1 Thyroid Research Laboratory, Nuclear Medicine Center, University Hospital, and 2 Institute of Genetic Engineering and Molecular Biology, University of Buenos Aires, 1120 Buenos Aires, Argentina
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ABSTRACT |
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The effects of long-term cold exposure on brown adipose tissue (BAT) thermogenesis in hypothyroid rats have been examined. Thyroid ablation was performed in normal rats after 2 mo of exposure to 4°C, when BAT hypertrophy and thermogenic activity were maximal. After ablation, hypothyroid and normal controls remained in the cold for 2 additional months. At the end of the 4-mo cold exposure, all untreated hypothyroid rats were alive, had normal body temperature, and had gained an average 12.8% more weight than normal controls. Long-term cold exposure of hypothyroid rats markedly increased BAT weight, mitochondrial proteins, uncoupling protein (UCP)-1, mRNA for UCP-1, and oxygen consumption to levels similar to those seen in cold-exposed normal rats. The results indicate that thyroid hormones are required for increased thermogenic capacity to occur as an adaptation to long-term cold exposure. However, cold adaptation can be maintained in the absence of thyroid hormone.
cold acclimation; uncoupling protein-1; hypothyroidism; oxygen consumption; norepinephrine
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INTRODUCTION |
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THE IMPORTANCE OF THE BROWN
ADIPOSE TISSUE (BAT) thermogenic response to acute cold stress
has been widely recognized (for reviews see Refs. 21,
22, 30). Numerous complex phenomena take
place in BAT after exposure to low temperatures, leading to the
synthesis of mitochondrial proteins involved in heat production. A
critical role in this process is the synthesis of uncoupling protein-1
(UCP-1), strongly promoted by norepinephrine (NE) through a synergism
between - and
-adrenergic receptors (24, 32, 40). The presence of the thyroid hormones is essential
to initiate BAT heat production, because triiodothyronine
(T3) potentiates the action of NE on UCP-1 gene
transcription (2-4, 37). This explains the
development of hypothermia in hypothyroid rats soon after exposure to
low temperatures, an effect corrected by the administration of thyroid
hormones but not by the administration of NE (39).
Thyroid hormones are active regulators of basal metabolic rate (BMR) and energy expenditure by a number of mechanisms (9, 12, 38, 39). However, earlier studies had suggested that the thyroid hormone may not be necessary for a sustained normothermia after acclimation to cold has been achieved (for review see Ref. 13). Thus Hsieh and Carlson (25) observed a high metabolic rate and normal life survival in hypothyroid rats adapted to cold before thyroidectomy. Despite numerous studies, the influence of thyroid function on the maintenance of normothermia in rodents exposed to prolonged low temperature is not clearly understood.
The purpose of the present study was to assess the role of the thyroid hormones in BAT thermogenesis during long-term cold exposure. After a period of time in the cold, rats were made hypothyroid. Hypothyroid and normal controls were then maintained for an additional period of time in the cold, and thereafter BAT was studied. Accordingly, hypothyroidism was induced after BAT hypertrophy and thermogenic activity were maximally activated. In contrast, room temperature-adapted hypothyroid rats are unsuitable for these studies, because they rapidly develop hypothermia in the cold.
The data presented here show that, although BAT is unable to initiate a thermogenic process in the cold without thyroid hormone, it can maintain a high BAT thermogenic capacity and capacity for a response to NE in hypothyroid rats living in a cold environment, resulting in normothermia and normal survival. The data confirm the accepted role for thyroid hormones in the initial phase of BAT thermogenesis.
