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1- or -
-deficient mice
Departments of 1 Physiology and Pharmacology and 3 Cellular and Molecular Biology, Karolinska Institute, S-171 77 Stockholm, Sweden; and 2 Institute for Experimental Medical Research, Ullevaal Hospital, Oslo, Norway
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The specific role of each subtype of thyroid hormone
receptor (TR) on skeletal muscle function is unclear. We have therefore studied kinetics of isometric twitches and tetani as well as fatigue resistance in isolated soleus muscles of R-
1- or
-
-deficient mice. The results show 20-40% longer contraction
and relaxation times of twitches and tetani in soleus muscles from
TR-1-deficient mice compared with their wild-type
controls. TR--deficient mice, which have high thyroid hormone
levels, were less fatigue resistant than their wild-type controls, but
contraction and relaxation times were not different. Western blot
analyses showed a reduced concentration of the fast-type sarcoplasmic
reticulum Ca2+-ATPase (SERCa1) in
TR-1-deficient mice, but no changes were observed in
TR--deficient mice compared with their respective controls. We
conclude that in skeletal muscle, both TR-1 and TR-
are required to get a normal thyroid hormone response.
skeletal muscle; tetanic force; contraction; relaxation; fatigue
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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THYROID HORMONES AFFECT almost all organs and organ systems in the body, including the brain, liver, heart, and skeletal muscle. Patients with both increased and reduced thyroid hormone levels show disturbances in heart function, including increase in heart rate and cardiac output in hyperthyroidism and bradycardia and decreased cardiac output in hypothyroidism (18). They also display skeletal muscle weakness and increased fatigability (31, 25).
Studies of protein turnover have shown that thyroid hormone increases both global protein synthesis and degradation rates (1). Results from studies of muscle mechanics indicate that alterations in thyroid hormone levels induce 1) changes in maximum shortening velocity (V0) determined from isotonic measurements and 2) changes in contraction and relaxation times measured in the isometric twitch. V0 mainly depends on the myosin isoform composition of the contractile proteins; the slow-type myosin heavy chain (MHC) I and the fast types MHC IIa/x and b (7, 27). Stimulation by 3,5,3'-triiodothyronine (T3) shifts the isoform pattern toward faster types (MHC II) (5), whereas it is shifted toward the slower-type MHC I in hypothyroidism. The contraction and relaxation times depend both on myosin isoform composition and on the Ca2+ transport capacity of sarcoplasmic reticulum Ca2+-ATPase (SERCa). In skeletal muscle, there are two types of SERCa: SERCa1 (fast) and SERCa2 (slow). T3 treatment of rats induces an increase in the total amount of sarcoplasmic reticulum (SR) and the percentage of fibers expressing SERCa1 (10, 22). In hypothyroidism, a reduction in Ca2+ uptake is observed (28, 9), as well as a decrease in both SERCa1 and SERCa2 expression (26). Furthermore, the number of Na+-K+ pumps has been shown to be affected (8, 3), but the significance of this is under debate.
Thyroid hormone exerts its effect mainly through specific nuclear
receptors inducing synthesis of new proteins (23), although extranuclear effects of the hormone have also been observed (6). The
receptors belong to the superfamily of intranuclear receptors and are
encoded by two different genes ( and ). To date, four different
mammalian thyroid hormone receptors (TR) have been characterized (TR-1, TR-2, TR-1, and
TR-2; Ref. 14). The different subtypes of TRs are known
to be distributed widely and are known to be expressed in skeletal
muscle (15). However, the specific physiological role, with respect to
skeletal muscle function, of each subtype of TR is not known. In the
present study, we used mice deficient in either TR-1 or
both TR-1 and TR-2 (i.e.,
TR--deficient mice), which were generated by homologous
recombination as described previously (12, 30). The
TR-1-deficient mice appear normal with respect to gross
anatomy and reproduction (30). Measurement of pituitary thyroid
stimulating hormone (TSH) and serum L-thyroxine (T4) showed that the levels were slightly lower in young
male TR-1-deficient animals compared with wild-type
control mice, indicating a mild hypothyroidism. However, female and old
male TR-1-deficient mice have normal TSH and
T4 levels. Furthermore, even young male
TR-1-deficient mice have a normal concentration of
T3, which is the main biologically active form. The
TR--deficient mice also appear grossly normal, but they have about
three times higher thyroid hormone and TSH levels than their wild-type
controls (12).
