Urocortin III-Immunoreactive Projections in Rat Brain: Partial Overlap with Sites of Type 2 Corticotrophin-Releasing Factor Receptor Expression

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The Journal of Neuroscience, February 1, 2002, 22(3):991-1001

Urocortin III-Immunoreactive Projections in Rat Brain: Partial Overlap with Sites of Type 2 Corticotrophin-Releasing Factor Receptor Expression
Chien Li¹, Joan Vaughan¹, Paul E. Sawchenko², and Wylie W. Vale¹
¹ The Clayton Foundation Laboratories for Peptide Biology and ² Laboratory of Neuronal Structure and Function, The Salk Institute for Biological Studies, La Jolla, California 92037

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Urocortin (Ucn) III, or stresscopin, is a new member of the corticotropin-releasing factor (CRF) peptide family identifiedin mouse and human. Pharmacological studies showed that Ucn IIIis a high-affinity ligand for the type 2 CRF receptor (CRF-R2).To further understand physiological functions the peptide mayserve in the brain, the distribution of Ucn III neurons and fiberswas examined by in situ hybridization and immunohistochemistryin the rat brain. Ucn III-positive neurons were found predominatelywithin the hypothalamus and medial amygdala. In the hypothalamus,Ucn III neurons were observed in the median preoptic nucleus andin the rostral perifornical area lateral to the paraventricularnucleus. The Ucn III fibers were distributed mainly in the hypothalamusand limbic structures. Hypothalamic regions that were innervatedprominently by Ucn III fibers included the ventromedial nucleus,medial preoptic nucleus, and ventral premammillary nucleus. Outsidethe hypothalamus, the densest projections were found in the intermediatepart of the lateral septum, posterior division of the bed nucleusstria terminalis, and the medial nucleus of the amygdala. Severalmajor Ucn III terminal fields identified in the present study,including the lateral septum and the ventromedial hypothalamus,are known to express high levels of CRF-R2. Thus, these anatomicaldata strongly support the notion that Ucn III is an endogenousligand for CRF-R2 in these areas. These results also suggest thatUcn III is positioned to play a role in mediating physiologicalfunctions, including food intake and neuroendocrineregulation.

Key words: urocortin; CRF; perifornical hypothalamus; medial amygdala; ventromedial hypothalamus; CRF-R2

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The corticotropin-releasing factor (CRF) family consists of a growing number of peptides identified in a variety of species(Perrin and Vale, 1999). In addition to CRF, three CRF-relatedpeptides, urocortin (Ucn) (Vaughan et al., 1995), Ucn II (Reyeset al., 2001), and Ucn III (Lewis et al., 2001), have been identifiedin humans, rodents, and other mammalian species. Human Ucn III,also known as stresscopin (Hsu and Hsueh, 2001), is the latestaddition to this family. Sequence analysis shows that the predictedhuman and mouse Ucn III mature peptides are 90% identical andclosely related to a urocortin-related peptide identified originallyin pufferfish (Brunner et al., 2000) but exhibit less relatednessto the other mammalian family members (Lewis et al., 2001). Invitro binding studies showed that both human and mouse Ucn IIIbound the type 2 CRF receptor (CRF-R2) with high affinity butdid not bind to the other known receptor for the family, CRF-R1(Hsu and Hsueh, 2001; Lewis et al., 2001). Accordingly, Ucn IIIstimulated cAMP production in cells expressing CRF-R2 but notin cells expressing CRF-R1 (Hsu and Hsueh, 2001; Lewis et al.,2001). These data identify Ucn III as a high-affinity ligand forCRF-R2.

In brain, CRF-R2 is expressed in discrete regions, including the lateral septum and ventromedial hypothalamus in the forebrainand dorsal raphe and nucleus of the solitary tract in the hindbrain(Chalmers et al., 1995; Van Pett et al., 2000). Central CRF-R2has been implicated as playing important regulatory roles in feeding(Spina et al., 1996; Makino et al., 1998; Nishiyama et al., 1999;Ohata et al., 2000), gastric motility (Martinez et al., 1997;Martinez and Tache, 2001), anxiety (Bale et al., 2000; Coste etal., 2000; Kishimoto et al., 2000), and stress-associated learning(Radulovic et al., 1999). However, an important question thathas remained unresolved is the ligand responsible for the activationof CRF-R2 in the brain. Ucn was originally proposed to be an endogenousligand for CRF-R2 in the brain based on its high affinity forthe receptor (Vaughan et al., 1995). However, anatomical datahave shown that most major sites of CRF-R2 expression are poorlyinnervated by Ucn-containing projections (Kozicz et al., 1998;Bittencourt et al., 1999), suggesting that additional family peptides,such as Ucn II or Ucn III, might serve as endogenous ligand forCRF-R2 in some brainregions.

