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Previous Article | Next Article
The Journal of Neuroscience, December 1, 1999, 19(23):10417-10427
Brain Uncoupling Protein 2: Uncoupled Neuronal Mitochondria Predict Thermal Synapses in Homeostatic Centers
Tamas L. Horvath1, 2, Craig H. Warden3, Mihaly Hajos4, Assunta Lombardi5, Fernando Goglia5, and Sabrina Diano1 1 Department of Obstetrics and Gynecology, and 2 Section of Neurobiology, Yale University School of Medicine, New Haven, Connecticut 06520, 3 Rowe Program in Human Genetics, Department of Pediatrics and Section of Neurobiology, Physiology, and Behavior, School of Medicine, University of California at Davis, Davis, California 95616, 4 Department of Clinical Pharmacology, University of Oxford, Oxford, United Kingdom OX2 6HE, and 5 Dipartimento di Fisiologia Generale ed Ambientale, Universita' degli Studi di Napoli "Federico II," Napoli, Italy 80134
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Distinct brain peptidergic circuits govern peripheral energy homeostasis and related behavior. Here we report that mitochondrial uncoupling protein 2 (UCP2) is expressed discretely in neurons involved in homeostatic regulation. UCP2 protein was associated with the mitochondria of neurons, predominantly in axons and axon terminals. UCP2-producing neurons were found to be the targets of peripheral hormones, including leptin and gonadal steroids, and the presence of UCP2 protein in axonal processes predicted increased local brain mitochondrial uncoupling activity and heat production. In the hypothalamus, perikarya producing corticotropin-releasing factor, vasopressin, oxytocin, and neuropeptide Y also expressed UCP2. Furthermore, axon terminals containing UCP2 innervated diverse hypothalamic neuronal populations. These cells included those producing orexin, melanin-concentrating hormone, and luteinizing hormone-releasing hormone. When c-fos-expressing cells were analyzed in the basal brain after either fasting or cold exposure, it was found that all activated neurons received a robust UCP2 input on their perikarya and proximal dendrites. Thus, our data suggest the novel concept that heat produced by axonal UCP2 modulates neurotransmission in homeostatic centers, thereby coordinating the activity of those brain circuits that regulate daily energy balance and related autonomic and endocrine processes.
Key words: uncoupling proteins; brain; neurons; axon terminals; cranial temperature; proton leak; autonomic and endocrine regulation
INTRODUCTION
The accumulation of body fat is influenced by both central and peripheral processes. CNS signals regulate feeding behavior and energy expenditure of peripheral tissues, whereas brain mechanisms that govern metabolic, autonomic, and endocrine systems are, in turn, influenced by peripheral signals, including leptin, insulin, glucose, glucocorticoids, gonadal steroids, and thyroid hormones (Campfield et al., 1995
; Halaas et al., 1995
In the attempt to elucidate ways to enhance energy expenditure to diminish fat stores, increasing attention is being paid to energy-dissipating processes and their regulatory components (Boss et al., 1998
The present study was undertaken to investigate UCP2 in the brain to determine whether this uncoupling protein is present in neurons and, if so, to reveal which neuronal circuits operate with this heat-producing mitochondrial device.
MATERIALS AND METHODS
Animals. A total of 40 adult female and male Sprague Dawley rats (200-250 gm) were used in this study. For the mRNA and protein analyses, 15 animals were kept under standard laboratory conditions, with tap water and regular rat chow available ad libitum; lights were maintained on a 12 hr light/dark cycle. Groups of males (n = 5) were killed after either 24 hr of fasting or 16 hr of cold exposure (at 4°C with food and water available ad libitum). All of these rats were killed under ether anesthesia by transaortic perfusion with 50 ml of heparinized saline followed by 250 ml of fixative. The fixative consisted of 4% paraformaldehyde, 15% saturated picric acid, and 0.08% glutaraldehyde in 0.1% sodium phosphate buffer (PB), pH 7.4. Brains were dissected, and 3-mm-thick coronal blocks were post-fixed for an additional 1-2 hr. Thirty- or 50-µm-thick sections were cut on a vibratome. Sections were rinsed in 1% sodium borohydride in PB for 15 min to eliminate unbound aldehydes. For the mitochondrial uncoupling and cranial temperature measurements, 10 and 5 male rats were used, respectively (see details below).