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EXPERIMENTAL PROCEDURES |
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Animals and Materials
Male and female Wistar rats with an initial body weight of 108-130 g were used. They had free access to tap water and rat chow. All drugs and reagents, unless otherwise specified, were purchased from Sigma Chemical (St. Louis, MO). Radioactive 131I was obtained from the Atomic Energy Commission of Argentina. The antibody against UCP-1 was purchased from Calbiochem (San Diego, CA). The antibody was free of cross-reactivity against UCP-2 or UCP-3, as determined by the manufacturer. The cDNA probe against rat UCP-1 was kindly provided by Dr. J. E. Silva, McGill University, Montreal, Canada.Experiments
Experiment 1: long-term cold exposure. For measurement of BAT UCP-1, UCP-1 mRNA, and mitochondrial oxygen consumption, rats were placed in individual cages either in a cold room at 4°C or at room temperature (~24°C) lighted between 0600 and 2000 and with unrestricted access to tap water and food pellets. The composition of the diet was 26% protein containing the essential amino acids, 6% fat, and 44% carbohydrates calculated from the nitrogen-free extract. Other components were 6% fiber, vitamins, and 7% ash containing several minerals. Seventy-six percent of the nitrogen was present in digestible form (Pilar Nutrients, Buenos Aires, Argentina). After 2 mo of cold exposure, groups of rats were made hypothyroid by intraperitoneal injection of 131I, and the others were left intact and served as euthyroid controls. Hypothyroid and normal rats were then maintained for an additional 2 mo in the cold. At the end of 4 mo of cold exposure, a group of five hypothyroid rats was injected subcutaneously with thyroxine (T4; 1.5 µg/100 g body wt) in divided doses daily for 3 days. All animals were killed by cervical dislocation, blood was collected, and interscapular BAT was removed, weighed, properly cleaned of adhering muscle and white fat, and immediately processed in the manner described in Technical Procedures.
Experiment 2: acute cold exposure. Other groups of rats were made hypothyroid at room temperature and thereafter were placed in the cold room at 4°C for 14 h. Normal and T4-treated rats were left in the cold room for 24 h, and their controls remained in the warm room. BAT was obtained for the measurement of mitochondrial oxygen consumption and UCP-1 content.
Experiment 3: Methimazole treatment and measurement of hepatic
mitochondrial -glycerophosphate dehydrogenase activity in
cold-acclimated rats.
Despite the fact that 131I treatment has been shown to be
an effective means to abolish thyroid gland function (5),
some of these animals might still have had minimal amounts of
T4 or T3 in serum that might distort the
interpretation of results. To eliminate any possible residual thyroid
hormone production, a group of six 131I-treated hypothyroid
rats in the cold room was given a second antithyroid treatment with
2-mercapto-1-methyl-imidazole (methimazole; 0.03%) in the drinking
water. The treatment began 1 mo after the injection of
131I (3 mo after commencement of cold exposure) and was
extended for 1 mo. Animals were killed, and BAT and liver were removed and processed.
Technical Procedures
Isolation of BAT mitochondria. BAT was homogenized on ice in buffer containing sucrose (0.25 M), N-tris-methyl-2-aminoethanesulfonic acid (K-TES; 5 mM), disodium ethylenediaminetetraacetic acid (EDTA; 2 mM), and bovine serum albumin (2%; pH 7.2). Mitochondria were isolated by differential centrifugation as described by Cannon and Lindberg (8). The final pellet was taken to 1-ml volume in sucrose buffer (0.24 M). Protein content was measured in an aliquot of this suspension by use of the method of Gornall et al. (19) and expressed as milligrams per milliliter.
Western blot analysis. SDS-PAGE electrophoresis was done according to Laemmli (27). Samples were treated with cracking buffer and heated for 3 min at 100°C. Mitochondrial protein (80, 15, or 20 µg) was loaded in each lane. After electrophoresis, gels were electrotransferred to nitrocellulose Hybond-C membranes (Amersham, Arlington Heights, IL). For Western blot assays, nitrocellulose Hybond sheets were blocked with 5% powdered milk in TBST buffer (50 mM Tris · HCl, pH 7.4, 0.15 M NaCl, 0.05% Tween 20) for 1-2 h. The membranes were incubated with polyclonal antisera anti-UCP-1 (Calbiochem) diluted in blocking solution for 2 h, subjected to three 5-min washes with TBST, and incubated with a second antibody linked to horseradish peroxidase (Amersham) and visualized by enhanced chemiluminescence detection (Renaissance, NEN-Du Pont). Quantifications were carried out with the PC-Software Image Scion.
Northern blot analysis. Northern blots were performed as described before (1), using a 1.1-kb cDNA probe against rat UCP-1 (34). Total RNA (15 µg) from BAT was electrophoresed onto 1.4% formaldehyde gels and then blotted onto Hybond N+ nylon membranes (Amersham) according to the manufacturer's procedures. The probe was labeled using the Prime a Gene labeling kit (Promega). Membranes were hybridized overnight with the UCP-1 32P-labeled probe at 65°C in Church's buffer. Sequential stringent washes were performed (2× SSC, 1× SSC, and 0.1× SSC with 0.1% SDS) at 65°C, and blots were exposed to X-OMAT Kodak film. Equal RNA loading was checked in the EtBr staining of the electrophoresis.