To further characterize the distribution of Ucn III in the brain and to highlight potential functional associations, we performedimmunohistochemical studies examining the distribution of UcnIII neurons and fibers in the rat brain. The wide distributionof Ucn III fibers observed in the present study suggests thatthe peptide may be involved in a variety of physiological functions.In addition, the presence of Ucn III fibers in many brain regionsthat also express CRF-R2 strongly suggested that Ucn III couldfunction as an endogenous ligand for CRF-R2.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Perfusion and fixation. Adult male Sprague Dawley rats weighing 275-350 gm were used for the present studies. To facilitatethe visualization of Ucn III cell body by immunohistochemistry,some animals (n = 5) received 10 µl of colchicine (10 µg/µl in0.9% saline) into a lateral ventricle 2 d before perfusion. Animalswere anesthetized with an overdose of choral hydrate (1 gm/kgbody weight, i.p.) and perfused transcardially with 150 ml ofsaline, followed by 350 ml of 4% paraformaldehyde in borate buffer,pH 9.5. The brains were removed and post-fixed in 25% sucrosein the same fixative at 4°C overnight. They were then quicklyfrozen in dry ice and sectioned at 25 µm using a sliding microtomeand stored in cryoprotectant at $-$ 20°C until use. All animal procedureswere approved by the Salk Institute Institutional Animal Careand UseCommittee.

Antiserum and controls. Anti-Ucn III serum (PBL #6570) was raised in rabbit against synthetic human GlyTyr-Ucn III conjugatedto human $alpha$ -globulins via bisdiazotized benzidine. To test thespecificity of the antiserum for immunohistochemistry, the antiserum(1:200) was preincubated for 24 hr at 4°C with 0-300 µM synthetichuman or mouse Ucn III, mouse Ucn II, rat Ucn, human-rat CRF,or fish urotensin I before incubation with brainsections.

Immunohistochemistry. Brain sections were removed from cryoprotectant and rinsed in 0.05 M potassium PBS (KPBS), followedby treatment with 1% NaBH₄-KPBS solution. Sections were incubatedin rabbit anti-Ucn III antiserum (1:19,000 final dilution) inKPBS with 0.4% Triton X-100 at room temperature for 1 hr and thenat 4°C for 48 hr. The tissues were then rinsed in KPBS and incubatedin biotinylated donkey anti-rabbit IgG (1:700; Jackson ImmunoResearch,West Grove, PA) in KPBS with 0.4% Triton X-100 for 1 hr at roomtemperature. This was followed by another 1 hr incubation at roomtemperature in avidin-biotin complex solution (Vectastain ABCElite kit; Vector Laboratories, Burlingame, CA). The antibody-peroxidasecomplex was visualized with a mixture of nickel sulfate (25 mg/ml),3,3-diaminobenzidine (0.2 mg/ml), and 3% H₂O₂ (0.83 µl/ml) in175 mM sodium acetate solution. When the staining had reachedthe appropriate intensity, the tissue was rinsed in KPBS and mountedon gelatin-coated glass slides. Slides were dehydrated throughgraded alcohols, cleared in xylenes, and coverslipped with DPXmountant (Electronic Microscope Science, Fort Washington, PA).Adjacent series of brain sections were processed for Nissl stainingfor referencepurposes.

In situ hybridization. Animals were quickly decapitated, and the brains were removed and frozen in dry ice. Coronal sections(20 µm thick) were cut on a cryostat, thaw-mounted onto glassslides, and stored at $-$ 80°C until use. An antisense cRNA probewas transcribed from a linearized 528 bp mouse Ucn III cDNA andlabeled with [³⁵S]UTP (PerkinElmer Life Sciences, Emeryville, CA). The specificactivity of the probe was ~1-3 × 10⁸ dpm/µg cRNA. The saturating concentration for the probe usedin the assay was 0.3 µg/ml·Kb.

