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The Journal of Neuroscience, April 1, 2001, 21(7):2413-2424
Leptin-Induced Nuclear Translocation of STAT3 Immunoreactivity in Hypothalamic Nuclei Involved in Body Weight Regulation
Thomas Hübschle1, Elke Thom1, Anna Watson1, Joachim Roth2, Susanne Klaus1, and Wolfgang Meyerhof1 1 German Institute of Human Nutrition, Departments of Biochemistry and Physiology of Nutrition and Molecular Genetics, D-14558 Potsdam-Rehbrücke, Germany, and 2 Institute of Veterinary Physiology, Justus-Liebig-University, D-35392 Giessen, Germany
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Leptin is involved in the hypothalamic control of food intake and body weight. Fos immunohistochemistry has been used to functionally map leptin target neurons involved in these regulatory processes. However, only a subset of hypothalamic neurons expressing the long form of the leptin receptor (Ob-Rb) also coexpress the neuronal activation marker Fos after leptin stimulation. To functionally map all leptin target neurons, regardless of whether leptin-mediated neuronal activation or inhibition occurs, we immunohistochemically investigated the leptin-induced nuclear translocation of the signal transducer and activator of transcription molecule STAT3, which represents a crucial step in the regulation of leptin-dependent gene expression. As proven by colocalization studies with the nuclear 4',6-diamidino-2-phenylindole dilactate stain, intracerebroventricular leptin treatment, but not intracerebroventricular application of pyrogen-free saline, induced a time-dependent nuclear translocation of STAT3 immunoreactivity in hypothalamic nuclei, with strong nuclear STAT3 signals detectable in the arcuate nucleus, the lateral hypothalamus, and the ventromedial and dorsomedial hypothalamic nuclei. This leptin-induced STAT3 translocation pattern proved to be distinct from that induced by interleukin-6, another cytokine using STAT3 in its signaling pathway. Combined immunohistochemical STAT3 and Fos detection after leptin treatment revealed a higher number of STAT3-positive than Fos-positive cell nuclei in the aforementioned hypothalamic structures and showed that Fos immunoreactivity colocalized only in a subset of all leptin-responsive STAT3 nuclei. These results suggest that the detection of nuclear STAT3 immunoreactivity represents a new neuroanatomical tool to functionally map central leptin actions. They further support the importance of ventrally located caudal hypothalamic structures representing the main leptin targets involved in body weight regulation.
Key words: hypothalamus; food intake; appetite control; leptin; interleukin-6; cytokines; transcription factors; signal transducers and activator of transcription; STAT3; c-Fos; immunohistochemistry; confocal microscopy
INTRODUCTION
Leptin is a cytokine that acts in the hypothalamus as a hormone to regulate food intake and body weight (BW) (Friedman, 1998
; Elmquist et al., 1999
To functionally map the actions of leptin on the brain, Fos immunohistochemical studies were performed, revealing Fos induction in all of the aforementioned hypothalamic structures, but with a distinct activation pattern in some of their subnuclei (van Dijk et al., 1996
We therefore hypothesized that the combination of central leptin treatment with the subsequent immunohistochemical detection of STAT3 should be a good tool to reveal direct leptin actions on the brain. Various studies examined the distribution of STAT3 immunoreactivity within the hypothalamus (Hakansson and Meister, 1998
MATERIALS AND METHODS
Animals. Adult male Wistar rats (Tierzucht Schönwalde GmbH, Schönwalde, Germany), with an initial BW ranging from 180 to 210 gm, were housed in individual cages in the animal house (Max Rubner Laboratory, Bergholz-Rehbrücke, Germany) and used in accordance with ethics authorities and local regulations (ethics approval number 48-3560-1/2). Lights were on from 6:00 A.M. to 6:00 P.M., and room temperature (RT) was adjusted to 22 ± 1°C. Animals had constant access to water and were fed standard lab chow available ad libitum. BW was monitored daily, and thereby the rats were handled at least once a day.
