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The Journal of Neuroscience, June 1, 1998, 18(11):4344-4352
Divergence in the Expression of Molecular Markers of Neuronal Activation in the Parvocellular Paraventricular Nucleus of the Hypothalamus Evoked by Alcohol Administration via Different Routes
Kathleen M. Ogilvie, Soon Lee, and Catherine Rivier The Clayton Foundation Laboratories for Peptide Biology, The Salk Institute for Biological Studies, La Jolla, California 92037
ABSTRACT
Top
Abstract
Introduction
Immediate early gene (IEG) expression has been routinely used by neuroscientists as an index of neuronal activation. In the case of the hypothalamic-pituitary-adrenal axis, induction of c-fos and/or NGFI-B mRNAs in the parvocellular paraventricular nucleus (pPVN) has been documented after a variety of stimuli that increase adrenocorticotropin (ACTH) in the systemic circulation. However, the functional relationship between expression of IEGs and transcription of the genes for the ACTH secretagogues corticotropin-releasing factor (CRF) and arginine vasopressin (AVP) is not clear. While investigating the neuroendocrine correlates of alcohol administration via different routes (intraperitoneal vs intragastric), we noted a difference in the time course of NGFI-B mRNA expression in the pPVN, despite comparable dynamics in ACTH secretion. By comparing the temporal cascade of transcriptional events in vivo after alcohol injection via either route, we sought to determine functional relationships between IEGs and the induction of CRF and AVP heteronuclear RNAs (hnRNAs). One advantage of our paradigm is the use of the same stimulus (systemic alcohol injection) in which access to the CNS does not differ between the groups to be compared. Intraperitoneal administration of the drug resulted in significant increases in c-fos mRNA, Fos protein, CRF hnRNA, and AVP hnRNA. In contrast, intragastric treatment evoked a brief, modest elevation in c-fos mRNA and Fos protein, increased AVP hnRNA, and caused no detectable change in CRF hnRNA. These data indicate that robust increases in CRF hnRNA are closely linked to full expression of c-fos mRNA and Fos protein. In addition, the expression of NGFI-B after both routes of administration is indicative of cellular activation within the pPVN in parallel with secretion of ACTH.
Key words: hypothalamic-pituitary-adrenal axis; adrenocorticotropin; corticotropin-releasing hormone; arginine vasopressin; c-fos mRNA; Fos protein; NGFI-B mRNA
INTRODUCTION
Secretion of adrenocorticotropin (ACTH) is largely regulated by neurons localized in the parvocellular paraventricular nucleus (pPVN) (Antoni, 1986
) that synthesize corticotropin-releasing factor (CRF) and arginine vasopressin (AVP) (Swanson and Sawchenko, 1983
Examination of immediate early gene (IEG) expression (e.g., c-fos and NGFI-B mRNAs) has been widely used as a marker of neuronal activation (Sagar et al., 1988
Because unselected laboratory rodents do not spontaneously consume alcohol, the study of the neuroendocrine effects of this drug relies on its forceful administration. Although we have used intraperitoneal cannulae in the past, we recently adopted intragastric cannulae that allow for alcohol delivery into the stomach, because this latter route may be more relevant to human use of the drug. Previously, we reported that intraperitoneal or intragastric alcohol administration evoked comparable ACTH secretion, with peak levels occurring at 30 min and lasting 2 hr. Although both groups of rats given alcohol had high levels of NGFI-B mRNA, peak expression was observed 1 hr after intraperitoneal treatment but 2 hr after intragastric treatment (Ogilvie et al., 1997a
MATERIALS AND METHODS