The procedure for in situ hybridization has been described previously (Li et al., 1998). Briefly, the brain sections werefixed in 4% paraformaldehyde and treated with 0.25% acetic anhydridein 0.1 M triethanolamine, pH 8.0, followed by a rinse in 2× SSC,dehydrated through a graded series of alcohols, delipidated inchloroform, rehydrated through a second series of alcohols, andthen air dried. The slides were exposed to the cRNA probe overnightin humidified chambers at 55°C. After incubation, the slides werewashed in SSC of increasing stringency, in RNase, and then in0.1× SSC at 63°C, dehydrated through a graded series of alcohols,and dried. Slides were dipped in NTB-2 emulsion (Eastman Kodak,Rochester, NY), exposed for 10 d at 4°C, and developed. Afterdevelopment, the slides were counterstained with cresylviolet.

Imaging. Slides were examined using a Leica (Nussloch, Germany) light microscope, and images were captured onto Kodak Ektachrome64T (tungsten) films. The films were scanned into a computer usinga Nikon (Tokyo, Japan) LS1000 35 mm film scanner. The images werecropped and adjusted to balance brightness and contrast in AdobePhotoshop (version 5.5; Adobe Systems, San Jose, CA) before importinto Canvas (version 6.0) for assembly into plates. Schematicmapping of Ucn III neurons and fibers in brain sections was performedin Adobe Illustrator (version 7.01) using coronal brain platesfrom the rat brain atlas of Swanson (Swanson, 1999) as templates.The brain plates were then imported into Canvas forreordering.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Antiserum specificity

To evaluate the specificity of the anti-Ucn III serum, the antiserum was preincubated with synthetic peptides of varying concentrationsbefore use for immunohistochemistry. The results of the competitionstudies are summarized in Table 1. Staining for Ucn III cellsand fibers in the brain was completely abolished by preincubationof the antiserum with synthetic mouse or human Ucn III at concentrationsin the low micromolar range [Fig. 1, Tables 1, 2 (Table 2 includesa list of abbreviations used in the figures)]. Ucn, Ucn II, andurotensin I each failed to block the Ucn III-specific staining,even at the highest concentration used (Table 1). CRF was alsoineffective in competing Ucn III-specific staining in all areasexamined, except the external zone of the median eminence, inwhich the Ucn III immunoreactivity was blocked by preabsorptionwith low concentration of CRF. Consequently, Ucn III antiserumwas routinely absorbed with 30 µM CRF before use to eliminatethe cross-reactivity observed in the median eminence.


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Table 1. Competition characteristics of Ucn III immunoreactivity in rat brain

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Figure 1. Representative photomicrographs showing Ucn III immunostaining in the LS (A, B) and VMH (C, D) with (B, D) or without (A, C) preabsorbing the anti-Ucn III serum with 3 µM human Ucn III before use. The dense crescent-shaped Ucn III terminal field in the LS (A) and abundant fibrous staining in the VMH (C) were effectively blocked by preabsorption with Ucn III (B, D). Note that some Ucn III-positive cells (arrow) in the dorsal hypothalamic area in C were also blocked (D). Scale bars, 50 µm.


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Table 2. List of abbreviations used in the figures

Distribution of Ucn III cell bodies

Both immunohistochemical and hybridization histochemical methods detected Ucn III-positive neurons in several restricted areasin the brain. The distribution of Ucn III-IR neurons identifiedby immunohistochemistry in colchicine-treated rats was similarto that identified by in situ hybridization (Figs. 2, 3), furthervalidating the specificity of the Ucn III antiserum used in thepresent study.

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Figure 2. Representative dark-field (left) and bright-field (right) photomicrographs showing the distribution of Ucn III mRNA and Ucn III immunoreactivity, respectively, in selected hypothalamic areas. In the MePO (A, B), both methods detected Ucn III-positive neurons along the midline of the rostral end of the third ventricle. In the rostral perifornical area near the anterior part of the PVH (C, D), both preparations labeled a cluster of cells medial to the fornix. At the level of mid-PVH (E, F), Ucn III neurons were observed medial to the fornix and lateral to the PVH, whereas only a few cells were found inside the PVH. Scale bars, 50 µm.