The use of animals was approved by the respective University Committees on Animal Use at Yale University, University of Oxford, and University of Naples.
RT-PCR. A fragment of 404 bp of cDNA of UCP2 was amplified based on the RT-PCR using specific oligonucleotide primers derived from the coding region of the rat UCP2 sequence (5'-GTC GAA TTC TAC AAG ACC ATT GCA CGA-3' and 5'-TGG GAT CCT CAT AGG TGA CAA ACA TTA-3'). As control, a 603 bp cDNA of rat
-actin was amplified using the following primers: 5' TAC AAC CTC CTT GCA GCT CC 3' and 5' GGA TCT TCA TGA GGT AGT CAG TC 3'. Total RNA was extracted from the hypothalamus by the guanidium thiocyanate-phenol-chloroform method using trizol reagent (Life Technologies, Grand Island, NY) and transcribed using First-Strand cDNA synthesis kit (Pharmacia, Piscataway, NJ). The PCR reaction was performed using the following protocol: 3 µg of cDNA templates reacted with 500 nM primers, 1.25 mM MgCl2, 80 µM dNTP, and 2 U Taq DNA polymerase. Thermal profiles were 94°C for 1 min, 60°C for 1 min, and 72°C for 1 min for 30 cycles with a final 10 min extension period.
Northern blot analysis. Ten micrograms of total RNA was electrophoresed on 1.2% agarose/formaldehyde gels, transferred onto Hybond-N nylon membranes (Amersham, Arlington Heights, IL) by capillary blotting with 10× SSC, and covalently cross-linked to the membranes using a UV cross-linker (Stratagene, La Jolla, CA). Membranes were prehybridized for 3 hr at 42°C in a solution containing 50% formamide, 5× SSC, 5× Denhardt's solution, 1% SDS, and 100 µg of denatured salmon sperm DNA. Hybridization was performed overnight at 42°C in the hybridization solution containing 2 × 106 cpm/ml of 32P-labeled UCP2 probe. After hybridization, membranes were washed in 2× SSC/0.1% SDS, followed by two washes in 0.2× SSC/0.1% SDS at 55°C. Membranes were then exposed to x-ray film for 48 hr at
80°C. For internal control, membranes were stripped in 0.1× SSC and 0.5% SDS at 95°C and then reprobed with 32P-labeled
-32P]dCTP (10 mCi/ml; Amersham) using a random oligonucleotide primer (Amersham).