The present study was undertaken to investigate the specific role of
TR-1 and TR- on skeletal muscle function. In soleus muscles, we have measured kinetics of isometric twitches and tetani as
well as the fatigue resistance. We have also performed Western blot
(slot blot) to analyze the relative abundance of SERCa and Na+-K+ pump subunits, which are known to be
affected by thyroid hormone (8, 22, 26, 28), as well as ryanodine
receptors (RyR), i.e., the Ca2+ release channels of the SR,
which may also be affected by thyroid hormones (2). The results show
that lack of TR-1 gives a phenotype similar to that
associated with hypothyroidism; that is, both contraction and
relaxation times were markedly slowed. Soleus muscles of
TR--deficient mice were less fatigue resistant than their wild-type
controls, but contraction and relaxation times were not affected in
these mice.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Animals. The contractile performance was studied in five young
(9-14 wk of age) male TR-1-deficient mice and five
wild-type control animals of the same age and weight (28-35 g).
The force-frequency relationship (see below) was studied also in
muscles from four female TR-1-deficient mice and four
wild-type control mice of the same age and weight. The
TR-1-deficient mice represent a cross between the
SV-129/OLa and BALB/c (30). Contractile studies were performed on four
male TR--deficient (12) and four control mice of the same age and
weight as above. This group of mice has a mixed 129/Sv and C57Bl/6J
genetic background, and was generated from
TR-+/
heterozygote backcrosses. The
wild-type mice were obtained from crosses of heterozygote
TR-1- or TR--deficient mice. The two homozygote
wild-type strains were bred in parallel with the respective knockout
strains. Thus the knockout strains have the same genetic background as
their respective knockout strains: 129/Ola and BALB/c for
TR-1, 129/Sv and C57Bl/6J for TR-.
All animals were housed in a temperature (21-23°C)- and humidity (55-60%)-regulated room. Water and food were provided ad libitum. The experimental procedures were approved by the local animal ethics committee.
General. Animals were killed by cervical dislocation. The right and left soleus muscles were then isolated, and the tendons were clamped with a small piece of aluminum foil (4). Muscles were mounted in a stimulation chamber, which had a volume of 50 ml and was filled with continuously stirred Tyrode solution of the following composition (in mM): 121 NaCl, 5 KCl, 0.5 MgCl2, 1.8 CaCl2, 0.4 NaH2PO4, 0.1 NaEDTA, 24 NaHCO3, and 5.5 glucose. Fetal calf serum (0.2%) was added to the solution. The solution was continuously bubbled with 95% O2-5% CO2, which gives a bath pH of 7.4. All experiments were carried out in room temperature (24°C).
Muscles were mounted between a fixed stainless steel hook and a hook attached to a lab-built force transducer. A lab-built stimulation unit was used to give supramaximal electrical pulses (duration 0.5 ms; intensity ~120% of that giving maximum contractile response). The stimulation pulses were applied via two platinum plate electrodes placed on each side of the muscle and extending the whole length of the muscle. The resulting force was recorded and digitized (500 Hz; Axotape, Axon Instruments) and stored in a personal computer. After being mounted, a few tetanic contractions were produced to find the length that gave the maximum tetanic force response and muscles were kept at this length throughout the experiments. Muscles were then allowed to rest for at least 30 min in the oxygenated Tyrode solution before measurements were conducted. While one muscle was being studied, the other was maintained in the oxygenated Tyrode solution.
