are inducedin some GnRH neurons during the LH surge (Lee et al., 1990a, 1992a).This induction appears to be inseparable from the occurrence ofthe LH surge and dependent on synaptic transmission (Lee et al.,1990a, 1993). This suggests that increased transcription of oneor more genes in GnRH neurons accompanies the release of GnRHand may be responsible for initiating events that are crucialfor either the enhancement of GnRH secretion during the surgeor replenishment of depleted stores of GnRH or other gene productsin these cells after the surge.

GnRH and galanin are coexpressed in GnRH neurons in the female rat (Coen et al., 1990; Merchenthaler et al., 1990; Marks etal., 1992), and their genes are plausible targets for activationby Fos and Jun (Bond et al., 1989; Anouar et al., 1994). Reportson whether a rise in GnRH gene expression subserves the occurrenceof the GnRH and LH surge have been equivocal and conflicting (seeSagrillo et al., 1996); however, galanin mRNA levels in GnRH neuronsclearly increase during the LH surge (Marks et al., 1993, 1994).As is the case with the expression of Fos in GnRH neurons, theincrease in galanin expression is inseparable from the occurrenceof the LH surge and is dependent on synaptic activation of GnRHneurons (Lee et al., 1990a, 1993; Marks et al., 1994; Rossmanithet al., 1996a). Although these observations point toward an activationof galanin gene expression in GnRH neurons at the time of theLH surge, other work from our laboratory suggests that galaningene expression in GnRH neurons is also activated (as measuredby elevated mRNA levels) on estrus 24 hr after the preovulatoryLH surge (Marks et al., 1993). Therefore, the precise role thatgalanin plays in these neurons remains unclear.

If Fos activates either galanin or GnRH gene expression in GnRH neurons, then c-fos mRNA levels should increase immediatelybefore a detectable rise in these mRNAs. Furthermore, if eitherGnRH or galanin is involved in the generation of the LH surge,one would predict that their messages would increase before thesurge and decline after its completion. To help clarify the physiologicalroles of c-fos, galanin, and GnRH in GnRH neurons and to determinethe temporal relationships among these parameters, we measuredcirculating LH levels and cellular levels of c-fos, galanin, andGnRH mRNAs in GnRH neurons in ovariectomized rats over a 30 hrperiod bracketing a steroid-induced LH surge.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animals
Adult, 60-d-old female Sprague Dawley rats were obtained from Simonsen Laboratories (Gilroy, CA). They were maintained underconstant temperature and a 14/10 hr light/dark cycle with lightson at 0700 hr. They were given free access to tap water and ratchow. Ovariectomies were performed under Ketamine (100 mg/ml)/Xylazine(20 mg/ml) anesthesia mixed at a ratio of 5.0:1.6. Rats were handledfour to five times weekly until killed. All procedures were approvedby the Animal Care Committee of the School of Medicine at theUniversity of Washington in accordance with the National Institutesof Health Guide for Care and Use of Laboratory Animals.

Experimental design
Experiment 1. Before assessing c-fos, GnRH, and galanin mRNA expression during the LH surge, a preliminary experiment wasconducted to determine the precise temporal pattern of LH releasein response to steroid priming. Eleven rats were ovariectomizedand allowed to recover for 3 weeks. On day 0 at 1030 hr the animalswere injected with estradiol benzoate (E₂B; 30 µg in 0.2 ml ofpeanut oil, s.c.). On day 1 cannulae were implanted into the rightatrium as described previously (Steiner et al., 1982). On day2 at 1200 hr, P (5 mg/0.1 ml, s.c.) was injected, and serial bloodsamples were drawn at 1400, 1600, 1700, 1800, 1900, 2000, 2200,and 2400 hr. An additional blood sample was collected at 0200hr on day 3. The serum was frozen for subsequent determinationof LH concentration by radioimmunoassay (RIA).
Experiment 2. To determine the temporal pattern of cellular levels of the mRNAs coding for GnRH, c-fos, and galanin in GnRHneurons during the course of the LH surge, nine sets of femalerats were ovariectomized, and 3-4 weeks later, they were treatedwith E₂B and P as described for Experiment 1. Sets of rats (n= 4-6) were killed on day 2 at 1200 hr (before P injection), 1400,1500, 1600, 1800, and 2400 hr and on day 3 at 0600, 1200, and1800 hr.

Tissue preparation
After asphyxiation with CO₂, the rats were decapitated immediately. Their brains were rapidly removed, frozen on dry ice,and stored at $-$ 80°C. Trunk blood was collected and serum was storedat $-$ 20°C until assayed for LH contents. Twenty-micrometer-thickcoronal brain sections were cut on a cryostat, thaw-mounted ontoSuperFrost glass slides (Fisher Scientific, Fair Lawn, NJ), andstored in airtight boxes at $-$ 80 C until used in the assay. Sectionswere collected beginning at the level of Plate 16, according tothe rat atlas of Paxinos and Watson (1986), and ending at thelevel of the caudal aspect of the decussation of the anteriorcommissure (~0.08 mm rostral to Plate 21). The tissue sectionswere collected onto four sets of slides, each one representinga one-in-four series of sections.