Intracerebroventricular cannulation of the lateral ventricle. Animals were anesthetized with intraperitoneal injections of a ketamine-xylazine solution [100 mg/kg BW Ketamin Gräub (Albrecht, Aulendorf, Germany); 10 mg/kg BW Rompun (2%; Bayer Vital, Leverkusen, Germany)]. During surgery, body temperature was kept constant at ~37°C using a self-regulating heating pad (Fine Science Tools, Heidelberg, Germany). A modified 23 gauge cannula (Braun, Melsungen, Germany) attached to a PP30 tubing (Portex, Hythe, UK) and a 1 ml syringe (Braun) was filled with pyrogen-free saline (Sigma, Deisenhofen, Germany) and inserted stereotaxically (Ultra Precise Small Animal Stereotaxic Instrument, model 963; David Kopf Instruments, Tujunga, CA) into the left lateral ventricle of the brain. With a general +0.5 mm tooth bar adjustment, the coordinates used from bregma point were 0.4 mm posterior, 1.5 mm lateral, and 4 mm ventral (brain surface). Three small screws with a diameter of 1.4 mm (M1,4 V4A; Föhr Medical Instruments, Seeheim, Germany) were secured on the skull before the screws and the inserted cannula were embedded into dental cement. Finally, the cannula was sealed at the remaining opening with a plastic blocker, and the probe was checked daily during BW measurements to ensure that it remained sealed.
Accuracy of the cannula placement was tested by performing a drink test with a 50 ng intracerebroventricular bolus application of angiotensin II (Bachem Biochemica GmbH, Heidelberg, Germany) dissolved in 5 µl of 0.9% pyrogen-free saline (Sigma). The cumulative water intake was monitored for the following 60 min. Only those animals that showed an adequate drinking response of 9.8 ± 0.6 ml (n = 35; mean ± SEM) were used for additional studies. These drink tests were conducted 7-8 d after intracerebroventricular cannulation and 3-4 d before experimental stimulation.
Intracerebroventricular cytokine stimulation. On the day of experimental stimulation, BW of the rats reached 222.5 ± 3.4 gm compared with 198.5 ± 3.6 gm on the day of surgery (n = 35; mean ± SEM); hence, the rats had recovered from the surgical procedure and were gaining weight. In vivo cytokine stimulation was conducted in conscious animals with a 25 µl Hamilton syringe attached to the intracerebroventricular cannula via PP30 tubing. The central treatments consisted of an intracerebroventricular bolus injection of either 3.5 µg of recombinant murine leptin (kindly provided by Aventis Pharma, Frankfurt, Germany) or 200 ng of species homologous rat interleukin-6 (IL-6) (kindly provided by Dr. S. Poole, National Institute for Biological Standard and Control, Potters Bar, UK) (for details, see Rees et al., 1999
Catalyzed reporter deposition amplification protocol for STAT3 detection. Initially, standard immunohistochemical procedures were used for STAT3 detection (rabbit anti-STAT3 antibody, sc-482; Santa Cruz Biotechnology, Heidelberg, Germany), resulting in a very weak and nonsatisfying STAT3 signal. As shown in a recent publication investigating STAT3 distribution in the rat CNS, amplification procedures are a helpful tool to investigate STAT3 immunoreactivity (Strömberg et al., 2000
Coronal 20-40 µm free-floating hypothalamic sections (bregma levels, 0.00 to
4.80 mm) were cut on a freezing microtome (model 1205; Jung, Heidelberg, Germany) for double- and triple-labeling experiments, and 40 µm free-floating sections of the forebrain, midbrain, and hindbrain were used for STAT3 detection alone. Sections were placed into 10% fetal calf serum and 0.3% Triton X-100 in 0.1 M phosphate buffer, pH 7.2, for 1 hr at RT. For tyramide signal amplification, sections were then transferred to the blocking reagent provided in the kit for 30 min at RT. This was followed by the primary STAT3 antibody incubation (1:12000 diluted in 0.1 M phosphate buffer, 2% fetal calf serum, and 0.1% Triton X-100) for 24-48 hr at 4°C. The tyramide amplification protocol was continued according to the kit description but using a phosphate buffer system and not the suggested borate buffer. Primary STAT3 antibody was detected with a secondary biotinylated anti-rabbit antibody (Vector BA-1000; Linaris Biologische Produkte, Wertheim-Bettingen, Germany) for 1 hr at RT (diluted 1:200 in 0.1 M phosphate buffer and 2% fetal calf serum). The additional immunohistochemical processing was performed with an avidin-biotin-horseradish peroxidase complex (Vector Elite Kit; Linaris Biologische Produkte), which was visualized by either diaminobenzidine hydrochloride (Sigma) reaction in the presence of hydrogen peroxide or fluorescein (FITC)-conjugated avidin D (Vector A-200; Linaris Biologische Produkte).