Protocol. First, each muscle was stimulated to give a single twitch or 600-ms tetani at 10, 15, 20, 30, 50, 70, and 100 Hz. These contractions were produced at 1-min intervals. Peak force in each contraction was measured and is presented as percentage of the maximal force obtained at 100 Hz in that muscle. Twitch kinetics were assessed by measuring the contraction time (i.e., from the onset of force production until peak force was produced) and the half-relaxation time (i.e., from peak force production until force was reduced to 50% of the peak). Kinetics were also assessed in 100-Hz tetani by measuring the half-contraction time (i.e., from the onset of contraction until 50% of the maximum tetanic force was produced) and the half-relaxation time (i.e., from the last stimulation pulse until force was reduced to 50% of the maximum).
After the force-frequency relationship was established, the muscle was fatigued by 50 repeated 70-Hz tetani with a duration of 600 ms and given at 3-s intervals. The recovery of force was studied by giving a 70-Hz tetanus at 1, 2, 5, 10, 15, and 20 min after the end of fatiguing stimulation. The muscle was then allowed to recover for an additional 30 min and was thereafter continuously stimulated at 30 Hz for 2 min. After this, as much as possible of the tendons was cut off. The muscle weight was then measured before it was frozen in liquid nitrogen.
Protein immunoblot analysis (Western blot). The soleus muscles were thawed. Two soleus muscles of each animal were pooled, and muscle proteins were isolated as previously described (24). Protein concentration was determined by the bicinchoninic acid assay (Pierce 23235) using bovine serum albumin as standard. For semiquantitation of different proteins, 1, 2, and 5 µg of the protein preparation were loaded onto a polyvinylidene difluoride (PVDF) filter membrane by the use of a slot blot filtration manifold (Minifold II, Schleicher & Schuell, Dassel, Germany). PVDF membranes were blocked by incubation for 1 h at room temperature or overnight at 4°C in 10% nonfat dry milk in Tris-buffered saline, pH 7.5, with 0.1% Tween 20 (TBS-T). The PVDF membranes were then incubated with primary antibodies diluted in 10% dry milk in TBS-T, washed by five changes of TBS-T, and then incubated for 1 h with either anti-mouse (NA931) or anti-rabbit (NA934) immunoglobulin G conjugated to horseradish peroxidase (Amersham, Oakland, Ontario, Canada). The PVDF membranes were washed by five changes of TBS-T, and the immunoreactive bands were detected by the enhanced chemiluminescence method (RPN2106, Amersham). The membranes were exposed to Hyperfilm-ECL (RPN3103H, Amersham) for various times, and the signal intensity of the slots on the film was quantified with the ImageQuant software (Molecular Dynamics, Queensland, Australia). The mean signal intensity of muscles from each wild-type strain was set to 100%, and all values are presented relative to this.
The primary antibodies used were
anti-Na+-K+-ATPase 2-subunit
(MA3-929, Affinity Bioreagents, 1:250),
anti-Na+-K+-ATPase 2-subunit
(06-168, Upstate Biotechnology, 1:1,000), anti- Na+-K+-ATPase 1-subunit
(06-170, Upstate Biotechnology, 1:1,000), anti-SERCa1 (MA3-912, Affinity Bioreagents, 1:2,500), anti-SERCa2
(MA3-919, Affinity Bioreagents, 1:1,000), and anti-RyR
(MA3-925, Affinity Bioreagents, 1:5,000). As controls we used rat
kidney and rat brain microsomal preparation (Upstate Biotechnology,
12-146 and 12-144, respectively).
Statistics. All values were expressed as means ± SE. Student's unpaired t-tests were used to determine statistical significance between TR-deficient mice and their respective control strains. The significance level was set at P < 0.05 or as indicated. When measurements of contractile parameters were performed on both soleus muscles of one animal, the mean of the two measurements was used in further statistical analyses. Evaluation of the force produced during fatiguing stimulation was performed by calculation of the integral (sum of the force development) in each muscle before comparisons between groups were performed with the t-test.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Typical examples of twitches and 100-Hz tetani produced in
TR-1- and TR--deficient mice and their respective
controls are shown in Fig. 1. In male
TR-1-deficient mice contraction and relaxation times
were significantly increased in both twitches and tetani compared with
their wild-type controls (Table 1). The
female TR-1-deficient mice also showed significantly
longer contraction and relaxation times compared with their controls (data not shown). In TR--deficient mice, on the other hand, no significant changes of the contraction and relaxation times were noticed, although a tendency of a faster tetanic relaxation was observed (not significant with the limited number of experiments performed).