In situ hybridization. The PCR product was inserted in Bluescript vector and subcloned. Linearized DNA was transcribed using T7 polymerase (antisense cRNA probe) and T3 polymerase (sense cRNA probe; Riboprobe Combination System T3/T7; Promega, Madison, WI). The radiolabeled cRNA probe was purified by passing the transcription reaction solution over a G50 column (Pharmacia Biotech), and fractions were collected and counted by using a scintillation counter. In situ hybridization: the purified cRNA probes were heated at 80°C for 2 min with 500 mg/ml yeast tRNA and 50 mM dithiothreitol (DTT) in water before being diluted to an activity of 5.0 × 107 dpm/ml with hybridization buffer containing 50% formamide, 0.25 M sodium chloride, 1× Denhardt's solution, and 10% dextran sulfate. The brains (n = 5) were perfused and frozen on dry ice. The frozen brains were allowed to equilibrate in a cryostat at
Western blot analysis. Rats were killed by decapitation under ether anesthesia. The hypothalamus of each animal was removed and homogenized in lysis buffer containing 50 mM Tris-HCl, pH 7.5, 50 mM MgCl2, 5 mM EGTA, 0.25% Triton X-100, and protease inhibitors (proteinase inhibitor cocktail tablets; Boehringer Mannheim, Indianapolis, IN). Coomassie-stained SDS-polyacrylamide gels were routinely used to evaluate the quality of the extracts. Western blots were performed using 10% SDS-polyacrylamide gels run on a minigel apparatus; 25 µg of protein was loaded per lane. The gels were transferred to polyvinylidene fluoride (PDVF; Millipore, Bedford, MA) membranes by electroblotting overnight (30 V). The filters were blocked in 6% nonfat dry milk and 0.1% Tween 20 for 1 hr at room temperature. Blots were then incubated with rabbit anti-UCP2 (1:2000) diluted in TBS Tween 20 (TTBS; 20 mM Tris, 137 mM NaCl, pH 7.6) for 1 hr at room temperature. Blots were also incubated with rabbit anti-actin (1:10,000) (Sigma, St. Louis, MO) as controls to evaluate the amount of proteins loaded for each lane. Membranes were washed three times for 10 min in the same buffer and incubated for 1 hr with horseradish peroxidase-conjugated goat anti-rabbit IgG (Vector Laboratories, Burlingame, CA) diluted 1:10,000 in TTBS. Subsequently, the blots were washed five times for 10 min in the same buffer. Immunoreactive proteins were revealed using enhanced chemiluminescence method (ECL; Amersham).
Light and electron microscopic immunocytochemistry. Sections were incubated with the primary antisera [rabbit anti-UCP2 (1:2000)] for 24 hr at room temperature. After several washes with PB, sections were incubated in the secondary antibody (biotinylated goat anti-rabbit IgG; 1:250 in PB; Vector Laboratories) for 2 hr at room temperature, then rinsed in PB three times 10 min each time, and incubated for 2 hr at room temperature with avidin-biotin-peroxidase (ABC; 1:250 in PB; ABC Elite kit, Vector Laboratories). The immunoreaction was visualized with a modified version of the nickel-diaminobenzidine (Ni-DAB) reaction (15 mg of DAB, 0.12 mg of glucose oxidase, 12 mg of ammonium chloride, 600 µl of 0.05 M nickel ammonium sulfate, and 600 µl of 10%
Multiple labeling immunohistochemistry for UCP2 and different neuropeptides and hormone receptors was performed according to previously published protocols (Horvath, 1997
Under approved institutional animal protocols, rats (n = 5) were food-deprived for 24 hr before killing. Control animals received food ad libitum. Groups of male rats (n = 5) were also exposed to 16 hr of cold (4°C) during which time food and water was available ad libitum. Brains were perfusion-fixed, and sections of the hypothalami and forebrain were immunolabeled for either c-fos alone or UCP2 and c-fos (sheep anti-c-fos, 1:2000; Cambridge Research Biochemicals, Wilmington, DE) using the protocol described above. Sections from experimental and control groups were identified by placing marks on them and were processed in the same vials using the same reagents and timetable. The number of c-fos-expressing cells was calculated for each region. After determination of homogeneity within treatment groups using an F test, values were compared between experimental and control groups using Student's t tests.