Riboprobe preparation
³⁵S-labeled GnRH cRNA probe The original plasmid containing a 462 bp insert complementary to prepro-GnRH (Adelman et al., 1986)was generously provided by Dr. Anthony Mason (Genentech, SouthSan Francisco, CA). The insert, which is complementary to 170bases of 5 $'$ untranslated message, the entire 276 bases of openreading frame, and the first 16 bases of 3 $'$ untranslated message,was subcloned into pGEM 4 (Marks et al., 1992). SalI was usedto linearize the cDNA. The ³⁵S-labeled cRNA antisense probe was synthesized in vitro usingan Ambion (Austin, TX) MAXIscript kit in the presence of 50 µM $alpha$ -thio-UTP (New England Nuclear, Boston, MA), of which 14% was³⁵S-labeled and 86% was unlabeled. Yeast tRNA was added as carrier,and the cRNA probe was separated from unincorporated nucleotideswith a Sephadex G-50 column (Boehringer Mannheim, Indianapolis,IN).
³⁵S-labeled galanin cRNA probe. The plasmid vector Bluescript (Stratagene, La Jolla, CA) containing a cDNA to rat galanin mRNAwas provided by Drs. Henry Friesen and Maria Vrontakis (Universityof Manitoba, Winnipeg, Manitoba, Canada) (Vrontakis et al., 1987).The 680 bp insert is complementary to 124 bases of 5 $'$ untranslatedmessage, the entire 372 bases of open reading frame, and 184 basesof 3 $'$ untranslated message. HindIII was used to linearize thecDNA. The ³⁵S-labeled cRNA antisense probe was synthesized in vitro in a reactioncontaining the following ingredients: 50 µM $alpha$ -thio-UTP, of which25% was ³⁵S-labeled and the remaining 75% was unlabeled; linearized cDNA(1 µg/µl); T7 RNA polymerase (2 U/µl, Boehringer Mannheim); 1×transcription buffer (provided with polymerase); 500 µM ATP, CTP,and GTP; RNase inhibitor (4 U/µl); and 10 mM dithiolthreitol (DTT).Residual DNA was digested with 0.5 U/µl DNase, and the DNase reactionwas stopped by adding 80 mM EDTA. Yeast tRNA was added as carrier,and the cRNA was purified with a Sephadex G-50 column.
³³P-labeled c-fos cRNA probe. The original plasmid (pSP65) containing the rat c-fos insert was generously provided by Dr. TomCurran (Roche Institute of Molecular Biology, Nutley, NJ) (Curranet al., 1987). A 1352 bp EcoRI and XhoI fragment of the cDNA wassubcloned into pBluescript S/K (Burton et al., 1995). The cDNAwas linearized with EcoRI, and the ³³P-labeled antisense cRNA probe was synthesized in vitro usingan Ambion MAXIscript kit in the presence of 12.5 pmol of [³³P]UTP (DuPont NEN, Wilmington, DE). Yeast tRNA was added as carrier,and the cRNA probe was purified with an NENsorb column (DuPontNEN).
Digoxigenin-labeled GnRH cRNA probe. The digoxigenin-labeled cRNA probes for GnRH mRNA were synthesized in vitro in reactionscontaining the following ingredients: linearized DNA (1 µg/µl);1× digoxigenin DNA labeling mixture (Boehringer Mannheim); SP6RNA polymerase (2 U/µl; Boehringer Mannheim); 1× transcriptionbuffer (provided with polymerase); RNase inhibitor (2 U/µl); and10 mM DTT. Residual DNA was digested with 0.5 U/µl DNase. TheDNase reaction was stopped by adding 80 mM EDTA. The cRNA probewas separated from unincorporated nucleotides with a SephadexG-50 column. The final concentrations of the digoxigenin-labeledGnRH probes were determined to be optimal based on preliminarytest assays.

Single-label in situ hybridization
³⁵S-labeled GnRH. To identify cells containing GnRH mRNA, we performed single-label in situ hybridization based on previouslypublished protocols (Wiemann et al., 1990; Marks et al., 1992)with slight modifications. In brief, tissue sections were fixed,acetylated, and delipidated. Next, hybridization solution [freshlydenatured ³⁵S-labeled GnRH probe (0.30 µg · ml¹ · kb¹) and yeast tRNA (2 mg/ml) in hybridization buffer consistingof 52% deionized formamide, 10% dextran sulfate, 0.3 M NaCl, 8mM Tris, pH 8.0, 0.08 mM EDTA, 0.02% bovine serum albumin, 0.02%Ficoll, 0.02% polyvinylpyrrolidone, and 200 mM DTT] was appliedto the tissue (30 µl/slide). The slides were covered with silane-coatedglass coverslips and incubated in humid chambers overnight at51°C. The next day the tissue was treated with RNase-A and washedunder conditions of increasing stringency, including a 30 minwash at 60°C in 0.1× SSC. The tissue was then dehydrated in alcoholsand air-dried. The slides were dipped in Kodak (Rochester, NY)NTB-2 emulsion diluted 1:1 in 600 mM ammonium acetate, exposedfor 8 d, developed, and counterstained with cresyl violet.