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Figure 3. Representative dark-field (left) and bright-field (right) photomicrographs showing Ucn III neurons in the MEA and the superior paraolivary nucleus (SPO) detected by in situ hybridization (left) and immunohistochemistry (right), respectively. In the MEA (A, B), Ucn III-positive neurons were seen closely associated with the optic tract (opt). In the brainstem (C, D), scattered Ucn cells (arrowheads) were found close to the medial edge of the superior paraolivary nucleus (E, F). Scale bars, 50 µm.

In agreement with our previous hybridization histochemical analysis (Lewis et al., 2001), Ucn III neurons were found in discretesubcortical regions of the brain, including the preoptic region,hypothalamus, and amygdala. In the hypothalamus, labeled neuronswere localized in two major areas. The first group of Ucn IIIneurons was found in the median preoptic nucleus (MePO) liningthe rostral margin of the third ventricle (Fig. 2A,B), with afew lightly labeled cells found in the ventrolateral part of themedial preoptic area and also in the lateral preoptic area. Thesecond group of Ucn III neurons was located in a poorly definedarea closely associated with the fornix (Fig. 2C-F) at the levelof paraventricular nucleus (PVH). The cell group extended rostrallyinto several subnuclei of the posterior division of the bed nucleusof stria terminalis (BST), with a few scattered cells seen atthe caudal part of the anterior division. Intensely stained cellswere observed mostly in the perifornical area between the fornixand the PVH, with a few cells found in the anterior parvicellular(Fig. 2C,D) and the magnocellular (Fig. 2E,F) parts of the PVH.More caudally, the cell group remained closely lateral to thePVH, whereas the fornix gradually shifted laterally toward thelateral hypothalamic area. A few scattered cells were found inthe rostral part of the dorsomedial hypothalamic area. No UcnIII cells were seen within the hypothalamus caudal to the levelof the compact zone of the dorsomedial hypothalamus. ScatteredUcn III neurons were present in the periventricular zone alongthe third ventricle and in the area dorsal to the supraopticnucleus.

Outside the hypothalamus, most of the Ucn III neurons were found in the amygdala, in which Ucn III neurons were concentratedin the dorsal division of the medial nucleus of the amygdala (MEA).In the anterodorsal division of the MEA, Ucn III cells were foundclosely associated with the optic tract (Fig. 3A,B). In the posterodorsalpart of the MEA, the cell population shifted away from the optictract and was concentrated in the lateral part of the MEA. Scatteredcells were also observed in the posterior cortical nucleus ofthe amygdala and the amygdalohippocampal transition area. In thebrainstem, Ucn III neurons were found in the auditory complex,including the superior paraolivary nucleus (Fig. 3E,F) and extendingto the nucleus of trapezoidbody.

Distribution of Ucn III fibers

Immunohistochemical staining using the Ucn III antiserum revealed staining of axons and varicosities in the subcortical regions,including several limbic structures and the hypothalamus, althoughno fibers were found in the cortex and the cerebellum. The distributionof Ucn III-IR fibers in the brain is illustrated in Figure 4 atseveral representative levels.

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Figure 4. Schematic drawings of 25 µm coronal sections showing the distribution of Ucn III-immunoreactive cells bodies (black dots) and fibers in the rat brain. (Figure 4 continues.)

In the hypothalamus, the densest Ucn III-IR fibers were found in the ventromedial nucleus (VMH), the predominate site of CRF-R2expression within the hypothalamus (Chalmers et al., 1995; VanPett et al., 2000). An extremely high concentration of Ucn III-IRfibers was observed in the dorsomedial part of the VMH (Fig. 5B),whereas the central and ventrolateral parts of the nucleus receiveda somewhat less dense innervation. This pattern was most salientat caudal levels of the VMH (Fig. 5C). Abundant Ucn III-IR fiberswere also found in the area between the VMH and the arcuate nucleusand extended into the lateral part of the arcuate nucleus proper(Fig. 5B). Abundant Ucn III fibers and terminals also innervatedthe rostral part of the arcuate nucleus and extended into theretrochiasmatic area (Fig. 5E). Very few fibers were found inthe dorsomedial nucleus (Fig. 5B,C) and the lateral hypothalamus(Fig. 4). In the anterior hypothalamic region, abundant Ucn III-IRfibers were observed in the rostral perifornical area (Fig. 5D)surrounding the Ucn III neurons. Very few fibers terminated inthe anterior hypothalamus, the supraoptic nucleus, and neurosecretorysubdivisions of the PVH (Fig. 5D). In the preoptic area, Ucn III-IRfibers were found predominately in the medial preoptic nucleus(Fig. 5A), with scant fibers observed in the organum vasculosumof lamina terminalis, the subfornical organ, and the MePO. Inthe posterior hypothalamic region, Ucn III-IR fibers coursed throughthe supramammillary nucleus and terminated in the ventral premammillarynucleus (Fig. 5G). Scattered fibers were found in posterior hypothalamus.In the median eminence, Ucn III-IR fibers were seen only in theinternal zone (Fig. 5F).