Brain mitochondria preparation and measurements of oxygen consumption and membrane potential. In male rats (n = 40), mitochondria were isolated from the UCP2-containing basal hypothalamus and from the striatum and lateral thalamus (where both UCP2 mRNA and peptide were absent) according to previously published protocols (Lombardi et al., 1998
Intracranial temperature measurements. Brain temperature measurements were performed in chloral hydrate (450 mg/kg, i.p.)-anesthetized rats (n = 5) using a Digitron thermometer. Animals were placed in a stereotaxic apparatus (Kopf Instruments) and, after craniotomy, a precalibrated thermocouple (diameter, 0.6 mm; resolution, 0.1°C) was lowered into discrete regions of the thalamus and hypothalamus, in the midline, 2.8 mm posterior to bregma. Temperature readings were taken in the mediodorsal thalamus (ventral coordinate, 5.4 mm), central medial thalamus (ventral coordinate, 6.4 mm), dorsal hypothalamus (ventral coordinate, 7.4 mm), medial hypothalamus (ventral coordinate, 8.4 mm), and basal hypothalamus (ventral coordinate, 9.4 mm). Temperatures were also recorded 1 mm lateral to the midline (2.3 mm posterior to bregma) in the laterodorsal thalamus (ventral coordinate, 5 mm) and lateral hypothalamus (ventral coordinate, 8.4 mm). Temperature measurements were taken at 1 min intervals, three times in each region. The same dorsoventral temperature gradients were observed independent of whether readings were made during lowering or raising the probe. Brain sites at various anteroposterior and mediolateral locations were chosen randomly. Core body temperature was also monitored and kept constant at 36°C (Harvard Instruments). At the end of each experiment, the brain was subjected to routine histological examination to verify the positions of the probes.
RESULTS
UCP2 mRNA in the brain
Our goal was to examine UCP2 in the CNS. We first confirmed the presence of UCP2 mRNA in hypothalamic tissue fragments of rats (Fig. 1A; 4-6). In situ hybridization with a UCP2-specific, 35S-labeled riboprobe was then used to demonstrate that UCP2 mRNA is present in distinct hypothalamic nuclei. Labeled cells were localized in the hypothalamic paraventricular, supraoptic, suprachiasmatic, and arcuate nuclei (Fig. 1C-E).
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Figure 1. UCP2 mRNA and peptide expression in the brain. A, RT-PCR (top row) and Northern blot analyses of rat hypothalamic tissue demonstrates the expression of UCP2 mRNA. B, Western blot analysis of rat hypothalamic tissue revealed the expression of UCP2 peptide. Two major bands (arrows) were visible using the affinity-purified antisera: a band at 33 kDa that corresponds to the predicted molecular weight of UCP2 and another strong band at 23 kDa was also detected. C-E, In situ hybridization of UCP2 mRNA shows the concentration of labeled cells in four nuclei of the hypothalamus: the paraventricular (PVN), supraoptic (SON), suprachiasmatic (SCN), and arcuate nuclei (ARC). F-I, Although immunolabeling for UCP2 in the rat hypothalamus resulted in perikarya labeling of cells in the nuclei that contained UCP2 mRNA (SON, PVN, SCN, ARC), labeled cellular processes were abundant throughout the hypothalamus. For example, the median eminence (ME) that contains axonal fibers en route to the portal capillaries and the posterior lobe of the pituitary abundantly expressed UCP2. K, Schematic illustration (based on the rat brain atlas of Paxinos and Watson, 1997
UCP2 protein in the brain
We determined the localization of UCP2 protein in brain using an affinity-purified antiserum against human UCP2 that has been shown to react with UCP2 in skeletal muscle (Simoneau et al., 1998
In spite of the fact that antibodies to UCP2 have a slight cross reactivity with UCP3, the UCP2 antibody can be used for immunohistochemistry in the brain because there is no UCP1 or UCP3 present. The overall distribution of UCP2-immunoreactive cell bodies agrees with the in situ hybridization results: the most impressive perikaryal labeling was in the supraoptic, paraventricular, suprachiasmatic, and arcuate nuclei of the hypothalamus (Fig. 1F-I). UCP2-containing axons were present in divergent hypothalamic and limbic sites corresponding to the projection fields of the regions where UCP2 mRNA and peptide were detected in neuronal cell bodies. These areas included the lateral septum, medial septum-diagonal band of Broca region, bed nucleus of the stria terminalis, organum vasculosum of the laminae terminalis, anteroventral periventricular area, medial preoptic area, periventricular regions, anterior hypothalamus, suprachiasmatic nucleus, retrochiasmatic area, supraoptic, paraventricular, arcuate, ventromedial, dorsomedial nuclei, lateral hypothalamus, external and internal layers of the median eminence, central and medial nucleus of the amygdala, and mediodorsal and paraventricular nuclei of the thalamus (Figs. 1K, 2). Immunoreactive profiles were also present in different brainstem nuclei (data not shown), including the parabrachial nucleus, area postrema, nucleus of the solitary tract, the spinotrigeminal tract, and to a lesser extent, the raphe, locus coeruleus, and dorsal motor root ganglion of the vagus. Immunolabeling for UCP2 was negligible in cortical regions, the hippocampal formation, and thalamic relay nuclei of ascending and descending cortical pathways (Fig. 1K).