Double-label in situ hybridization
³⁵S-labeled galanin and digoxigenin-labeled GnRH. To identify cells containing both GnRH mRNA and galanin mRNA, we performeddouble-label in situ hybridization following a protocol describedpreviously (Marks et al., 1992; Finn et al., 1996) with slightmodifications. The tissue sections were fixed, acetylated, anddelipidated. Next, hybridization solution [freshly denatured ³⁵S-labeled galanin probe (0.25 µg · ml¹ · kb¹), digoxigenin-labeled GnRH probe (diluted 1:1200), and yeasttRNA (1.8 mg/ml) in hybridization buffer] was applied to the tissue(70 µl/slide). The slides were covered with Parafilm, sealed withrubber cement, and incubated in humid chambers overnight at 68°C.The next day the tissue was treated with RNase-A and washed underconditions of increasing stringency, including a 30 min wash at65°C in 0.1× SSC. Next the sections were incubated for 60 minin blocking buffer, rinsed, and then incubated for 3 hr at 37°Cwith anti-digoxigenin fragments conjugated to alkaline phosphatase(Boehringer Mannheim) diluted 1:1000. After rinsing, the sectionswere incubated in chromagen solution containing nitroblue tetrazolium-chloride(Boehringer Mannheim), 5-bromo-4-chloro-3-indolyl phosphate (BoehringerMannheim), and levamisole. To stop the reaction, the sectionswere rinsed in 10 mM Tris containing 1 mM EDTA. Next, the slideswere dipped in 70% ethanol, air-dried, dipped in 3% parlodionfollowed by Kodak NTB-2 emulsion that was diluted 1:1 in 600 mMammonium acetate, exposed for 7 d, and developed.
³³P-labeled c-fos and digoxigenin-labeled GnRH. We performed a double-label in situ hybridization to identify cells containingboth GnRH mRNA and c-fos mRNA by the use of a protocol similarto that described in the preceding section with the followingmodifications. First, 35 µl/slide hybridization buffer (withoutDTT) containing freshly denatured ³³P-labeled c-fos probe (538,000 dpm/1 µl of hybridization solution),digoxigenin-labeled GnRH probe (diluted 1:4000), and yeast tRNA(1.8 mg/ml) was applied to the tissue. Second, the slides werecovered with silane-coated coverslips and incubated overnightin humid containers at 60°C. Third, the final stringent wash wasperformed in 0.1× SSC at 60°C. Fourth, the slides were dippedin Kodak NTB-3 and exposed for 52 d.

Control experiments
The identity and integrity of all radioactively labeled cRNA probes were verified by PAGE against known standards. The controlexperiments used to validate the binding kinetics and specificityof the GnRH and galanin cRNA probes have been described previously(Marks et al., 1992), as have specificity experiments for thec-fos cRNA probe (Burton et al., 1995).

Semiquantitative analysis of cellular galanin mRNA levels in GnRH neurons
Slides were assigned a random three-letter code and read in alphabetical order with an automated image-processing system byan operator unaware of the experimental group of the animal. Thenumber of silver grains per cell was determined with a grain-countingprogram, as described previously (Marks et al., 1992).
In the double-label in situ hybridization assays, GnRH neurons were identified under bright-field illumination by the appearanceof a purple precipitate in the cytoplasm, indicating the presenceof the digoxigenin-labeled cRNA probe for GnRH mRNA. The silvergrains overlying these GnRH neurons were counted under dark-fieldillumination by the computerized image processor, and their anatomicallocalization was noted. To minimize differences among experimentalgroups and to make conservative estimates of the changes in galaninmRNA levels (or c-fos mRNA levels), all identifiable GnRH neuronswere analyzed for silver grain counts and included in the totals.This avoided making subjective decisions about whether a particularGnRH cell was double-labeled for galanin mRNA or c-fos mRNA. Thus,if not all GnRH neurons express galanin or c-fos mRNA, the graincounts would underestimate actual mRNA signal levels in the subsetof GnRH neurons that do express the mRNAs. For galanin mRNA expressionin GnRH neurons, 15 sections per animal, equally spaced from thediagonal band of Broca (DBB) through the caudal part of the preopticarea (POA), were analyzed for the number of grains per cell. Forc-fos mRNA expression in GnRH neurons, nine sections per animal,equally spaced from the caudal DBB to the mid-POA, were analyzedfor the number of grains per cell; this area contains the majorityof GnRH neurons that express Fos at the time of an LH surge (Hoffmanet al., 1990; Lee et al., 1990a).
In the single-label in situ hybridization assay for GnRH mRNA, 15 sections per animal, equally spaced from the DBB throughthe caudal part of the POA, were analyzed for the number of grainsper cell. GnRH mRNA-expressing neurons were identified by thepresence of a discrete grain cluster localized to areas in whichGnRH neurons are found. The silver grains associated with clustersthat had a signal-to-noise ratio >10 were counted under dark-fieldillumination by the computerized image processor, and their anatomicallocalization was noted. Two separate analyses were performed,based on the assignment of GnRH mRNA-expressing neurons to differentanatomically described areas (Paxinos and Watson, 1986). In thefirst analysis, GnRH mRNA-expressing neurons were assigned tostandard anatomically described areas, which included the DBB,POA, and medial septum. In the second analysis, GnRH mRNA-expressingneurons were assigned to areas based on their location withincertain rostral-to-caudal divisions, which included the DBB (Plates16 and 17), the rostral POA at the level of the vascular organof the lamina terminalis (rPOA/OVLT; caudal to Plate 17 throughtPlate 19), or the remaining POA (immediately caudal to Plate 19to ~0.08 mm rostral to Plate 21). This second analysis was undertakento compare our results with those of two other laboratories thatused a similar approach to study the regulation of GnRH gene expressionat the time of an LH surge (Porkka-Heiskanen et al., 1994; Petersenet al., 1995).

LH assay
Serum levels of LH were measured under the auspices of the RIA core of the Population Center for Research in Reproductionat the University of Washington (Dr. William Bremner, Director)with reagents provided by National Institutes of Health. The standardwas rLH-RP3, and the antiserum was anti-rLH-S11 (National Instituteof Diabetes and Digestive and Kidney Diseases, Bethesda, MD).The tracer was purchased from Corning Hazelton, Inc. (Vienna,VA). All samples were measured in a single assay. Based on theduplicate values of the samples run in the assay, the intraassaycoefficient of variation was 4.5%.