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Figure 5. Dark-field photomicrographs showing abundant Ucn III-immunoreactive fibers in discrete hypothalamic areas, including the medial preoptic nucleus (A), the rostral (B) and caudal part (C) of the ventromedial nucleus, the rostral part of the arcuate nucleus (E), and the ventral premammillary nucleus (G), whereas only a few fibers were found in the PVH (D). Also note that only a few scatter fibers were found in the dorsomedial nucleus (C). In the median eminence (F; ME), Ucn III fibers (indicated by arrowheads) were found only in the internal zone of the median eminence. Scale bar, 50 µm.

Outside the hypothalamus, Ucn III-IR fibers were most abundant in discrete aspects of limbic structures, including the lateralseptum (LS), the posterior division of the BST, and the medialamygdala, areas also known to express high levels of CRF-R2 (Chalmerset al., 1995; Van Pett et al., 2000). In the LS, an exceedinglydense Ucn III terminal field in a crescent-shaped pattern occupiedthe lateral edge of the intermediate part of the LS along thelateral ventricle (Fig. 6A). At this level, a few scattered fiberswere also observed around the anterior commissure. In the BST,dense Ucn III-IR fibers were found occupying the posterior division(Fig. 4E, 6B), whereas very few labeled fibers were observed inthe rostral division. In the amygdala (Fig. 6C), the majorityof the Ucn III-IR fibers were observed in the medial nucleus,including both its dorsal and ventral subnuclei. Scattered fibersalso extended into the basomedial subnuclei and the posteriorcortical nuclei of the amygdala. More caudally, Ucn III-IR fibersextended into the ventral hippocampus (Fig. 6D). In the thalamus,a few scattered fibers were found in the posterior part of theparaventricular nucleus and in the lateral habenula.

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Figure 6. Representative dark-field photomicrographs showing dense Ucn III-immunoreactive fibers in the intermediate (LSi) and ventral (LSv) parts of the LS (A), the posterior part of the BST (B), the MEA (C), and the caudal part of the hippocampus and amygdaloid areas (D). Note that the rostral portion of the anterior hypothalamus and supraoptic nucleus (SON) received little Ucn III innervation (B). Scale bars, 50 µm.

In the midbrain and brainstem, scattered fibers were observed in several areas with low levels of CRF-R2 expression (Van Pettet al., 2000). These areas include the dorsal and dorsolateralcolumns of the periaqueductal gray, the superior and inferiorcolliculi, and the ventral lateral lemniscus (Fig. 4O). Very fewor no fibers were observed in the dorsal raphe, interpeduncularnucleus, area postrema, and the nucleus of the solitary tract,regions with moderate to high levels of CRF-R2expression.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ucn III neuronal distribution

In the present study, Ucn III-expressing neurons were identified by in situ hybridization and immunohistochemistry. The immunostainingwas blocked by preabsorbing the antiserum with either mouse orhuman Ucn III but not by structurally related peptides, includingCRF, Ucn, and Ucn II. In addition, the distributions of Ucn IIIperikarya revealed by the two methods were in close accord, andneither approach produced any evidence of cross-reactivity withother known CRF family members (Swanson et al., 1983; Kozicz etal., 1998; Bittencourt et al., 1999). These results thus supportthe specificity of the localization reported here. The presentfindings confirm previously reported (Lewis et al., 2001) majorsites of Ucn III mRNA expression in the brain, including the MePOand the rostral perifornical area in the hypothalamus, dorsaldivision of the MEA, and the auditory complex in the brainstem.Colchicine pretreatment did not reveal additional populationsof Ucn III-expressing neurons in thebrain.