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Figure 2. UCP2 in extrahypothalamic limbic sites. A1-C2, Light micrographs reveal the expression of UCP2 immunoreactivity in extrahypothalamic limbic sites. These areas included the bed nucleus of the stria terminalis (BNST; A1, A2), the central nucleus of the amygdala (CeA; B1, B2), and the thalamic paraventricular nucleus (tPV; C1, C2). The higher power magnifications (A2, B2, C2) demonstrate the robust expression of UCP2 in neuronal processes in each of these areas. Scale bars: A1, 100 µm; A2, 25 µm.
Electron microscopy revealed that UCP2 immunolabeling was associated with the mitochondria and adjacent cytosol of neurons in all regions studied (Figs. 3, 4, 5C). Remarkably, although UCP2-containing mitochondria were detectable in all compartments of neurons, the vast majority of immunolabeled profiles were axons and axon terminals (Figs. 4, 5C). However, the synaptic vesicles seemed to be devoid of labeling (Figs. 4, 5C). UCP2-immunoreactive axon terminals established basket-like structures around the perikarya of postsynaptic neurons in different hypothalamic, limbic, and brainstem sites (Fig. 5A,B). Synapses between UCP2-containing axons and their postsynaptic targets were symmetrical (Figs. 4D, 5C).
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Figure 3. UCP2 in perikaryal mitochondria. Light (A) and electron (B) micrographs demonstrate UCP2 immunolabeling of perikaryal mitochondria (arrows) in the rat SCN. Immunoperoxidase is also associated with cytosol in close apposition to labeled mitochondria. Note the infolded nucleus of this SCN neuron. Scale bars: A, 10 µm; B, 1 µm.
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Figure 4. UCP2 in axonal mitochondria of the hypothalamus. A-G, Electron micrographs reveal the association of the UCP2 immunolabeling with mitochondria of different hypothalamic axons (arrows). Arrowheads in D point to a symmetrical synapse established by a UCP2-immunoreactive axon terminal in the arcuate nucleus. In F, note the abundance of UCP2-labeled mitochondria in an axon of the internal layer of the median eminence, which is the neuronal link between the magnocellular, paraventricular, and supraoptic nuclei and the posterior lobe of the pituitary. G, A large axon terminal containing UCP2-labeled mitochondria (arrows) in the external layer of the median eminence is in direct apposition to a portal capillary (cap), which provides the humoral link between the hypothalamus and the anterior pituitary. Asterisks indicate mitochondria with no UCP2 immunolabeling. Note that synaptic vesicles seem to be devoid of UCP2 labeling. Scale bar, 1 µm.