BAT mitochondrial oxygen consumption.
BAT mitochondrial oxygen consumption was measured as described
elsewhere (7). It was determined polarographically in an oxygraph (Gilson Medical Electronic, Middleton, WI) with the use of a
Clark electrode at 30°C. The reaction medium had a volume of 0.9 ml
and contained potassium chloride (100 mM), K-TES (20 mM), magnesium
chloride (2 mM), EDTA (1 mM), and 2% BSA, pH 7.2. An aliquot of the
mitochondrial suspension was added to the respiration medium (final
concentration 1.5 mg protein/ml medium). Oxygen uptake was initiated in
state 4 (without ADP). After the velocity of oxygen
consumption was determined, a phosphate acceptor (0.82 mM ADP) was
added to the medium (state 3), and respiration
was allowed to proceed. Results were expressed in nanograms of oxygen per minute per milligram of protein. -GDP was used as substrate because of the presence in BAT of a highly active
-GPD enzyme (8).
-GPD activity.
Mitochondrial
-GPD activity was measured spectrophotometrically at
500 nm and 37°C in liver and BAT by the microassay procedure described by Gardner (14).
Other methods. Serum T4 and T3 concentrations were measured by a double-antibody technique (5) The limits of sensitivity were 5 nmol/l for T4 and 0.12 nmol/l for T3. Body temperature was determined with a clinical thermometer introduced 4 cm into the rectum and kept in place for 3 min. Statistical analysis was performed by analysis of variance and Duncan's test.
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RESULTS |
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Body Weight
After an initial weight loss, all animals gained weight steadily during acclimation to cold, much more so in male than in female rats. At the end of 4 mo, the mean body weight in normal males was 347 ± 17 g and in hypothyroid males 387 ± 15 g, values about three times higher than the initial body weight. In control rats in the warm, body weight increased twofold during this period (data not shown). Body weight in males exceeded that in females by 30.8% in normal rats and 29.2% in hypothyroid rats (P < 0.001). Thyroid ablation did not interrupt weight gain. Body weight in cold-acclimated male and female hypothyroid rats exceeded that in normal rats by an average of 12.8% (P < 0.001). Despite differences in body weight, BAT thermogenic parameters showed no sex differences, and the data were pooled. After 4 mo of cold acclimation, all hypothyroid rats were alive and had normal body temperature (Table 1).
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UCP-1 in hypothyroid BAT was increased by cold acclimation. Figure
1 shows that mitochondrial UCP-1
synthesis in both hypothyroid and normal rats was markedly increased by
acclimation to cold. Figure 1A shows results after loading
80 µg of protein per lane. There was an overexpression of UCP-1 in
both hypothyroid and normal rats. However, the high intensity of the
UCP-1 band prevented comparison of the levels of UCP-1 from rats
exposed to acute (24-h) cold or with rats left in the warm. To
overcome this effect, lanes were loaded with 15 µg of protein. The
results, shown in Fig. 1B, illustrate that, regardless of
the thyroidal state, cold acclimation induced a marked increase in
UCP-1 synthesis compared with rats exposed to 1 day of cold, whereas no
UCP-1 was detected in rats left in the warm. T4 replacement
did not increase the UCP-1 response. Figure 1C depicts the
UCP-1 in normal rats and in rats treated with 131I alone or
131I plus methimazole. Both hypothyroid groups had levels
of UCP-1 similar to those observed in normal rats, thus confirming the deep hypothyroid state in rats treated with the radioisotope alone.
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BAT mRNA Levels
Prolonged cold exposure of normal and hypothyroid rats produced similar and significant increases in BAT UCP-1 mRNA (Fig. 2). T4 treatment failed to alter the results.
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Mitochondrial Oxygen Consumption in State 4 and State 3
Cold acclimation increased about four times the state 4 oxygen uptake in BAT mitochondria of hypothyroid and normal rats (Fig. 3). The administration of T4 did not change the results, which suggests that the hypothyroid BAT was under maximal stimulation. This was confirmed by the same values of maximal oxygen consumption in the presence (state 3) or the absence (state 4) of ADP. These findings are consistent with total uncoupling of the mitochondria. Other indexes of increased BAT thermogenesis in cold-acclimated hypothyroid rats were a fourfold rise in BAT weight and a sevenfold increase in mitochondrial proteins, compared with values in the warm (Table 1).