Ucn III fiber distribution

As summarized in Figure 4, Ucn III-positive fibers showed a distribution distant from those of CRF and Ucn (Swanson et al.,1983; Kozicz et al., 1998; Bittencourt et al., 1999). An importantcharacteristic of the fiber distribution, shown in Table 3, isthat most of the Ucn III fiber terminal fields in the forebrainalso express CRF-R2 (Chalmers et al., 1995; Van Pett et al., 2000).Areas with densest Ucn III innervation include the VMH, the LS,the posterior division of the BST, and the MEA, areas known toexpress high levels of CRF-R2. The close association between UcnIII terminal fields and the expression of the CRF-R2 supportsthe notion that Ucn III is an endogenous ligand for CRF-R2 inthese areas. In the hindbrain, however, some discrepancy betweenthe distribution of Ucn III fibers and the expression of CRF-R2was observed. Very few or no Ucn III fibers were found in thedorsal raphe, area postrema, and the nucleus of the solitary tract,regions that contain high levels of CRF-R2 (Chalmers et al., 1995;Van Pett et al., 2000). Interestingly, as summarized in Table3, these areas are innervated by Ucn fibers (Bittencourt et al.,1999), suggesting that the endogenous ligand for CRF-R2 in theseareas is Ucn rather than Ucn III. Together, the evidence suggeststhat Ucn III is positioned to serve as a major ligand for CRF-R2in the forebrain, whereas Ucn mediates the effects of CRF-R2 inthe hindbrain. Several brain regions, including the hippocampusand the cortical regions, have been shown to express CRF-R2 (Chalmerset al., 1995; Van Pett et al., 2000) but fail to possess impressiveUcn inputs (Bittencourt et al., 1999) or Ucn III innervations(present study). It is conceivable that another CRF-R2-selectiveligand, Ucn II, may innervate these areas. A detailed analysisof Ucn II distribution may resolve this issue.


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Table 3. Distribution of Ucn III and Ucn fibers relative to CRF-R2 mRNA expression in selective areas in rat brain

The distribution of Ucn III-IR fibers observed in the present study also appears to confirm the results from anatomical studiesdemonstrating the projections of major Ucn III cellular expressionsites. It has been shown that neurons in the rostral perifornicalarea project heavily into the LS, the posterior division of theBST, and the VMH (Wiegand and Price, 1980; Kita and Oomura, 1982;Risold et al., 1994). MEA has also been shown to project to thehypothalamus, including the VMH and the ventral premammillarynucleus, as well as to the BST and the amygdala (Canteras et al.,1995). This anatomical data suggests that Ucn III neurons in theperifornical area and the MEA are positioned to provide the majorityof the Ucn III innervations in thebrain.

It has been shown that the MePO projects heavily to neurosecretory neurons in the magnocellular part of the PVH and the supraopticnucleus (Sawchenko and Swanson, 1983; Weiss and Hatton, 1990)and into the circumventricular organs (Camacho and Phillips, 1981;Lind et al., 1982; Oldfield et al., 1992). However, in the presentstudy, only a few Ucn III fibers were observed in these areas,although Ucn III-positive cells were found in the MePO. It shouldbe pointed out that the MePO appeared to express relatively lowlevels of Ucn III mRNA compared with other Ucn III-expressingloci, such the rostral perifornical areas and the medial amygdala.Thus, it is possible that the peptide expression levels in theseareas are beneath the level of detectability by theantiserum.