Animals. Male Holtzman rats weighing 180-200 gm were purchased from Harlan Sprague Dawley (Indianapolis, IN) and were maintained in groups (three to four rats per cage) on a 12 hr light/dark cycle (lights on at 6:00 A.M.). Under halothane anesthesia, all animals were implanted with both intragastric and intraperitoneal cannulae 7-8 d before experimentation. This approach was used to ensure identical surgical procedures in all rats and to eliminate the possibility that differences in RNA expression might be, at least in part, attributable to the surgical process. Intragastric cannulae were constructed of polyethylene tubing (PE90) expanded twice, ~5 mm apart, at the end inserted into the stomach. Using a dorsal approach, a small hole was cut in the skin and body musculature below the ribs on the rat's left side. The stomach was pulled through the opening, and a hole was made with spreader forceps in the fundus through which the cannula was inserted into the stomach. The cannula was sutured in place between the two bubbled parts of the cannula to retain the tip in the lumen of the stomach. With the aid of a trochar, the cannula was exteriorized through the body wall and passed under the skin to exit at the nape of the neck, where it was capped with a steel pin. Intraperitoneal cannulae were made of PE60 so that they could be distinguished from intragastric cannulae and placed as previously described (Ogilvie and Rivier, 1996
Experimental protocol. On the day of an experiment, animals were removed to a soundproof room and their cannulae were extended with PE tubing connected to syringes containing sterile saline. Rats were housed individually in opaque buckets with pine shavings and left undisturbed for 3 hr. Beginning at 11:00 A.M. animals were injected with alcohol (see below) via either the intraperitoneal or intragastric cannula and killed 10-240 min later (n = 5 per group). Uninjected controls were killed throughout the experimental session and processed in parallel with treated animals. Previous work in our laboratory has shown that rats injected with the vehicle do not have upregulated levels of c-fos mRNA, Fos protein, NGFI-B mRNA, CRF hnRNA, or AVP hnRNA after either route of injection, intraperitoneal (Lee and Rivier, 1994
20°C if they were intended for immunocytochemistry or placed in 4% paraformaldehyde and stored at 4°C for an additional 4 d if they were intended for in situ hybridization. Tissues from the first replicate of this experiment were probed for NGFI-B mRNA, CRF hnRNA, and AVP hnRNA. Sections from the second replicate were analyzed for Fos protein, c-fos mRNA, and CRF hnRNA.
Alcohol treatment. Alcohol was given at a dose of 3 gm/kg of body weight in a solution of saline containing 10% lidocaine to minimize discomfort. We chose this dose of alcohol, which produces a moderate degree of intoxication, based on preliminary experiments in which changes in expression of CRF and AVP mRNAs in the PVN were found to be most consistent and robust after intraperitoneal administration (Lee and Rivier, 1998
Immunocytochemistry. Because of the number of samples generated, immunocytochemistry was done in batches. To control for variation between these cohorts, samples were processed such that half of each group (time and injection route) were subject to immunocytochemistry at the same time.
Immunocytochemistry for Fos was performed as previously described (Ogilvie and Rivier, 1997
-globulin for 45 min, washed, and incubated with horseradish peroxidase-avidin complex for 45 min. To enhance the specificity of the reaction, sections were treated again with second antibody (30 min), washed, and incubated a second time with horseradish peroxidase-avidin complex (30 min). Color product was formed by incubating with DAB and hydrogen peroxide with nickel intensification (black product). Sections were mounted on poly-L-lysine-coated slides, vacuum-dried overnight, dehydrated through an alcohol series, cleared in xylenes, and coverslipped with a mixture of distrene, tricresyl phosphate, and xylene (DPX) (13512, Electron Microscopy Sciences).