Statistical analysis
For the experiment, n refers to the number of experimental animals within a group, and this n was used for the analysis. Forgalanin, c-fos, and GnRH mRNA content determinations, the meangrains per cell from individual animals were used to calculatethe mean ± SEM for each group. Differences among groups in LHlevels, numbers of cells counted, and grains per cell were assessedby ANOVA. When the ANOVA indicated a significant difference, Duncan'snew multiple range test was used to detect differences betweengroups. The rejection level for statistical tests was set at $alpha$ = 0.05.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Experiment 1

Serum LH levels in experiment 1 are shown in Figure 1. LH values began to rise by 1600 hr, peaked between 1800 and 1900 hr,and returned to baseline between 2200 and 2400 hr.

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Figure 1. Time course of serum LH concentrations in estrogen- and progesterone-primed ovariectomized rats in experiment 1. Values representthe mean ± SEM serum LH concentrations of serial blood samplesobtained via jugular cannulae from 11 animals.

Experiment 2

LH Levels
Again, serum LH levels showed the pattern characteristic of a typical LH surge. As seen in Figure 2A, LH levels on day 2 weresignificantly higher in animals killed at 1600 hr (n = 6) thanin animals killed earlier on that day (p < 0.05 for 1600 hr vsall earlier time points that day; 1200 hr, n = 4; 1400 hr, n =6; 1500 hr, n = 6). Mean LH levels were highest at 1800 hr (p< 0.01 vs 1600 hr; n = 5) and returned to baseline by 2400 hr(p < 0.01 vs 1600 hr and 1800 hr; n = 5). LH levels remained lowat all time points sampled on day 3 (0600 hr, n = 6; 1200 hr,n = 5; 1800 hr, n = 6).

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Figure 2. Time course of serum LH concentrations (A), relative levels of c-fos mRNA (B), relative levels of galanin mRNA (C), and relativelevels of GnRH mRNA (D) in estrogen- and progesterone-primed ovariectomizedrats during a 30 hr period bracketing the time of the expectedLH surge (experiment 2). Values represent the mean ± SEM of fourto six animals per group. Values with different letters are significantlydifferent from one another (p < 0.05). Values with the same letterare not significantly different from one another (p > 0.05). Thedashed line indicates the time of the peak of the LH surge.

c-fos mRNA
The c-fos mRNA content of GnRH neurons varied significantly over the nine time points that were sampled (p < 0.001; Fig. 2B).c-fos signal levels were twofold to sixfold higher on day 2 at1600 hr than at any other time point sampled (p < 0.01 vs allother time points). This increase in c-fos gene expression wascoincident with the first significant increase in LH levels. Althoughc-fos mRNA levels appeared to be elevated on day 2 at both 1500and 1800 hr relative to the levels at 1200 and 1400 hr on thesame day, the apparent differences among these times were notstatistically significant. The photomicrographs in Figure 3, Aand B, illustrate higher levels of c-fos mRNA expression in GnRHneurons at the beginning of the LH surge (day 2, 1600 hr) thansubsequent (day 2, 2400 hr) to the LH surge (Fig. 3E,F). Therewere no significant differences among groups in the number ofGnRH neurons counted.

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Figure 3. A, Bright-field photomicrograph of two GnRH neurons (black arrows) labeled with a digoxigenin-labeled cRNA probe for GnRHmRNA in an ovariectomized estrogen- and progesterone-primed femalerat killed at 1600 hr on the day of the expected LH surge. B,Dark-field photomicrograph of the same view as in A showing thelocation of the same two GnRH neurons labeled with a ³³P-labeled probe for c-fos mRNA (white arrows). Note the abundanceof silver grains (clusters of white dots) over each cell indicatingthe high level of c-fos mRNA expression in these neurons. C, Bright-fieldphotomicrograph of three GnRH neurons (black arrows) labeled witha digoxigenin-labeled cRNA probe for GnRH mRNA in the same animalshown in A and B. D, Dark-field photomicrograph of the same viewas C, showing the location of the same three GnRH neurons labeledwith a ³⁵S-labeled probe for galanin mRNA (white arrows). Note the relativeabsence of silver grains indicating the low level of galanin mRNAexpression in these neurons. E, Bright-field photomicrograph oftwo GnRH neurons (black arrows) labeled with a digoxigenin-labeledcRNA probe for GnRH mRNA in an ovariectomized estrogen- and progesterone-primedfemale rat killed at 2400 hr on the day of the expected LH surge.F, Dark-field photomicrograph of the same view as in E showingthe location of the same two GnRH neurons labeled with a ³³P-labeled probe for c-fos mRNA (white arrows). Note the relativeabsence of silver grains indicating the low level of c-fos mRNAexpression in these neurons. G, Bright-field photomicrograph oftwo GnRH neurons (black arrows) labeled with a digoxigenin-labeledcRNA probe for GnRH mRNA in the same animal shown in E and F.H, Dark-field photomicrograph of the same view as G, showing thelocation of the same two GnRH neurons labeled with a ³⁵S-labeled probe for galanin mRNA (white arrows). Note the abundanceof silver grains (clusters of white dots) over each cell indicatingthe high level of galanin mRNA expression in these neurons. Magnification,1200×.