Functional implication of Ucn III in the terminal fields

The involvement of CRF receptors and their ligands in the regulation of feeding has been extensively studied. Activation ofCRF receptors in the brain by central administration of CRF ligandssuppresses food intake (Spina et al., 1996; Cullen et al., 2001).Furthermore, injections of Ucn into the VMH significantly inhibitsfood intake (Ohata et al., 2000), suggesting that CRF-R2 in theVMH is involved in the regulation of feeding. Several studieshave shown that the expression levels of CRF-R2 mRNA in the VMHare sensitive to the energy status of the animals (Makino et al.,1998; Nishiyama et al., 1999), further supporting the importanceof CRF-R2 in the VMH in regulating energy homeostasis. The majorityof the CRF-R2 in the VMH was found in the dorsomedial part ofthe nucleus (Chalmers et al., 1995; Van Pett et al., 2000), whichcoincided with the pattern of Ucn III fibers in this nucleus observedin the present study. Thus, Ucn III is likely to be the endogenousligand in the VMH mediating the effect of CRF-R2. In additionto the VMH, Ucn III fibers were also present in areas such asthe arcuate nucleus of the hypothalamus and the posterior amygdalohippocmapalarea. These areas not only express CRF-R2 (Van Pett et al., 2000)but are also known to be involved in the regulation of food intake(King et al., 1994; Sawchenko, 1998; Coscina et al., 2000). Together,this data suggests that central Ucn III may regulate feeding byacting through CRF-R2.

It has been shown that the CRF-R2-deficient mice exhibited heightened anxiety levels (Bale et al., 2000; Coste et al., 2000;Kishimoto et al., 2000), suggesting that CRF-R2 is involved inthe modulation of anxiety. Other studies have proposed that CRF-R2in the LS might play an important role in stress-induced anxiety(Radulovic et al., 1999; Ho et al., 2001). Ucn has been consideredas a candidate endogenous ligand for CRF-R2 (Kozicz et al., 1998;Bittencourt et al., 1999) in the LS, in which Ucn terminals occupythe medial part of the LS near the medial septum. The presentstudy shows that dense Ucn III fibers were localized in the intermediateand ventral parts of the LS along the lateral ventricle. Thus,Ucn and Ucn III inputs into the LS appear to be organized to occupydifferent subdivisions of the LS. It is not clear whether thetwo ligands mediate the same effects or are involved in differentfunctions. Additional studies are needed to elucidate thisissue.

Currently, the function of CRF-R2 in the MEA has not been examined in detail. Therefore, it is difficult to predict the functionof Ucn III in this region. Anatomical and physiological studieshave shown that the MEA is involved in the regulation of neuroendocrineand autonomic nervous system functions (Docke et al., 1983; Pfeifferand Johnston, 1994; Canteras et al., 1995). In addition, the MEAhas been suggested to modulate reproduction-related behavior (Rajendrenand Moss, 1993; Dominguez et al., 2001). Therefore, Ucn III andCRF-R2 in the MEA may play an important role in mediating neuroendocrinestatus andbehaviors.

Similar to the MEA, the ventral premammillary nucleus has been viewed as part of the circuitry involved in neuroendocrineand autonomic regulation (Beltramino and Taleisnik, 1985; Canteraset al., 1992) and in mediating agonistic behavior (Van den Berget al. 1983; Yokosuka et al., 1999). However, no known CRF receptorshave been found in this area (Van Pett et al., 2000), suggestingthat either the levels of CRF receptors are very low or can onlybe detected under certain conditions. In addition, it cannot beruled out that a new splice variant of known CRF receptors ora new receptor might be present in this area for mediating theactions of UcnIII.

In conclusion, the close association of the identified Ucn III terminal fields with the expression of CRF-R2 in most of brainareas examined strongly suggests that Ucn III is an endogenousligand for CRF-R2 in these regions. These results also providean anatomical framework to facilitate an understanding of thefunction of Ucn III and CRF-R2 in thebrain.

  FOOTNOTES

Received Aug. 23, 2001; revised Oct. 24, 2001; accepted Nov. 9, 2001.

This work was supported by National Institutes of Health Program Project DK-26741, The Kleberg Foundation, The Adler Foundation,The Foundation for Medical Research, Inc., and The Foundationfor Research. W.W.V. is a FFR Senior Investigator. P.E.S. is anFMR, Inc. Senior Investigator. C.L. is supported by National ResearchService Award MH-12654. We thank J. Gulyas and J. Rivier who madethe peptides used in the study. We also thank Dr. P. Jamison andB. Henry for comments on thismanuscript.
Correspondence should be addressed to Dr. Wylie W. Vale, The Clayton Foundation for Peptide Biology Laboratories, The SalkInstitute for Biological Studies, 10010 North Torrey Pines Road,La Jolla, CA 92037. E-mail:vale{at}salk.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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