In situ hybridization. Protocols for riboprobe synthesis, hybridization, and autoradiography were adopted from those of Simmons et al. (1989)
The pBluescript SK-1 vector (Stragene, La Jolla, CA) containing a 2.0 kb EcoRI fragment of rat c-fos cDNA (Dr. I. Verma, The Salk Institute, La Jolla, CA) was linearized with SmaI. The pGEM3 plasmid containing a 530 bp fragment of CRF intron (Dr. S. Watson, University of Michigan, Ann Arbor, MI) and pGEM3 plasmid containing a 700 bp PvuII fragment of rat vasopressin gene fragment of intron I (Dr. T. Sherman, Georgetown University, Washington, DC) were linearized with HindIII. Radioactive cRNA copies were synthesized by incubation of 250 ng of linearized plasmid in 6 mM MgCl2, 36 mM Tris, pH 7.5, 2 mM spermidine, 8 mM dithiothreithol, 25 mM ATP, GTP, and CTP, [
-35S]UTP or [33P]UTP, 1 U of RNasin (Promega, Madison, WI), and 10 U of T7 (for c-fos, CRF intron, and AVP intron) for 60 min at 37°C. Unincorporated nucleotides were removed using Quick-Spin columns (Boehringer Mannheim, Indianapolis, IN). A sense probe, of the same size as the corresponding antisense probe, was used as a control for nonspecific signal in some adjacent sections (negative control).
Before hybridization, tissue sections (every fifth section) were mounted onto gelatin- and poly-L-lysine-coated slides and dried under vacuum overnight, fixed (4% paraformaldehyde, 30 min), digested by proteinase K (catalog #24568; Merck, Darmstadt, Germany; 10 µg/ml at 37°C for 25 min), rinsed in triethylamine (0.1 M TEA, pH 8.0), acetylated (25% acetic anhydride in TEA), and dehydrated through an alcohol series (50, 70, 100, and 100%, 3 min each). After vacuum-drying, the c-fos, CRF intron, and AVP intron cRNA probes were applied to each slide in 90 µl of hybridization mixture [107 cpm/ml, 10 mM formamide, 36 mM NaCl, 1.2 mM Tris HCl, 1.2 mM EDTA, 1× Denhardt's solution, 10% dextran sulfate, 0.5 mg/ml tRNA (catalog #109541, Boehringer Mannheim), and 10 mM DTT] and sealed under a coverslip with DPX (13512, Electron Microscopy Sciences). After incubation at 60°C overnight, coverslips were removed, and sections were rinsed in four washes of 4× SSC (20× SSC = 3 M NaCl and 0.3 M citric acid, pH 7.0). Sections were digested in RNase A (20 µg/ml) at 37°C, for 30 min, washed in decreasing concentrations of SSC (2, 2, 1, and 0.5× for 5 min each), washed in 0.1× SSC (60°C for 30 min), and dehydrated through an alcohol series (50, 70, 95, 100, and 100%, 3 min each). Sections were dried under vacuum and exposed on x-ray film (1-3 d; Biomax, Eastman Kodak, Rochester, NY), defatted in xylenes, and dipped in nuclear emulsion (NTB2 diluted 1:1 in distilled water, Kodak). Slides were then exposed for 10 d-6 weeks and developed (D19, Kodak; 15°C for 3.5 min), fixed (Kodak; 15°C for 6 min), rinsed, counterstained with thionin (0.25%), dehydrated through an alcohol series (95, 100, and 100%, 3 min each), cleared with xylenes, and coverslipped with DPX.
Because of the number of samples generated, in situ hybridization was done in two parts for each probe, segregated by injection route to maximize detection of temporal changes. However, we also included brain tissues within each batch that were known to express transcripts of the RNA to be measured (slides from animals treated with alcohol intraperitoneally in a separate experiment; positive control) to ensure that the absence of signal in some groups was not attributable to failed hybridization. In addition, we prolonged exposure times such that we were able to detect very low in situ hybridization signal.
Semiquantitative analysis of in situ hybridization results. Densitometric analysis of hybridization signals for c-fos mRNA, CRF hnRNA, and AVP hnRNA was performed in nuclear emulsion-dipped slides. The mean optical density (OD) of hybridization signal was measured under dark-field illumination using a Leitz (Wetzlar, Germany) optical system coupled with a Macintosh Power PC and Image software (version 1.60; W. Rasband, National Institutes of Health). Under bright-field illumination, first the parvocellular (pPVN) subdivision of the PVN (Swanson and Sawchenko, 1983
Statistical analysis. Levels of hybridization were subject to two-way ANOVA with route of injection (intraperitoneal vs intragastric) and time as the variables. Post hoc analysis was accomplished using the least squares means test.