Immunohistochemical colocalization studies and nuclear 4',6-diamidino-2-phenylindole dilactate stain. In double-labeling experiments, coronal 20-40 µm free-floating hypothalamic sections already stained for STAT3 were coanalyzed using additional antibodies. A coincubation was performed with a 1:2000 mouse anti-glial fibrillary acidic protein (GFAP) antibody (MAB3402; Chemicon, Hofheim, Germany) and with a 1:200 mouse anti-adenomatous polyposis coli (APC) protein (OP80; Oncogene Research Products, Calbiochem, Bad Soden, Germany). Both antibodies are used as cytoskeletal and cytoplasmatic markers of glia cells in the CNS for either astrocytes (GFAP) or mature oligodendrocytes (APC).
STAT3 detection was also combined with the immunohistochemical analysis of the immediate early gene Fos. Fos-like immunoreactivity was detected with an anti-c-fos antibody (sc-52; Santa Cruz Biotechnology) at a 1:500-1:1000 dilution. In this experiment, both primary antisera were raised in rabbits, and therefore a consecutive detection of first STAT3 and then Fos was performed according to the method described previously by Shindler and Roth (1996)
In a final step, all sections were stained for 5 min at RT with the nuclear stain 4',6-diamidino-2-phenylindole dilactate (DAPI) (Molecular Probes Europe BV, Leiden, Netherlands), which was diluted 1:400 in phosphate buffer.
Microscopical analysis. The free-floating sections were mounted onto gelatin-coated slides and for the enzyme-histochemical detection coverslipped with Entellan (Merck, Darmstadt, Germany), whereas for fluorescent detection, slides were coverslipped with Crystal/Mount (Biomedia, Foster City, CA). The sections were analyzed using a conventional Zeiss (Jena, Germany) Axioplan light microscope and a Zeiss confocal microscope. Confocal images were taken with an inverted Zeiss Laser Scanning Microscope (model LSM 410) attached to an internal helium-neon ion laser and two external lasers, one argon ion and one argon UV laser with individual excitation outputs of 543, 488, and 364 nm, respectively. Images were individually processed for the color channel red, green, and blue (RGB) using a 570 long-pass emission filter for Cy3 detection (R), a 510-525 bandpass emission filter for FITC detection (G), and a 397 long-pass emission filter for DAPI detection (B). The images shown are the result of one optical section; the color images show individual color channels or the overlay of two of such individually taken RGB images. Image editing software (Adobe Photoshop; Adobe Systems, San Jose, CA) was used to change the graphic mode from RGB to CMYK (cyan, magenta, yellow, and black) and to combine the images into plates.
RESULTS
Intracerebroventricular leptin treatment induces a time-dependent nuclear translocation of STAT3 immunoreactivity within the hypothalamus
To investigate the basal and the leptin-induced hypothalamic STAT3 expression at the cellular level, immunohistochemical procedures were used. Basal STAT3 expression levels in the rat forebrain were evaluated in controls via intracerebroventricular pyrogen-free saline application and found to be highest in the caudal hypothalamus (Fig. 1A). In particular, ventrally located hypothalamic structures, such as the ARC (Figs. 1A, 2A), its adjacent periarcuate area (PAA), and areas ventral to the fornix in the LHA (Figs. 1A, 2G), were labeled. Weaker STAT3 immunoreactivity was observed in several other hypothalamic nuclei, such as the VMH, the DMH, the retrochiasmatic area (RCH), the PVN, the supraoptic nucleus (SON), and the medial preoptic area (MPO). By confocal microscopy and the nuclear DAPI stain, the subcellular distribution of the basal STAT3 expression was investigated. Under control conditions, STAT3 immunoreactivity was predominantly found in the cell cytoplasm and in nerve fibers (Fig. 2A-C, G-I, insets in B/C, H/I), with nuclear STAT3 labeling being rarely detectable in the aforementioned hypothalamic structures.