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Figure 5. Brain UCP2 in axons predicts increased mitochondrial proton leak and heat production. Light (A, B) and electron (C) micrographs demonstrate the abundant expression of UCP2 in presynaptic axon terminals. Arrows on the light micrographs of A and B point to UCP2-containing presynaptic terminals in the central amygdaloid nucleus that establish symmetrical synapses (C, arrowheads) on the postsynaptic target. D, The measurement of mitochondrial respiration in brain regions (left panel) where UCP2 is present (hypothalamus) and where no UCP2 was detected (thalamus/striatum) showed a lower mitochondrial phosphorylation level (lower RCR) in the hypothalamus that was caused exclusively by an increased proton leak of mitochondria in UCP2-containing regions. E, In agreement with this increased mitochondrial uncoupling activity, brain temperature in the UCP2-expressing hypothalamus was significantly higher than that of the thalamus (right panel) and the core body temperature. F, The presence of UCP2 in axon terminals together with the significant, positive correlation between UCP2 and mitochondrial uncoupling and local brain temperature suggests that heat produced presynaptically by UCP2 may have a direct influence on axonal temperature leading to the modulation of presynaptic and postsynaptic events.
Proton leak of brain mitochondria
If UCP2 in the above-described neuronal circuits is a functional uncoupler in a manner similar to what was found in a yeast model (Fleury et al., 1997
Cranial temperature measurements
The presence of decreased mitochondrial energy coupling efficiency (increased proton leak) in UCP2-containing brain regions supports the hypothesis that a thermogenic mechanism is intrinsic to distinct neuronal pathways. To test this further, brain tissue temperature in the face of steady core body temperature was determined at several dorsoventral and mediolateral locations in the brains of anesthetized rats (Fig. 5E). Cortical temperature never reached 35°C. Just lateral to the midline, temperatures of the dorsal thalamus and the central thalamus were 36.1 ± 0.09°C and 36.3 ± 0.12°C, respectively. The more ventrally located hypothalamic nuclei displayed significantly higher temperatures (37.1 ± 0.09°C; p < 0.01). However, there was only a small temperature gradient within the hypothalamus along a 2 mm dorsoventral extent. The significant increase in diencephalic temperature coincided with the appearance of UCP2 immunoreactivity in the dorsal hypothalamus (Fig. 5E). A dorsoventral temperature gradient was also found further lateral to the midline. Temperatures of the laterodorsal thalamus and the lateral hypothalamus were 36.3 ± 0.10°C and 36.9 ± 0.05°C, respectively. These temperatures were recorded at 36.0°C rectal (core) temperature. There was no change in rectal temperature during the intracranial measurements. Comparison of cranial temperature values from different sites in the brain versus the core body temperature revealed significant differences between the hypothalamic values and the core body temperature (Fig. 5E).
UCP2 in neuronal circuits involved in homeostatic regulation
We explored the relationship between UCP2 and different brain receptors for peripheral hormones, hypothalamic peptidergic systems involved in autonomic metabolic and endocrine regulation, and neuronal pathways that are activated by fasting or cold exposure by multiple-label immunocytochemical experiments (Figs. 6, 7).
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Figure 6. UCP2 in hypothalamic peptidergic circuits. Fluorescence double labeling using heterologous antisera revealed UCP2 immunoreactivity (left panels, green fluorescence) in paraventricular neurons producing CRF (top right panel, red fluorescence; arrows point to the double-immunolabeled cells in A1 and A2), in CRF-containing axon terminals in the external layer of the median eminence (B1, B2), in NPY-containing arcuate nucleus neurons (C1, C2), and in VP-expressing cells of the supraoptic nucleus (D1, D2).