RESULTS
Expression of c-fos mRNA and Fos protein
There was a significant effect of the route of alcohol injection on expression of c-fos mRNA in the pPVN (p = 0.0027), as well as significant changes in mRNA levels over time (p = 0.0124). After intraperitoneal injection of alcohol, levels of pPVN c-fos mRNA were already significantly elevated within 10 min and peaked 60 min after injection, at which time expression of c-fos mRNA was 35-fold higher than in noninjected controls (1.10 ± 0.62 OD units; Table 1, Fig. 1). Levels of c-fos mRNA continued to be elevated in the pPVN of these rats for the duration of the experiment (240 min). In contrast, rats injected with alcohol intragastrically had two smaller rises in c-fos mRNA levels (~10-fold over a control value of 1.29 ± 0.80 OD units), with the greatest levels detected 30 and 240 min after injection. In the mPVN, expression of c-fos mRNA was not significantly increased over control values of 3.31 ± 1.51 (intraperitoneal) or 1.38 ± 0.68 (intragastric) OD units by exposure to alcohol via either route (p = 0.3881), nor did levels change over time (p = 0.3414).
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Table 1. Levels of pPVN and mPVN RNA after intraperitoneal and intragastric injection of alcohol
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Figure 1. Expression of c-fos mRNA (dark-field photomicrographs) and Fos protein (bright-field photomicrographs) in the paraventricular nucleus of male rats injected with alcohol intraperitoneally (left panels, ip) or intragastrically (right panels, ig) at the times indicated (in minutes). Note that in contrast to the robust activation in response to the drug administered intraperitoneally, rats that received alcohol into the stomach had only small elevations in c-fos mRNA (at 30 and 240 min) and expressed Fos protein only in scattered cells (at 60 min). Magnification, 145×.
Congruent with the results for c-fos mRNA, Fos protein was robustly increased in the pPVN after intraperitoneal injection of alcohol (Fig. 1). Maximal activation, involving cells throughout the pPVN, was observed at 120 min after injection and persisted until 240 min after alcohol. We also observed a few cells that contained Fos in the pPVN of rats injected intragastrically with the drug 60 min before killing.
Expression of CRF hnRNA
There was a significant effect of the route of alcohol injection on expression of CRF hnRNA in the pPVN (p = 0.0060), as well as significant changes in transcript levels over time (p = 0.0002). As we have described previously, constitutive levels of CRF hnRNA in the pPVN are very low (intraperitoneal controls, 1.13 ± 0.71 OD units; intragastric controls, 1.83 ± 0.94 OD units) but readily induced by intraperitoneal injection of alcohol (Rivier and Lee, 1996
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Figure 2. Expression of CRF hnRNA in the paraventricular nucleus of male rats injected with alcohol intraperitoneally (top) or intragastrically (bottom) at the times indicated (in minutes). Note that CRF hnRNA was expressed robustly in animals injected intraperitoneally, whereas levels were not detectable in rats that received alcohol intragastrically. Magnification, 130×.
Expression of AVP hnRNA
Although initially suppressed after intraperitoneal injection of alcohol, levels of AVP hnRNA in the pPVN were elevated by administration of alcohol (p = 0.0402) via either route (p = 0.0125), with the highest level of expression measured at 180 min (Table 1, Fig. 3). There was no interaction of these two variables (p = 0.6172), indicating that the time course of the response was similar regardless of route of injection. Constitutive expression of AVP hnRNA was greater in the mPVN than in the pPVN, reflecting the larger number of cells in this area of the nucleus that synthesize this peptide (Sawchenko et al., 1984
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Figure 3. Expression of AVP hnRNA in the paraventricular nucleus of male rats injected with alcohol intraperitoneally (top) or intragastrically (bottom) at the times indicated (in minutes). Note that expression of AVP hnRNA in the parvocellular portion of the nucleus increased over time, regardless of the route of injection. Magnification, 130×.