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Figure 1. Hypothalamic leptin targets mapped by the detection of STAT3 immunoreactivity under control conditions (A) and after intracerebroventricular leptin application (B). Immunofluorescence photomicrographs show an overview at caudal hypothalamic levels approximately
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Figure 2. Leptin induces a nuclear translocation of STAT3 immunoreactivity in hypothalamic nuclei. Immunofluorescence photomicrographs of hypothalamic sections of the ARC (A-F) and ventral aspects of the LHA (G-L) are shown under control conditions (CTRL; A-C, G-I; 30 min after pyrogen-free saline) and leptin-stimulated conditions (D-F, J-L; 30 min after leptin). STAT3 immunoreactivity in green (A, D, G, J) is compared with the blue nuclear DAPI stain (B, E, H, K). The overlays of these individual confocal images are shown in C, F, I, and L. Note that, under basal control conditions, STAT3 immunoreactivity is predominantly located within the cytoplasm and also nerve fibers of ARC and LHA neurons, whereas most of the cell nuclei seem to be devoid of STAT3 labeling (see arrowheads in A-C and G-I and also the insets in B/C and H/I showing this at higher magnification). Leptin treatment (30 min) not only led to a nuclear translocation of STAT3 immunoreactivity in both hypothalamic structures the ARC and the LHA (see arrows showing the light blue double-labeled cell nuclei in F and L and also the insets in E/F and K/L showing this at higher magnification) but also to a general increase of STAT3 labeling (compare A with D and G with J). VIII, Third ventricle; f, fornix. Scale bars, 50 µm.
The subcellular distribution and the intensity of STAT3 signals within some of these hypothalamic structures dramatically changed after the intracerebroventricular leptin administration. As shown in overview in Figure 1B, leptin treatment led to a marked increase of STAT3 immunoreactivity in the caudal hypothalamus. Although all parts of the ARC seemed to be heavily labeled, a distinct subdistribution of the STAT3 signal became obvious for the VMH or the DMH, with dorsal (VMH) and ventral (DMH) parts being the most leptin-responsive hypothalamic targets besides the ARC. Within the PAA, the RCH, and the LHA, intense but more scattered labeling of individual medium- to large-sized neurons occurred. In addition, cells within the ependymal lining of the third ventricle, the adjacent periventricular nucleus, and in ventrally located meninges showed strong STAT3 immunoreactivity. A subcellular analysis of the leptin-induced STAT3 signals revealed that a massive shift of STAT3 immunoreactivity from the cytoplasm into the cell nucleus occurred 30 min after the intracerebroventricular leptin application, as shown for example within the ARC (Fig. 2D-F, inset in E/F) or the LHA (Fig. 2J-L, inset in K/L). Such a nuclear translocation of STAT3 was observed in various hypothalamic but also extrahypothalamic forebrain structures (Table 1). Besides the induction of this intense nuclear STAT3 signal, intracerebroventricular leptin treatment additionally induced a massive increase of the STAT3 signal in nerve fibers and axons, being most prominent within the ARC (Fig. 2D,F, inset in E/F) and the ventral LHA (Fig. 2J,L, inset in K/L).
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Table 1. Forebraina distribution of leptin- and interleukin-6 (IL-6)-induced nuclear STAT3 immunoreactivityb compared with basal nuclear STAT3 expression in the control The time dependency of this nuclear STAT3 translocation is demonstrated for the ARC using a post-application period ranging from 15 to 180 min (Fig. 3). Compared with the basal STAT3 expression in the control (Fig. 3A), intracerebroventricular leptin application rapidly induced a nuclear translocation of STAT3 immunoreactivity already present at 15 min (Fig. 3B), which became even more pronounced at 30 min (Fig. 3C). When using post-application periods longer than 30 min, the high intensity of the STAT3 signal present at 30 min slowly decreased (Fig. 3D-F), with only a small number of STAT3-positive cell nuclei being left 180 min after leptin treatment (Fig. 3F).