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Figure 7. Relationship between UCP2 and neuronal circuits involved in endocrine and metabolic regulation. A1-A3, Green fluorescent UCP2-immunoreactive axon terminals (A1, red arrowheads) in close proximity to an arcuate nucleus neuron expressing immunoreactivity for receptor of the peripheral metabolic hormone leptin (ObR; A2). The image of A3 was taken using filters sensitive for both red and green fluorescence. B1-B3 , Green fluorescent, UCP2-immunoreactive perikaryonin the arcuate nucleus containing labeling for the peripheral sex hormone estradiol (ER; red fluorescence). C1-C3 , Green fluorescent UCP2-immunoreactive axon terminals (red arrowheads) in close proximity to a perikaryon of the dorsomedial hypothalamic nucleus (DMN) that was activated by fasting (red fluorescent, nuclear c-fos labeling). Fasting-induced c-fos expression was also detected in the lateral hypothalamus-perifornical region, arcuate nucleus, medial preoptic area, central amygdaloid nucleus, and the paraventricular thalamic nucleus. D1-D4 , Green fluorescent UCP2-producing parvicellular neurons of the paraventricular nucleus (PVN; D1, arrows) are neuroendocrine as revealed by retrograde tracing from the periphery using fluorogold (D2 , FG; FG labeling vas visualized using transillumination with ultraviolet light). The UCP2-expressing neuroendocrine cell located to the right (D3, D4, green arrows) also contains leptin receptors (ObR; D3 , red fluorescence). E, Red fluorescent, UCP2-containing axon terminals (red arrows) in close proximity to a neuronal perikaryon (green arrowhead) in the lateral hypothalamus (LH) that expresses the appetite-inducing peptide orexin. F, Red fluorescent, UCP2-containing axon terminals (red arrows) in close proximity to a hypophyseotropic neuron that produce luteinizing hormone-releasing hormone (LHRH) in the medial preoptic region (MPO). G, Green fluorescent UCP2-immunoreactive axon terminals (red arrowheads) in close proximity to a perikaryon of MPO that was activated by cold exposure (red fluorescent, nuclear c-fos labeling). Other cold-activated neurons were distributed in the paraventricular nucleus, medial preoptic area, bed nucleus of the stria terminalis, central amygdaloid nucleus, and the paraventricular thalamic nucleus.
In the rat, bright-field and fluorescent microscopy revealed that UCP2 is coexpressed with CRF in neurons of the parvicellular region of the paraventricular nucleus, with VP and, to a lesser extent, OX in neurons of the supraoptic nucleus, and with NPY in neurons of the arcuate nucleus (Fig. 6). These systems are known to regulate behavioral and hormonal aspects of metabolism, are present in the hypothalamus and brainstem, but do not send extended projections to higher brain regions. No UCP2 immunolabeling was present in lateral hypothalamic melanin-concentrating hormone (MCH) or hypocretin/orexin (HCRT)-containing cells that are important regulators of feeding behavior and are known to send projections to the cerebral cortex and the hippocampus (Qu et al., 1996
After analysis of those hypothalamic pathways that were activated either by fasting or cold exposure, neurons containing c-fos induced by either of these manipulations were massively innervated by UCP2-containing axon terminals (Fig. 7C1-C3). In fasted rats, c-fos expression was detected in the lateral hypothalamus-perifornical region, arcuate nucleus, dorsomedial nucleus, paraventricular nuclei, medial preoptic area, central amygdaloid nucleus, and the paraventricular thalamic nucleus. While fasting-induced changes in the number of c-fos-expressing cells differed in the different subnuclei (data not shown), all of the (100%) 3654 c-fos-expressing cells counted in the basal brain of five fasted rats received multiple inputs expressing UCP2 (Fig. 7C1-C3). In cold-exposed rats, c-fos-expressing cells were distributed in the paraventricular nucleus, medial preoptic area, bed nucleus of the stria terminalis, central amygdaloid nucleus, and the paraventricular thalamic nucleus. Similar to what was found after fasting, all (100%) of the cold-activated, c-fos-expressing cells (1765) were contacted by numerous UCP2-containing axon terminals (Fig. 7G).