Galanin mRNA
Galanin mRNA levels in GnRH neurons also differed significantly over the sampling period (p < 0.001). As illustrated in Figure2C, animals killed at 1800 hr on day 2 had twofold higher galaninmRNA signal levels in GnRH neurons than those killed earlier onday 2 (p < 0.05 for 1800 hr vs all earlier time points that day).This initial increase in galanin mRNA in GnRH neurons coincidedwith maximal serum LH levels and occurred after c-fos mRNA inGnRH neurons had peaked. Levels of galanin mRNA in GnRH neuronsincreased another twofold by 2400 hr on day 2 (p < 0.01 vs 1800hr) and remained elevated at all time points sampled on day 3(p < 0.01 for 1800 hr on day 2 vs all time points on day 3), wellafter the completion of the LH surge. The photomicrographs inFigure 3, G and H, illustrate higher galanin mRNA in GnRH neuronsafter the peak of the LH surge (day 2, 2400 hr) than during theLH surge (day 2, 1600 hr) (Fig. 3C,D). There were no significantdifferences among the groups in the number of GnRH neurons counted.

GnRH mRNA levels
GnRH mRNA levels did not differ significantly among groups, whether analyzed by brain area or by the time of killing relativeto the LH surge (p > 0.05; Fig. 2D). There were no differencesamong groups in the number of GnRH mRNA-expressing cells countedacross the nine time points sampled bracketing the LH surge. Becauseother laboratories have reported finding differences in GnRH mRNAexpression when their analysis was restricted to specific areas(Porkka-Heiskanen et al., 1994; Petersen et al., 1995), we performedan analysis similar to these others and again could detect nosignificant differences among groups in either the number of GnRHmRNA-containing neurons counted (p > 0.05) or the level of GnRHmRNA measured per cell for the DBB, the rPOA/OVLT, or the remainingPOA (p > 0.05).

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

We report here that levels of c-fos mRNA in GnRH neurons are elevated significantly coincident with the first increase inLH levels at the time of an E- and P-induced LH surge in femalerats. Similarly, Fos protein increases in GnRH neurons near thetime of the LH surge in rats (Lee et al., 1990a; Hrabovszky etal., 1995; Wang et al., 1995), mice (Wu et al., 1992), hamsters(Berriman et al., 1992; Doan and Urbanski, 1994), and sheep (Moenteret al., 1993). In rats, Fos protein is first detectable in GnRHneurons after the onset of the expected LH surge, and the numberof GnRH neurons expressing Fos increases during the ascendingphase of the LH surge (Lee et al., 1990a, 1992b). These resultsagree with those of the present study showing that c-fos geneexpression increases in GnRH neurons near the onset of the LHsurge. Synaptic blockade with phenobarbital or MK-801 (an NMDAchannel blocker) inhibits the LH surge and the induction of Fosin GnRH neurons (Lee et al., 1990a, 1993), suggesting that thisinduction is dependent on trans-synaptic activation of GnRH neurons.GnRH neurons also express Jun concomitantly with the LH surge(Lee et al., 1992a). Together, Fos and Jun form a heterodimer,activator protein 1 (AP-1), that regulates a variety of genes(Morgan and Curran, 1991). Among the possible targets for AP-1regulation in GnRH neurons is the gene for galanin, which haselements in the 5 $'$ -flanking region that can bind members of theFos/Jun family of transcription factors (Anouar et al., 1994),and the gene for GnRH itself, which has an AP-1 site in its upstreamregulatory region (Bond et al., 1989).

GnRH levels in the portal circulation increase before the onset of the LH surge (see Freeman, 1994); however, it is unclearwhether this increase is associated with alterations in GnRH geneexpression (see Sagrillo et al., 1996). In the present study,we detected no significant differences in GnRH gene expressionacross a 30 hr period bracketing an E- and P-induced LH surge(6 hr before and 24 hr after), either by the number of detectableGnRH mRNA-expressing neurons or by signal levels of GnRH mRNAper cell. Similarly, two other laboratories found no differencesin cytoplasmic GnRH mRNA levels at the time of a E- and P-inducedLH surge, as measured by RNase protection assay (Gore and Roberts,1995) or by in situ hybridization (Park et al., 1990). However,a third laboratory found that GnRH mRNA levels in the rPOA/OVLTand POA increased ~8 hr before a steroid-induced LH surge (Petersenet al., 1995), earlier than we began sampling and which wouldhave gone unrecognized in our study. The results of studies examininglevels of GnRH mRNA relative to a preovulatory LH surge are morecontradictory. Although our laboratory (Marks et al., 1993) andMalik and colleagues (1991) found no differences in GnRH mRNAover the estrous cycle, others have found that GnRH mRNA levelsincrease before or at the time of a preovulatory LH surge in atleast a subset of GnRH neurons (Zoeller and Young, 1988; Parket al., 1990; Porkka-Heiskanen et al., 1994; Gore and Roberts,1995; Suzuki et al., 1995). However, these reports disagree withone another on detailed aspects of this putative phenomenon (seeSagrillo et al., 1996). If it is true that GnRH mRNA levels increaseon the day of the LH surge, the consensus of the studies thattestify to finding such an increase would have it occur severalhours before the induction of c-fos mRNA (reported here) and Fosprotein in GnRH neurons (Lee et al., 1992b; Porkka-Heiskanen etal., 1994; Gore and Roberts, 1995; Petersen et al., 1995). Thus,it would be unlikely that Fos is involved in the induction ofGnRH gene expression.