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Figure 3. Leptin induces a time-dependent nuclear translocation of STAT3 immunoreactivity in the ARC. Immunofluorescence photomicrographs of STAT3 immunoreactivity in ARC sections are shown under control conditions (A, CTRL; 30 min pyrogen-free saline) and under leptin-stimulated conditions (B-F). Under basal control conditions, STAT3 immunoreactivity is detectable in all subnuclei of the ARC and is predominantly located in the cytoplasm and nerve fibers of ARC neurons (A). As soon as 15 min after leptin application, a massive increase in nuclear STAT3 labeling is detectable in all parts of the ARC (B), which becomes even more pronounced after 30 min (C). However, 60-180 min after leptin application (D-F), the nuclear STAT3 signal slowly starts to decrease again, which is indicated by the shift from a sharp-edged round-shaped STAT3 signal in the nucleus (B, C) to a more blurred and less defined nuclear labeling and a decrease in the intensity of STAT3 immunoreactivity (D-F). VIII, Third ventricle; ME, median eminence. Scale bar, 50 µm.
Intracerebroventricular leptin treatment shows a nuclear STAT3 translocation pattern distinct from that induced by intracerebroventricular interleukin-6 application
The specificity of the leptin-induced nuclear STAT3 translocation in distinct forebrain structures was additionally checked using IL-6, another cytokine also capable of activating the Jak-STAT3 signal transduction pathway. Indeed, for both cytokines, a specific pattern of nuclear STAT3 translocation became obvious within the rat forebrain (Fig. 4, Table 1). Whereas in controls most (extra)hypothalamic structures proved to be devoid of nuclear STAT3 labeling, both intracerebroventricular leptin and intracerebroventricular IL-6 induced a shift of the STAT3 signal into the cell nucleus (Table 1). However, the densities of nuclear STAT3 labeling and the brain sites affected were different for the two cytokines. Whereas leptin seemed to predominantly target ventral parts of the caudal hypothalamus, IL-6 additionally induced a massive STAT3 translocation in the rostral hypothalamus, in particular within the MPO and its ventromedial part, the VMPO (Fig. 4B, inset in A/B), which was not detectable in the leptin-treated animals (Fig. 4A). When looking at other forebrain structures, the two cytokine stimuli expressed a differing pattern of nuclear STAT3 translocations. This included the anterior piriform cortex (PIR), which showed a high density of nuclear STAT3-labeled layer II neurons in the intracerebroventricular leptin but not in the intracerebroventricular IL-6-treated animals (Fig. 4C,D), and also the SON (Fig. 4E,F) and some thalamic nuclei (Table 1) in which IL-6 but not leptin induced a nuclear translocation of STAT3 immunoreactivity. In the caudal hypothalamus, the overall pattern of STAT3 immunoreactivity induced by leptin or IL-6 again proved to be different (Fig. 4G,H). Whereas leptin induced nuclear STAT3 translocation in medial and lateral parts of the ARC as well as in dorsal parts of the VMH, IL-6 did not lead to STAT3 translocation in the medial ARC and only to a minor nuclear labeling in the dorsal VMH.
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Figure 4. Distinct cytokine-induced nuclear STAT3 translocation patterns in forebrain structures induced by intracerebroventricular leptin or by intracerebroventricular IL-6 treatment. Immunofluorescence photomicrographs of STAT3 immunoreactivity are shown at rostral (A-D), medial (E, F), and caudal (G, H) hypothalamic levels under leptin-stimulated (A, C, E, G) or IL-6-stimulated (B, D, F, H, inset in A/B) conditions. Only basal, predominantly non-nuclear STAT3 signals are expressed in the 30 min leptin-treated animal within lateral parts of the organum vasculosum of the lamina terminalis (OVLT) and the adjacent ventromedial preoptic area (VMPO) (A). IL-6 treatment on the other hand induced an increase and shift of STAT3 immunoreactivity into cell nuclei, particularly in the MPO, including the ventromedial preoptic area, as well as in the lateral and dorsal aspects of the organum vasculosum of the lamina terminalis (B, inset A/B). Intracerebroventricular leptin (C) but not IL-6 application (D) induced nuclear STAT3 labeling in neurons of layer II of the PIR. For orientation, note that C and D have been rotated. Within the hypothalamic SON, IL-6 (F) but not leptin treatment (E) led to nuclear STAT3 labeling. Note that the basal expression of STAT3 immunoreactivity depicted from the leptin-treated animal (E) is almost completely located within the cytoplasm of magnocellular SON neurons. In caudal hypothalamic aspects shown in overview for leptin (G) and IL-6 treatment (H), a distinct cytokine-induced pattern of nuclear STAT3 immunoreactivity could be detected in the ARC, the PAA, and the VMH. VIII, Third ventricle; oc, optic chiasm; lot, lateral olfactory tract; f, fornix; ME, median eminence. Scale bars: A-D, G, H, 100 µm; E, F, inset in A/B, 50 µm.