DISCUSSION
UCP2 in brain thermogenesis
Temperature differences in various brain regions have been observed in rodents and more recently in humans, by invasive and noninvasive techniques (Mellergard and Nordstrom, 1990
UCP2 in thermoregulation
In a recent study, Richard et al. (1998)
UCP2 affecting neuronal activity
Taking into account that the majority of UCP2 was localized to axons and axon terminals, the novel concept is proposed that in distinct brain circuits, synapses may exist in which heat is produced to modulate neurotransmission (Fig. 5F). It may seem surprising that a mechanism directly related to heat production in peripheral tissues under the apparent control of the thermogenic coactivator PGC-1 (Wu et al., 1999
The present study showed that brain sites other than those containing UCP2, such as the striatum and thalamus, also show significant mitochondrial proton leak. Temperature elevations in association with increased neuronal activity were also observed in the hippocampus and cerebral cortex (Andersen and Moser, 1995
UCP2 in homeostatic centers
Even though other neuronal and glial uncouplers may be discovered, the intriguing feature of brain UCP2 expression is that, unlike BMCP1 and UCP4, UCP2 was present predominantly in neuronal populations of subcortical regions that are involved in the central regulation of autonomic, endocrine, and metabolic processes. In agreement with the known projection fields of the paraventricular, supraoptic, suprachiasmatic, and arcuate nuclei where UCP2-producing perikarya were located, there was very minimal UCP2 in axonal processes of the cerebral cortex and hippocampus. This observation suggests that the selective regulation of UCP2 may influence homeostatic regulation without directly affecting higher brain functions. The assertion that the UCP2 input of neurons in the CNS is of significance can be inferred from the fact that UCP2 boutons predominantly established basket-like structures around neuronal perikarya. Because it is on the perikaryon where axon terminals can affect the postsynaptic target with the most efficacy, the UCP2 network, when activated, could readily modulate and coordinate the activity of central homeostatic circuits.
The robust expression of UCP2 in neuronal processes of the hypothalamo-neurohypophyseal and adenohypophyseal systems suggests that a mitochondrial thermogenic mechanism participates in the regulation of vasopressin and oxytocin release in the posterior pituitary and the secretion of CRF into the portal vessels in the external layer of the median eminence. Thus, in future experiments in which selective regulation of UCP2 will be achieved, the role of UCP2 in water homeostasis, lactation, and the activity of the hypothalamo-pituitary-adrenal axis will be able to be determined.
The abundant coexpression of UCP2 and NPY in the arcuate nucleus indicates that acute activation of UCP2 by peripheral signals could readily affect the activity of this key hypothalamic peptidergic system that was shown to be crucial for feeding behavior and endocrine regulation (for review, see Kalra and Horvath 1998
While it is known that there are hypothalamic peptidergic circuits, such as the opiate, NPY, and orexin cells, that participate in the regulation of divergent hypothalamic functions (Elmquist et al., 1999
In summary, we have shown that UCP2 is expressed in neurons involved in the regulation of homeostasis in brain regions with the highest proton leak and thermogenesis. UCP2 expression in mitochondria of neurons, particularly in axon terminals, suggests that a mitochondrial uncoupling/thermogenic mechanism plays a direct role in interneuronal communication in circuits involved in the central regulation of homeostasis. Thus, UCP2 in the many neuronal networks regulating body weight may coordinate the behavioral, autonomic, and endocrine responses to a changing environment.
FOOTNOTES Received July 27, 1999; revised Sept. 13, 1999; accepted Sept. 21, 1999.
This work was supported by National Science Foundation Grant IBN-9728581, National Institutes of Health Grants DK-52581 and DK-35747, the University of California at Davis Health System Research Fund, and Grant LR 3112994 noBO41 from Regione Campania. We are indebted to Drs. Pasko Rakic, Anthony van den Pol, Herold Behrman, and Ferenc Livak for their helpful comments and suggestions. This article is dedicated to the memory of Ilona Csapo (1906-1999), whose life has been an inspiration to all who knew her.
Correspondence should be addressed to Tamas L. Horvath, Department of Obstetrics and Gynecology, Yale Medical School, 333 Cedar Street, New Haven, CT 06520. E-mail: tamas.horvath{at}yale.edu.
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