On the basis of several observations, Fos may be involved in the induction of galanin gene expression in GnRH neurons. First,like Fos, galanin mRNA levels in GnRH neurons increase coincidentwith a preovulatory or steroid-induced LH surge (Hoffman et al.,1990; Lee et al., 1990a; Marks et al., 1993, 1994), and galaninmRNA is expressed in the majority of GnRH neurons that colocalizeFos at the time of a steroid-induced LH surge (Hrabovszky et al.,1995). Second, blockade of the steroid-induced LH surge with eitherphenobarbital or MK-801 is associated with an inhibition of Fosprotein and galanin gene expression in GnRH neurons (Lee et al.,1990a, 1993; Marks et al., 1994; Rossmanith et al., 1996a). Third,in E-primed rats, P increases both the number of GnRH neuronsthat express Fos and the level of galanin gene expression in GnRHneurons (Lee et al., 1990b; Rossmanith et al., 1996b). Finally,we demonstrate here that the first detectable rise in galaninmRNA levels in GnRH neurons occurs 2 hr after c-fos mRNA risesin GnRH neurons, providing sufficient time for translation ofc-fos mRNA into Fos protein and the initiation of galanin geneexpression by an AP-1-dependent mechanism. Therefore, we postulatethat the induction of c-fos mRNA in GnRH neurons at the time ofthe LH surge is involved directly in the activation of galaningene expression in GnRH neurons.

Here we show that galanin mRNA levels in GnRH neurons increase only after the onset of the LH surge and remain elevated forat least 24 hr, confirming our previous observation that galaninmRNA levels in GnRH neurons increase between the morning and afternoonof proestrus and are elevated 24 hr later on estrus (Marks etal., 1993). This increase could reflect an increase in galaningene transcription or a decrease in mRNA degradation, but regardlessof the mechanism, there is more galanin mRNA in GnRH neurons forpossible translation into protein. However, the time course ofgalanin protein levels in GnRH neurons relative to an LH surgeis unclear. Merchenthaler and colleagues (1991), using immunocytochemistry,found no difference in the number of GnRH neurons that colocalizegalanin over the estrous cycle. However, the interpretation ofthis "negative" result is complicated by two factors. First, colchicine,which by itself can induce galanin mRNA (Cortes et al., 1990),was used to visualize galanin in GnRH neurons. Second, double-labelimmunocytochemistry may not be sufficiently sensitive to detectsmall changes in protein levels. Therefore, although galanin mRNAin GnRH neurons is increased dramatically in association withan LH surge, the consequences of this transcriptional regulationon galanin peptide production await further clarification.

We have proposed that the galanin deriving from GnRH neurons is needed for the production of an LH surge. This is supportedby the observations that galanin stimulates GnRH from median eminencefragments (López and Negro-Vilar, 1990; Merchenthaler et al.,1990; Sahu et al., 1994), central infusions of galanin stimulateLH secretion in E-primed rats (Sahu et al., 1987, 1994), galaninantagonists and antiserum blunt the LH surge (López et al., 1993;Sahu et al., 1994), and galanin mRNA expression in GnRH neuronsis inhibited by pharmacological agents that block the LH surge(Marks et al., 1994; Rossmanith et al., 1996a). Therefore, weexpected galanin mRNA levels in GnRH neurons to rise before theLH surge. It is possible that galanin gene expression in GnRHneurons increases in response to the depletion of galanin storesthat occurs during the early stages of the GnRH and LH surge.If this is the case, then it is puzzling that levels of galaninmRNA remain elevated for so long after the onset of the LH surge(>24 hr). Under laboratory conditions, female rats undergo a preovulatorysurge of LH every 4-5 d (see Freeman, 1994), whereas in the wild,they are more likely to show preovulatory surges at much longerintervals, with the majority of the intervening time spent inpregnancy or lactation. Thus, it is reasonable to postulate thatthe increase of galanin mRNA at the time of the LH surge reflectsa need for the production of galanin to be involved in processesthat occur subsequent to the LH surge rather than in replenishinggalanin stores that would be used to generate the next LH surge;this remains to be explored.

The present results suggest that the expression of Fos protein in GnRH neurons is a reflection of events culminating in thehypersecretion of GnRH, and that Fos is involved in the activationof galanin, but not GnRH, gene expression in GnRH neurons. Wepostulate that the increase in galanin mRNA levels in GnRH neuronsat the time of the LH surge reflects either the need to replenishgalanin stores depleted during the preceding LH surge or the prolongedproduction of galanin required to serve physiological events occurringon the day of estrus or thereafter.

  FOOTNOTES

Received Sept. 22, 1997; revised Nov. 4, 1997; accepted Nov. 5, 1997.