Leptin-induced nuclear STAT3 immunoreactivity within the piriform cortex and the hypothalamus does not colocalize with glial cell markers
For the light microscopic analysis, the enzyme immunohistochemical STAT3 detection was combined with cresyl violet counterstaining, indicating a predominant neuronal location of the STAT3 immunoreactivity under both basal and leptin-stimulated conditions within the hypothalamus (data not shown). However, non-neuronal, nuclear STAT3 labeling was also detected, e.g., in ependymal and meningeal cells, and also near to the probe site in small, noncircular-shaped cell nuclei, which presumably belonged to glial cells (Table 1). Former electron microscopic investigations have shown that, within the brain tissue, leptin receptors are located on both neurons and glia. It was therefore of importance to analyze the cell types in which intracerebroventricular administration of leptin induced nuclear translocation of STAT3. To demonstrate the cellular origin of the STAT3 signals, double-labeling experiments combining the STAT3 detection with the immunohistochemical localization of the cytoskeletal and cytoplasmatic glial cell markers GFAP (Fig. 5A-E) and APC (Fig. 5F) were performed after intracerebroventricular leptin application. The size and shape of the STAT3-stained nuclei within most cells of the PIR (Fig. 5A) and the hypothalamus (Fig. 5B-F) again indicated a predominant neuronal cell origin. Indeed, no cellular colocalization of the nuclear STAT3 signal was found within the astrocytes in layer II of the anterior PIR (Fig. 5A) or within the astrocytes in the main hypothalamic leptin targets, such as the ARC (Fig. 5B), the LHA (Fig. 5C), and the DMH and VMH (Fig. 5D,E). In addition, leptin-induced nuclear STAT3 signals within the VMH did not colocalize with the cytoplasmatic labeling of oligodendrocytes (Fig. 5F). Within the most intense nuclear STAT3-labeled hypothalamic regions, in no single case did a colocalization occur, suggesting that glia cells in these areas may express a leptin receptor isoform that is not capable to activate the full cytokine specific Jak-STAT pathway.
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Figure 5. Leptin-translocated nuclear STAT3 immunoreactivity does not colocalize with the glial cell markers GFAP (A-E) and APC (F) in forebrain structures. Immunofluorescence photomicrographs of leptin responsive-forebrain structures, such as the PIR (layer II, A), the ARC (B), ventral aspects of the LHA (C), the DMH (D), and the VMH (E, F) are shown 30 min after intracerebroventricular leptin stimulation. Nuclear STAT3 immunoreactivity (green) is compared with the cellular location of glial cells (red). Note that the STAT3-labeled nuclei do not colocalize with the cytoplasm or cytoskeletal structures of labeled astrocytes or oligodendrocytes, thereby indicating that within these forebrain structures the leptin-induced nuclear STAT3-translocation has occurred in neurons. f, Fornix. Scale bars: A, C, D, 25 µm; B, E, F, 10 µm.
Nuclear STAT3 and Fos immunoreactivity colocalizes only in a subset of leptin-responsive forebrain neurons
In double-labeling experiments, the leptin-induced nuclear STAT3 immunoreactivity within the forebrain was compared with the Fos response 60 min after intracerebroventricular leptin application. The time point used in these experiments was chosen as a compromise between the time necessary for nuclear translocation of STAT3 (15-30 min) (Fig. 3) and the time known to show the first peak of the nuclear Fos signal (90 min) in neurons. A clear difference between the number of STAT3-stained (green nuclei) versus Fos-stained (red nuclei) nuclei could be detected, with more STAT3-stained than Fos-stained nuclei after central leptin treatment (Fig. 6A-G,I,J). Individual detection of STAT3 and Fos immunoreactivity (Fig. 6A-D) showed a similar distribution of nuclear signals in layer II of the PIR (Fig. 6A,B) but distribution differences within the caudal hypothalamus. STAT3 was predominantly induced in medial parts of the ARC and dorsal aspects of the VMH (Fig. 6C), whereas nuclear Fos was mainly detectable in the ventrolateral ARC and the adjacent periarcuate area (Fig. 6D). At higher magnification, nuclear STAT3 and Fos immunoreactivity proved to be colocalized (yellow nuclei) only in a subset of neurons of the anterior PIR (Fig. 6E), the ventrolateral ARC (Fig. 6F), and ventral parts of the DMH (Fig. 6I). Minor colocalization of the two nuclear signals was detected within the LHA (Fig. 6G) and the dorsal part of the VMH (Fig. 6J).