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Effects of Acute (24 h) Cold Exposure
Both normal and T4-treated rats responded with a 100% increment in BAT oxygen consumption (Fig. 3) and a significant increase in UCP-1 content (Fig. 1) compared with control rats left in the warm. Hypothyroid rats, however, failed to increase BAT oxygen consumption after 14 h in the cold.Effects of Methimazole Treatment
Methimazole treatment reduced slightly more serum T4 levels in cold-acclimated hypothyroid rats but did not alter oxygen consumption (not shown) or UCP-1 synthesis (Fig. 1C).Changes in -GPD Activity
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DISCUSSION |
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The thermogenic effects of thyroid hormones are believed to result
from their widespread metabolic stimulation in many tissues. Their
contribution to BAT heat production was studied more intensively after
1980, when a large number of studies investigated the role of BAT in
nonshivering thermogenesis during acute cold exposure or after cold
acclimation of rodents. It was observed that cold produced rapid and
sustained increases in the activity of the mitochondrial conductance
pathway in BAT through the synthesis of UCP-1, a process accompanied by
hypertrophy and hyperplasia of this tissue (36). These
responses were largely under the control of NE inputs from the
sympathetic nerve endings. Bianco and Silva (3, 4) showed
that the prevention of hypothermia in cold-exposed hypothyroid rats
correlated with the degree of UCP-1 concentration and that this effect
was T3 dependent. Their data showed that 5'-deiodinase type
II (D2) activity in BAT was essential to generate sufficient
intracellular concentration of T3 through T4
deiodination, because circulating T3 alone could not
saturate the nuclear T3 receptor (TR) occupancy that would potentiate the cAMP response to NE stimulation (4). This
observation was recently confirmed in D2 gene-deficient mice showing
hypothermia despite normal UCP-1 concentration (10). The
D2 knockout mice are unable to generate enough T3 to
saturate the TR1 isoform, which appears responsible for
NE signal transduction, whereas the TR
isoform mediates primarily
UCP-1 synthesis (35).
Although there is abundant evidence that thyroid hormones are essential to initiate the thermogenic process in response to low temperature, no solid evidence is available to support a significant role for the thyroid hormones in the maintenance of normothermia in a cold environment. In fact, rats kept outdoors had a significant decrease in both BMR and thyroid function during the cold months (20), and the cold-acclimated mouse maintains a large capacity for nonshivering thermogenesis despite the return of D2 in BAT to a normal low level (26). The findings of high BMR and normal survival in cold-acclimated hypothyroid rats reported by Hsieh and Carlson (25) prompted the authors to suggest that the metabolic response to cold was not directly dependent on the amount of circulating T4. In the present study, the antithyroid treatment was given when BAT hypertrophy and thermogenic activity were maximally stimulated by 2-mo exposure to cold. The effects of cold regularly occur after 4 to 6 wk at low temperatures (22).
The presence of a pronounced hypothyroid state was critical to this
investigation. Because even small quantities of circulating T4 would produce T3, which could stimulate BAT
response to cold (3), emphasis was laid on determining
that these rats were indeed hypothyroid. The hypothyroid state was
confirmed by several lines of evidence. First, the concentrations of
serum T4 and T3 decreased to the limits of
sensitivity of the method, particularly in the eight rats segregated
from the hypothyroid group shown in Table 1 and in six rats treated
with methimazole. Second, further evidence was drawn from the
pronounced fall of hepatic -GPD, which is a reliable index of
T3 activity (29). Another important question
is whether negligible circulating levels of both T4 and
T3 may have been sufficient to stimulate BAT response to
cold. Earlier work by Bianco and Silva (3) showed that
acute cold exposure of hypothyroid rats whose serum T4 and
T3 concentrations were as low as those in the present study
resulted in a 90% fall of BAT UCP-1 and a drop in body temperature to
29°C. After physiological T3 replacement, serum
T3 concentration was normalized, but an 86% fall in UCP-1
synthesis occurred. Maximal (100%) saturation of BAT nuclear
T3 receptors is required for the full expression of UCP-1
synthesis (37). This degree of receptor occupancy could not be reached in cold-exposed, T3-treated hypothyroid rats
even after the administration of >15 times the physiological
T3 replacement and extremely hyperthyroid levels of serum
T3 (3). This phenomenon explains the
development of hypothermia during cold exposure of hypothyroid rats
treated with physiological amounts of T3 (6, 7). The foregoing data are consistent with the fact that thyroid hormone production in hypothyroid rats was nil or sufficiently low that
it resulted in a deep hypothyroid state. Furthermore, the negligible
levels of circulating thyroid hormones were insufficient to initiate,
or even maintain, BAT thermogenesis in a cold environment.