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Absolute forces in 100-Hz tetani were not significantly different in TR-deficient animals compared with their wild-type controls (Table 1). Muscle wet weight and force per wet weight were also not significantly different between the TR-deficient and wild-type animals (data not shown).
Mean data of the force-frequency relationship are shown in Fig.
2. Soleus muscles from the male
TR-1-deficient mice developed a significantly higher
force at 10 and 15 Hz compared with their wild-type controls (Fig.
2A). Soleus muscles from the female
TR-1-deficient mice showed a similar pattern, but force
was significantly higher also at 20 Hz (data not shown). Thus, at lower
stimulation frequencies, force was more fused (i.e., had a higher
degree of summation) in TR-1-deficient mice, which is in
agreement with the slowed kinetics described above. Soleus muscles from
TR--deficient mice and their wild-type controls showed no
significant difference in relative force at any stimulation frequency
(Fig. 2B).
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Mean data of force production during fatigue produced by intermittent
tetanic stimulation are shown in Fig. 3. It
can be seen that in muscles from TR-1-deficient mice
there was no significant difference in fatigue resistance compared with
their wild-type controls (Fig. 3A). During fatigue, muscles
from TR--deficient mice generally produced lower mean forces than
their wild-type controls, and the integral of force produced during the
50 fatiguing tetani was significantly lower in the TR--deficient
mice (Fig. 3B). This indicates that TR--deficient mice were
less fatigue resistant.
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All muscles in this study fully recovered after fatiguing stimulation.
There was no difference in the time course of recovery between muscles
from TR-1-deficient mice and their controls; at 10 min
of recovery, force was not lower than the prefatigue value in either
TR-1-deficient mice (102 ± 3%) or their controls (97 ± 4%). However, force recovery of muscles from the TR--deficient mice was somewhat slower compared with their controls; at 10 min recovery, force was still reduced to 87 ± 3% in TR--deficient mice, whereas it had fully recovered in the controls (99 ± 3%).
Continuous stimulation at 30 Hz for 2 min was performed as a final
test. During this kind of continuous tetanic stimulation, the rate of
force decline would depend on the function of surface membrane
Na+ channels and Na+-K+ pumps (16).
With this continuous stimulation, no significant difference in the
force integral was found in either TR-1- or TR--deficient mice compared with their wild-type controls (Fig. 4).
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Immunoblot analyses showed ~40% reduction in the SERCa1
concentration in soleus muscles of TR-1-deficient mice
compared with their controls (Table 2),
whereas there were no significant differences in the concentration of
SERCa2, RyRs, or 2- and 1-subunits of the
Na+-K+ pump. The concentration of the
Na+-K+ pump 1-subunit was higher
in the TR-1-deficient mice, but it should be noted that
the absolute concentration of this subunit is small in skeletal muscle
(32). No significant differences of any of the analyzed proteins were
observed when TR--deficient mice and their wild-type controls were
compared.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Thyroid hormone receptors (TR-1, TR-2,
and TR-) are known to be expressed in skeletal muscle (15, 17). In
the present study, we have been able to distinguish specific
physiological effects of TR-1 and TR- on skeletal
muscle function. We have found that lack of TR-1 renders
the muscle slower, both with respect to contraction and relaxation. On
the other hand, contraction and relaxation times were not altered in
soleus muscles from TR--deficient mice, perhaps because they have
high thyroid hormone levels, and these muscles were less fatigue
resistant than those from wild-type animals during repeated tetanic stimulation.