This work was supported by United States Public Health Service National Institutes of Health Grants RO1 HD27142 and T32 HD07453and by the Mellon Foundation. We express our appreciation to EmiliaKabigting, Yvonne Chan, and Darouny Phosarath for their excellenttechnical skill and assistance in performing these experimentsand Dr. William Bremner and the laboratory staff of the PopulationCenter for Research in Reproduction Assay Core for performingthe LH assays. We also thank MeiLan King, who contributed to theearly phases of this work as part of her honors thesis for graduationfrom the University of Washington with honors.
Correspondence should be addressed to Dr. Donald K. Clifton, Department of Obstetrics and Gynecology, Box 356460, Universityof Washington, Seattle, WA 98195.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Adelman JP, Mason AJ, Hayflick JS, Seeburg PH (1986) Isolationof the gene and hypothalamic cDNA for the common precursor ofgonadotropin-releasing hormone and prolactin release-inhibitingfactor in human and rat. ProcNatl Acad Sci USA 83:179-183[Abstract/Free Full Text].
Anouar Y, MacArthur L, Cohen J, Iacangelo AL, Eiden LE (1994) Identificationof a TPA-responsive element mediating preferential transactivationof the galanin gene promoter in chromaffin cells. JBiol Chem 269:6823-6831[Abstract/Free Full Text].
Berriman SJ, Wade GN, Blaustein JD (1992) Expressionof Fos-like proteins in gonadotropin-releasing hormone neuronsof Syrian hamsters: effects of estrous cycles and metabolic fuels. Endocrinology 131:2222-2228[Abstract/Free Full Text].
Bond CT, Hayflick JS, Seeburg PH, Adelman JP (1989) Therat gonadotropin-releasing hormone: SH locus: structure and hypothalamicexpression. Mol Endocrinol 3:1257-1262[Abstract/Free Full Text].
Burton KA, Kabigting EB, Steiner RA, Clifton DK (1995) Identificationof target cells for growth hormone's action in the arcuate nucleus. AmJ Physiol 269:E716-E722[Abstract/Free Full Text].
Coen C, Montagnese C, Opacka-Juffry J (1990) Coexistenceof gonadotropin-releasing hormone and galanin: immunohistochemicaland functional studies. JNeuroendocrinol 2:107-111.
Cortes R, Ceccatelli S, Schalling M, Hokfelt T (1990) Differentialeffects of intracerebroventricular colchicine administration onthe expression of mRNAs for neuropeptides and neurotransmitterenzymes, with special emphasis on galanin: an in situ hybridizationstudy. Synapse 6:369-391[Web of Science][Medline].
Curran T, Gordon MB, Rubino KL, Sambucetti LC (1987) Isolationand characterization of the c-fos (rat) cDNA and analysis of post-translationalmodification in vitro. Oncogene 2:79-84[Web of Science][Medline].
Doan A, Urbanski HF (1994) Diurnalexpression of Fos in luteinizing hormone-releasing hormone neuronsof Syrian hamsters. Biol Reprod 50:301-308[Abstract].
Finn PD, McFall TB, Clifton DK, Steiner RA (1996) Sexualdifferentiation of galanin gene expression in gonadotropin-releasinghormone neurons. Endocrinology 137:4767-4772[Abstract].
Freeman ME (1994) The neuroendocrine control of theovarian cycle of the rat. In: Thephysiology of reproduction (Knobil E, Neill JD, eds), pp 613-658. NewYork: Raven.
Gore AC, Roberts JL (1995) Regulationof gonadotropin-releasing hormone gene expression in the rat duringthe luteinizing hormone surge. Endocrinology 136:889-896[Abstract].
Hoffman GE, Lee W-S, Attardi B, Yann V, Fitzsimmons MD (1990) Luteinizinghormone-releasing hormone neurons express c-fos antigen aftersteroid activation. Endocrinology 126:1736-1741[Abstract/Free Full Text].
Hrabovszky E, Vrontakis ME, Peterson SL (1995) Triple-labelingmethod combining immunocytochemistry and in situ hybridizationhistochemistry: demonstration of overlap between Fos-immunoreactiveand galanin mRNA-expressing subpopulations of luteinizing hormone-releasinghormone neurons in female rats. JHistochem Cytochem 43:363-370[Abstract].
Lee W-S, Smith MS, Hoffman GE (1990a) Luteinizinghormone-releasing hormone neurons express Fos protein during theproestrous surge of luteinizing hormone. ProcNatl Acad Sci USA 87:5163-5167[Abstract/Free Full Text].
Lee W-S, Smith MS, Hoffman GE (1990b) Progesteroneenhances the surge of luteinizing hormone by increasing the activationof luteinizing hormone-releasing hormone neurons. Endocrinology 127:2604-2606[Abstract/Free Full Text].
Lee W-S, Abbun R, Smith MS, Hoffman GE (1992a) LHRHneurons express cJun protein during the proestrous surge of luteinizinghormone. Endocrinology 130:3101-3103[Abstract/Free Full Text].
Lee W-S, Smith MS, Hoffman GE (1992b) cFosactivity identifies recruitment of luteinizing hormone releasinghormone neurons during the ascending phase of the proestrous luteinizinghormone surge. J Neuroendocrinol 4:161-166[Web of Science].
Lee W-S, Abbud R, Hoffman GE, Smith MS (1993) Effectsof N-methyl-D-aspartate receptor activation on cFos expressionin luteinizing hormone-releasing hormone neurons in female rats. Endocrinology 133:2248-2254[Abstract/Free Full Text].
López FJ, Negro-Vilar A (1990) Galaninstimulates luteinizing hormone-releasing hormone secretion fromarcuate nucleus-median eminence fragments in vitro: involvementof an $alpha$ -adrenergic mechanism. Endocrinology 127:2431-2436[Abstract/Free Full Text].
López FJ, Meade EH, Negro-Vilar A (1993) Endogenousgalanin modulates the gonadotropin and prolactin proestrous surgesin the rat. Endocrinology 132:795-800[Abstract/Free Full Text].