Summary of data
Figure 4 summarizes all of our data on the expression of IEGs, CRF hnRNA, and AVP hnRNA in the pPVN after administration of alcohol intraperitoneally or intragastrically. In response to elevated BALs, male rats injected with the drug via either route secrete comparable amounts of ACTH over a similar time course (Ogilvie et al., 1997a
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Figure 4. Summary of the temporal activation of hypothalamic-pituitary-adrenal axis in male rats injected intraperitoneally (top) or intragastrically (bottom) with alcohol. Gray polygons indicate the duration of detectable increases in the measure, whereas the widest portion of the polygon indicates the time at which peak levels were attained. In response to rising blood alcohol levels, ACTH is released from the anterior pituitary. Although the secretion of ACTH is of similar magnitude and duration after either route of injection, alcohol-induced activation of CRF hnRNA in the parvocellular division of the paraventricular nucleus of the hypothalamus (pPVN) is only observed in rats that received the drug intraperitoneally. Furthermore, in rats injected with alcohol intragastrically, expression of the c-fos mRNA and Fos protein is confined to a few cells in the pPVN and is abbreviated in comparison to animals injected intraperitoneally.
DISCUSSION
We show here that upregulated primary transcription of CRF (as indicated by elevated expression of hnRNA) is accompanied by robust increases in c-fos mRNA and Fos proteins throughout the parvocellular PVN of rats injected with alcohol intraperitoneally. This contrasted with results obtained in animals treated with the drug intragastrically, which showed no increase in CRF hnRNA and significantly less expression of c-fos mRNA or its protein. These results indicate that the activation of c-fos and CRF gene expression might be closely linked. Because expression of c-fos mRNA precedes demonstrable increases in CRF hnRNA in this model, an observation also made after other homeostatic threats (Imaki et al., 1992
We have previously shown that levels of NGFI-B mRNA were elevated after alcohol injection regardless of route of injection in these same animals (Ogilvie et al., 1997a
Distinct combinations of IEGs are thought to confer specificity in the cellular response to different stimuli, and there are known differences in the kinetics and the magnitude of responses (Sheng and Greenberg, 1990
via different routes (intravenously vs intracerebroventricularly) (Rivest et al., 1992
In conclusion, our data show parallel activation of c-fos mRNA, Fos protein, and CRF hnRNA in male rats injected with alcohol intraperitoneally, suggesting that these cellular events may depend on the same primary phenomenon (possibly increased cAMP). On the other hand, expression of NGFI-B throughout the pPVN took place in all animals injected with alcohol, regardless of route. This latter finding confirms that cellular activation in the pPVN had occurred, despite the lack of robust increases in CRF hnRNA, c-fos mRNA, and Fos protein in rats that received the drug intragastrically. This demonstrates the requirement for careful interpretation of IEG data, especially when induction is not manifest. For instance, had we only examined expression of NGFI-B, we would have concluded that alcohol stimulated hypothalamic activity in a similar manner, regardless of route of administration. In contrast, reliance on either c-fos mRNA or Fos protein expression alone would have suggested that alcohol given intragastrically did not result in cellular activation at the level of the pPVN. Taken together, however, our data indicate that alcohol can evoke ACTH secretion via at least two mechanisms, both of which effect neurons in the pPVN.
FOOTNOTES Received Oct. 15, 1997; revised March 6, 1998; accepted March 13, 1998.
We are grateful to Drs. T. Sherman, I. Verma, and S. Watson for gifts of reagents and to W. Kau, P. Senarith, J. Lacsamana, J. Woo, and Y. Haas for technical assistance.
Correspondence should be addressed to Dr. Catherine Rivier, The Clayton Foundation Laboratories for Peptide Biology, The Salk Institute for Biological Studies, 10010 North Torrey Pines Road, La Jolla, CA 92037.
Dr. Ogilvie's present address: Department of Pharmacology, Ligand Pharmaceuticals, 10275 Science Center Drive, San Diego, CA 92121.
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