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Figure 6. Leptin-translocated nuclear STAT3 and Fos immunoreactivity colocalizes only in a subset of leptin-responsive forebrain neurons. Immunofluorescence photomicrographs of leptin-responsive forebrain structures, such as the PIR (A, B, E), the ARC (C, D, F), ventral aspects of the LHA (G), the DMH (I), and the VMH (C, D, J), are shown 60 min after intracerebroventricular leptin stimulation. The brain map (H) indicates the position of the photomicrographs shown in I and J. Nuclear STAT3 immunoreactivity (green) is compared with the nuclear localization of the protein product of the immediate early gene c-fos (red). Although within layer II of the PIR many STAT3-labeled (A) and Fos-labeled (B) nuclei could be detected, the overlay (E) at higher magnification (the exact location indicated by the white rectangles in A and B) clearly showed that only a small subset of layer II neurons coexpressed both transcription factors (yellow nuclei), whereas the majority responded with a nuclear translocation of STAT3 only (green nuclei). Red nuclei belong to those layer II neurons that responded with a nuclear translocation of Fos but not STAT3. Similar results, but with varying degrees of STAT3 and Fos colocalization, were also obtained in the hypothalamic leptin target structures, such as the ventrolateral ARC (C, D, F), the LHA (G), the ventral DMH (I), and the dorsal VMH (J). VIII, Third ventricle; lot, lateral olfactory tract; f, fornix. Scale bars: A-D, 100 µm; E-G, I, J, 25 µm.
DISCUSSION
The ventrobasal hypothalamus has been described as the primary central leptin target involved in the control of food intake and energy balance. Many physiological responses regulated by leptin, such as the inhibition of appetite via intracerebroventricular leptin treatment in rats, characteristically start with some delay and show long-lasting effects (Cusin et al., 1996
The leptin-induced nuclear STAT3 pattern matches with Ob-Rb receptor expression in the ventrobasal hypothalamus
One open question in the past was whether the extensive distribution of the Ob-Rb receptor within the rodent hypothalamus, detected via in situ hybridization techniques (Mercer et al., 1996
The present data also neuroanatomically confirm the finding of Vaisse et al. (1996)
The leptin-induced nuclear STAT3 pattern is distinct from that induced by interleukin-6
The specificity of the leptin-induced STAT3 translocation was verified with intracerebroventricular treatment of the endogenous pyrogen IL-6. Central IL-6 administration elicits a variety of (patho)physiological functions, such as the reduction of food intake and locomotor activity, the activation of the hypothalamic-pituitary-adrenocortical axis, and the mediation of fever responses (Lenczowski et al., 1999
STAT3 immunohistochemistry: a novel tool to map neurons responding to leptin
Leptin binding to the Ob-Rb receptor leads to nuclear translocation of the activated STAT3 isoform and finally induces transcriptional activation of genes (Ihle, 1996
Recent electrophysiological data have clearly demonstrated an inhibitory leptin action on the neuronal discharge rate of orexin-sensitive ARC neurons, suggesting that neuronal inhibition and not activation is the predominant mode of leptin action in this nucleus. Although in many cases a leptin-induced direct inhibition of neuronal activity in the ARC occurred, some direct activation of neuronal activity also existed (Rauch et al., 2000
FOOTNOTES Received Sept. 11, 2000; revised Dec. 14, 2000; accepted Dec. 22, 2000.
This work was supported in part by European Commission Grant QLG3-CT-1999-00908 to W.M. We thank Dr. E. Simon for critical reading of this manuscript.
Correspondence should be addressed to Dr. Thomas Hübschle, Institute of Veterinary Physiology, Justus-Liebig-University, Frankfurter Straße 100, D-35392 Giessen, Germany. E-mail: thomas.huebschle{at}vetmed.uni-giessen.de.
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