Malik KF, Silverman A-J, Morrell JI (1991) Gonadotropinreleasing hormone mRNA in the rat: distribution and neuronal contentover the estrous cycle and after castration in males. AnatRec 231:457-466[Medline].
Marks DL, Weimann JN, Burton KA, Lent KL, Clifton DK, Steiner RA (1992) Simultaneousvisualization of two cellular mRNA species in individual neuronsby use of a new double in situ hybridization method. MolCell Neurosci 3:395-405[Web of Science].
Marks DL, Smith MS, Vrontakis M, Clifton DK, Steiner RA (1993) Regulationof galanin gene expression in gonadotropin-releasing hormone neuronsduring the estrous cycle of the rat. Endocrinology 132:1836-1844[Abstract/Free Full Text].
Marks DL, Lent KL, Rossmanith WG, Clifton DK, Steiner RA (1994) Activation-dependentregulation of galanin gene expression in gonadotropin-releasinghormone neurons in the female rat. Endocrinology 134:1991-1998[Abstract].
Merchenthaler I, Lopez FJ, Negro-Vilar A (1990) Colocalizationof galanin and luteinizing hormone-releasing hormone in a subsetof preoptic hypothalamic neurons: anatomical and functional correlates. ProcNatl Acad Sci USA 87:6326-6330[Abstract/Free Full Text].
Merchenthaler I, López FJ, Lennard DE, Negro-Vilar A (1991) Sexualdifferences in the distribution of neurons coexpressing galaninand luteinizing hormone-releasing hormone in the rat brain. Endocrinology 129:1977-1986[Abstract/Free Full Text].
Moenter SM, Karsch FJ, Lehman MN (1993) Fosexpression during the estradiol-induced gonadotropin-releasinghormone (GnRH) surge of the ewe: induction in GnRH and other neurons. Endocrinology 133:896-903[Abstract/Free Full Text].
Morgan JI, Curran T (1991) Stimulus-transcriptioncoupling in the nervous system: involvement of the inducible proto-oncogenesfos and jun. Annu Rev Neurosci 14:421-451[Web of Science][Medline].
Park O-K, Gugneja S, Mayo KE (1990) Gonadotropin-releasinghormone gene expression during the rat estrous cycle: effectsof pentobarbitol and ovarian steroids. Endocrinology 127:365-372[Abstract/Free Full Text].
Paxinos G, Watson C (1986) In: Therat brain in stereotaxic coordinates. NewYork: Academic.
Petersen SL, McCrone S, Keller M, Shores S (1995) Effectsof estrogen and progesterone on luteinizing hormone-releasinghormone messenger ribonucleic acid levels: consideration of temporaland neuroanatomical variables. Endocrinology 136:3604-3610[Abstract].
Porkka-Heiskanen T, Urban JH, Turek FW, Levine JE (1994) Geneexpression in a subpopulation of luteinizing hormone-releasinghormone (LHRH) neurons prior to the preovulatory gonadotropinsurge. J Neurosci 14:5548-5558[Abstract].
Rossmanith WG, Marks DL, Steiner RA, Clifton DK (1996a) Inhibitionof steroid-induced galanin mRNA expression in GnRH neurons bya specific NMDA-receptor blockade. JNeuroendocrinol 8:179-184[Web of Science][Medline].
Rossmanith WG, Marks DL, Clifton DK, Steiner RA (1996b) Inductionof galanin mRNA in GnRH neurons by estradiol and its facilitationby progesterone. J Neuroendocrinol 8:185-191[Web of Science][Medline].
Sagrillo CA, Grattan DR, McCarthy MM, Selmanoff M (1996) Hormonaland neurotransmitter regulation of GnRH gene expression and relatedreproductive behaviors. BehavGenet 26:241-277[Web of Science][Medline].
Sahu A, Crowley WR, Tatemoto K, Balasubramaniam A, Kalra SP (1987) Effectsof neuropeptide Y, NPY analog (norleucine4-NPY), galanin and neuropeptideK on LH release in ovariectomized (ovx) and ovx estrogen, progesterone-treatedrats. Peptides 8:921-926[Web of Science][Medline].
Sahu A, Xu B, Kalra SP (1994) Roleof galanin in stimulation of pituitary luteinizing hormone secretionas revealed by a specific receptor antagonist, galantide. Endocrinology 134:529-536[Abstract/Free Full Text].
Steiner RA, Bremner WJ, Clifton DK (1982) Regulationof luteinizing hormone pulse frequency and amplitude by testosteronein the adult male rat. Endocrinology 111:2055-2061[Abstract/Free Full Text].
Suzuki M, Nishihara M, Takahashi M (1995) Hypothalamicgonadotropin-releasing hormone gene expression during the ratestrous cycle. Endocr J 42:789-796[Web of Science][Medline].
Vrontakis ME, Peden LM, Duckworth ML, Friesen HG (1987) Isolationand characterization of a complimentary DNA (galanin) clone fromestrogen-induced pituitary tumor messenger RNA. JBiol Chem 262:16755-16758[Abstract/Free Full Text].
Wang H-J, Hoffman GE, Smith MS (1995) IncreasedGnRH mRNA in the GnRH neurons expressing cFos during the proestrousLH surge. Endocrinology 136:3673-3676[Abstract].
Wiemann JN, Clifton DK, Steiner RA (1990) Gonadotropin-releasinghormone messenger ribonucleic acid levels are unaltered with changesin the gonadal hormone milieu of the adult male rat. Endocrinology 127:523-532[Abstract/Free Full Text].
Wu TJ, Segal AZ, Miller GM, Gibson MJ, Silverman A-J (1992) FOSexpression in gonadotropin-releasing hormone neurons: enhancementby steroid treatment and mating. Endocrinology 131:2045-2050[Abstract/Free Full Text].
Zoeller RT, Young WS (1988) Changesin cellular levels of messenger ribonucleic acid encoding gonadotropinreleasing hormone in the anterior hypothalamus of female ratsduring the estrous cycle. Endocrinology 123:1688-1689[Abstract/Free Full Text].

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