The general slowing of isometric contractions observed in
TR-1-deficient mice can, in principle, be due to slowed
cross-bridge kinetics or slowed intracellular Ca2+ handling
(29). Thyroid hormones are known to induce a shift in myosin isoenzyme
distribution so that an increase of the hormone causes a transition
toward faster myosin types, whereas a reduced level has the opposite
effect (17-19). Analyses of the MHC composition of muscles from
TR-1-deficient mice have shown a minor upregulation of
the slow type 1 MHC (33). Furthermore, thyroid hormone is also known to
affect the SR Ca2+ pumping and hypothyroidism results in
decreased mRNA for both SERCa1 and 2 in rat soleus muscles (26, 28). In
line with this, our Western blot analyses of muscles showed a
significant reduction of SERCa1 in TR-1-deficient mice
(Table 2). Thus changes in myosin composition and SERCa1 content in
TR-1-deficient mice can explain the slowed contraction
and relaxation of soleus muscles from these animals. Thus it seems
clear that TR-1 is important for mediating the effects
of thyroid hormone on skeletal muscle cells. However, the changes
observed in TR-1-deficient mice are rather small, which
might indicate that TR- also has a role (see below).
The TR--deficient mice had high thyroid hormone levels (12) and an
intact TR-1. This means that a complete hyperthyroid phenotype would be expected if the effect of thyroid hormone were exerted mainly via TR-1. However, this was not observed:
lack of TR- affected neither contraction nor relaxation times nor any of the proteins measured. Moreover, analyses of MHC subtypes have
shown no differences between these TR--deficient mice and their
controls (33). These data indicate that both TR-1 and TR- are needed for the normal response to thyroid hormone. In line
with this, mice lacking both TR-1 and TR- display
major changes in the MHC composition with a marked increase of the slow myosin type, whereas deficiency of only one type of TR has minor effects (33).
Thyroid hormone has been shown to alter the content of
Na+-K+-ATPase in skeletal muscle (3, 9). Our
Western blot results showed that neither TR-1 nor
TR--deficient mice displayed any consistent changes of the different
subunits of Na+-K+-ATPase (see Table 2). The
only significant change was an increase of the 1-subunit
in TR-1-deficient muscles, and this subtype is of
relatively low abundance in skeletal muscle (32) and hence this
increase may be of little physiological significance. In accordance, we
found no significant difference in force production between deficient
mice and their controls during continuous 30-Hz stimulation, a
stimulation protocol where the force decline is thought to depend on
the function of Na+ channels and
Na+-K+ pumps (16). Taken together, these
results suggest that regarding the expression of
Na+-K+ pump subunits, TR- can fully
substitute for TR-1 because no changes were observed in
TR-1-deficient animals. However, it seems that
TR-1 cannot fully substitute for TR-, because
TR--deficient animals did not display the expected increase of
Na+-K+ pumps with increased thyroid hormone levels.
We conclude that both TR-1 and TR- have effects on
skeletal muscle function and protein expression. Furthermore, the
changes of contractile function and protein content in the two types of TR-deficient mice used in this study were rather modest, which suggests
that the two types of TR can, to a large extent, substitute for each
other. Alternatively, major adaptations occur in TR-deficient animals
so that they have altered sensitivity to thyroid hormone.
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ACKNOWLEDGEMENTS |
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Dr. Kristina Nordström, at Cellular and Molecular Biology, Karolinska Institute, is gratefully acknowledged for breeding of mice.
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FOOTNOTES |
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This study was supported by grants from the Swedish Medical Research Council (nos. 4764 and 10842), Human Frontier Science program (RG0 318/1997), Cancerfonden, Swedish Heart and Lung Foundation, the Swedish National Centre for Sports Research, and funds from the Karolinska Institute.
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. §1734 solely to indicate this fact.
Address for reprint requests and other correspondence: C. Johansson, Dept. of Physiology and Pharmacology, Karolinska Institute, S-171 77 Stockholm, Sweden (E-mail: catarina.johansson{at}fyfa.ki.se).
Received 19 January 1999; accepted in final form 16 September 1999.
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TOP
ABSTRACT
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METHODS
RESULTS
DISCUSSION
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; n = 5 animals) and
wild-type control mice (
; n = 5 animals). B:
force-frequency relation of TR-
; n = 4 animals) and wild-type control mice (
; n = 4 animals).
Values are presented as means ± SE. * Significant difference
(P < 0.05) between TR-deficient mice and their wild-type
controls.