BAT hypertrophy and enhancement of thermogenesis in euthyroid rats
during long-term cold acclimation were shown long ago
(36), but the maintenance of a sustained hypertrophied
state and high indexes of BAT thermogenesis in cold-adapted hypothyroid
rats have not been previously reported and were unexpected. The
hypothyroid rats were normothermic and had elevated levels of UCP-1,
UCP-1 mRNA, and mitochondrial oxygen consumption. The magnitude reached by the thermogenic parameters suggests that this tissue was under maximal stimulation, a contention supported by the failure of exogenous
T4 to promote further increments of UPC-1 synthesis or
oxygen consumption. These findings agree with those in which the
addition of ADP to the respiration medium failed to stimulate oxygen
consumption, an indication that the mitochondria were uncoupled. The
results suggest that, despite the absence of T3, which is needed for full expression of -adrenergic receptors, there was sufficient sympathetic signaling to stimulate maximal BAT activation. The adequacy of sympathetic inputs in BAT and other tissues in the
absence of T3 can be seen in the normothermia of
cold-acclimated hypothyroid rats, as discussed below.
In a physiological setting, the metabolic activity in tissues other than BAT contributes to normothermia through a variety of pathways, including thyroid hormone modulation of mitochondrial oxygen consumption (9, 12, 15, 31, 38). These effects are exerted on the mitochondria of specific target tissues like liver and skeletal muscle, which are the most important oxygen consumers (33). It has been shown that the stimulation of thermogenesis by the thyroid hormones is related to the activity of the mitochondrial nitric oxide synthase, which is able to regulate mitochondrial and systemic oxygen consumption in different tissues and conditions through the production of nitric oxide (11). We have recently found an increased transcription and activity of liver and muscle mitochondrial nitric oxide synthase in hypothyroid rats and a decrease in hyperthyroid rats (9), which suggests that modulation of this enzyme is a substantial part of thyroid effects on mitochondrial oxygen consumption in the main heat-producing tissues.
From the findings that acclimated hypothyroid rats were normothermic, one can reasonably assume that heat production in other thermogenic tissues was not significantly affected by cessation of T3 supply. This effect is particularly important in skeletal muscle, where T3 is essential for the synthesis of UCP-3 (17, 28, 41). We have preliminary data showing that muscle mitochondrial oxygen consumption in cold-acclimated hypothyroid rats was lower than that in normal rats in the cold but twofold higher than that in hypothyroid controls in the warm, whereas consumption in cold-exposed muscle dropped to less than one-half after treatment with reserpine. These findings suggest that the hypothyroid muscle can respond to enhanced caloric demands in the cold with an increase in nonshivering heat production, mediated predominantly by sympathetic inputs. These findings agree with the reports of Gong et al. (18) and Himms-Hagen and Harper (23), suggesting that uncoupling of mitochondria by UCP-3 is not a major determinant of muscle thermogenesis.
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ACKNOWLEDGEMENTS |
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This work was supported by Grants PIP 4002 from the Consejo
Nacional de Investigaciones Cientificas y Tenicas and PICT 1678 from the Fondo Nacional para la Investigación Cientifica y
Tecnológica (FONCYT) in Argentina.
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FOOTNOTES |
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Address for reprint requests and other correspondence: Angel A. Zaninovich, Hospital de Clínicas, Nuclear Medicine Center, Av. Córdoba 2351, 1120 Buenos Aires, Argentina (E-mail: azaninovich{at}sinectis.com.ar).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
May 15, 2002;10.1152/ajpendo.00540.2001
Received 5 December 2001; accepted in final form 13 May 2002.
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