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Vol. 9, Issue 10, 2905-2916, October 1998
*Department of Pharmacology and
MD/Ph.D
Program, Emory University School of Medicine, Atlanta, Georgia 30322
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ABSTRACT |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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The widely used immunosuppressant cyclosporine A (CSA) blocks nuclear translocation of the transcription factor, NF-AT (nuclear factor of activated T cells), preventing its activity. mRNA for several NF-AT isoforms has been shown to exist in cells outside of the immune system, suggesting a possible mechanism for side effects associated with CSA treatment. In this study, we demonstrate that CSA inhibits biochemical and morphological differentiation of skeletal muscle cells while having a minimal effect on proliferation. Furthermore, in vivo treatment with CSA inhibits muscle regeneration after induced trauma in mice. These results suggest a role for NF-AT-mediated transcription outside of the immune system. In subsequent experiments, we examined the activation and cellular localization of NF-AT in skeletal muscle cells in vitro. Known pharmacological inducers of NF-AT in lymphoid cells also stimulate transcription from an NF-AT-responsive reporter gene in muscle cells. Three isoforms of NF-AT (NF-ATp, c, and 4/x/c3) are present in the cytoplasm of muscle cells at all stages of myogenesis tested. However, each isoform undergoes calcium-induced nuclear translocation from the cytoplasm at specific stages of muscle differentiation, suggesting specificity among NF-AT isoforms in gene regulation. Strikingly, one isoform (NF-ATc) can preferentially translocate to a subset of nuclei within a single multinucleated myotube. These results demonstrate that skeletal muscle cells express functionally active NF-AT proteins and that the nuclear translocation of individual NF-AT isoforms, which is essential for the ability to coordinate gene expression, is influenced markedly by the differentiation state of the muscle cell.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Transcription factors play important roles in tissue development and maintenance by regulating the expression of genes required for cell function. The best studied transcription factors in skeletal muscle cells are the muscle regulatory factor (MRF)1 and myocyte enhancer factor 2 (MEF2) families implicated in establishing the myogenic lineage as well as controlling muscle differentiation. Far less is known about other transcription factors in skeletal muscle.
Nuclear factor of activated T cells (NF-AT) is a transcription factor
discovered for its role in cytokine gene expression in lymphoid cells
(for review see Rao et al., 1997
). Four isoforms of NF-AT
with a high degree of homology to each other are known: NF-ATc, NF-ATp,
NF-AT4/x/c3, and NF-AT3 (Hoey et al., 1995). Under basal
conditions, NF-AT exists as a phosphorylated form in the cytoplasm, but
translocates to the nucleus upon dephosphorylation in response to
increased intracellular calcium levels and activation of the
phos- phatase, calcineurin. In the nucleus, NF-AT forms complexes with AP-1 family members on purine-rich enhancer elements of
specific genes leading to transcriptional activation. The phosphatase activity of calcineurin is blocked by the immunosuppressive drugs, cyclosporine A (CSA) and FK506, thereby preventing the nuclear translocation of NF-AT.
Lymphoid cells are not the only cells that express NF-AT. Skeletal
muscle tissue also expresses mRNA for NF-ATc, NF-ATp, and NF-AT4/x/c3
(Hoey et al., 1995). CSA, a potent immunosuppressive agent
used to reduce organ transplant rejection and to manage autoimmune
disease, can adversely affect skeletal muscle (Hardiman et
al., 1993; Hokanson et al., 1995; Mercier et
al., 1995). Paradoxically, CSA has been reported to have an
ameliorative effect on the muscle weakness of Duchenne muscular
dystrophy patients (Sharma et al., 1993). Together, these
studies suggest that NF-AT proteins may play functional roles in
skeletal muscle development or function.
In this report, we demonstrate that CSA has direct effects on both biochemical and morphological differentiation of skeletal muscle while having a minimal effect on cell proliferation. Skeletal muscle cells are shown to express functionally active NF-AT proteins that are activated by known pharmacological inducers of NF-AT in immune cells. Three isoforms of NF-AT are expressed by muscle cells, but each isoform undergoes calcium-induced nuclear translocation from the cytoplasm at only specific stages of myogenesis, suggesting specificity among NF-AT isoforms in gene regulation.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Antisera and Reagents
A mouse monoclonal antibody against NF-ATc (clone 7A6,
[Timmerman et al., 1997]) was purchased from Affinity
Bioreagents, (Golden, CO). A mouse monoclonal antibody against NF-ATp
(clone G1-D10, [Timmerman et al., 1997]) and a rabbit
polyclonal antibody against NF-AT4/c3/x (Ho et al., 1995)
were obtained from Dr. Gerald Crabtree. For immunoblots, a
rabbit polyclonal antibody against NF-ATp was purchased from Upstate
Biotechnology (Lake Placid, NY). Mouse ascites and normal rabbit serum
were purchased from Sigma Biosciences (St. Louis, MO). Secondary
antibodies were obtained from Jackson Immunoresearch Laboratories,
(West Grove, PA). Tyramide-green was purchased from NEN Dupont (Boston,
MA). SJL mice were purchased from The Jackson Laboratory (Bar Harbor,
ME), whereas C3H/HEN mice were purchased from Harlan Sprague Dawley
(Indianapolis, IN). NF-ATp null mice (Hodge et al., 1996)
were a gift of Dr. Laurie Glimcher. Expression plasmids for NF-ATp
(pSH210) (Ho et al., 1995), NF-ATc (pSH107c) (Northrop
et al., 1994), and NF-AT 4/x/c3 (pSH250A) (Ho et
al., 1995) were obtained from Dr. Gerald Crabtree. Except where
noted, all cell culture supplies were purchased from Life Technologies
(Grand Island, NY). FBS was obtained from Atlanta Biologicals
(Norcross, GA). Basic fibroblast growth factor (bFGF) was purchased
from Promega (Madison, WI). Calf skin collagen was purchased from
Sigma. [methyl-3H]Thymidine was purchased from Amersham
(Arlington Heights, IL). Amphotropic (ATCC CRL-11554) retroviral
producer cells were obtained from the American Type and Culture
Collection (Rockville, MD). D-Luciferin was purchased from
Molecular Probes (Eugene, OR). Thapsigargin was purchased from LC
Chemicals (San Diego, CA). Phorbol myristate acetate and ionomycin were
purchased from Sigma. CSA was a gift of Sandoz (Basel, Switzerland).
Cell Culture
Primary cultures were derived from the tibialis anterior of
adult SJL/J or NF-ATp null mice 2 d after induced muscle damage, and myoblasts were purified to >99% (Rando and Blau, 1994). Mouse myoblasts were grown in growth media (GM: Ham's F10, 20% FBS, 5 ng/ml
bFGF) on collagen-coated dishes in a humidified 5% CO2 atmosphere at 37°C. Dishes were coated with a solution of 0.01% calf
skin collagen in 0.1 N acetic acid, allowed to stand overnight, and
rinsed with sterile PBS. Differentiation was induced by switching confluent myoblast cultures to fusion medium (FM: DMEM, 2 or 15% horse
serum) for 44-48 h. Primary human myoblasts were derived from a muscle
biopsy taken from a 2-y-old donor and were purified to >99% using
flow cytometry (Webster et al., 1988). Human myoblasts were
grown in Ham's F10, 15% FBS, 5 ng/ml bFGF on collagen-coated dishes
in a humidified 5% CO2 atmosphere at 37°C.
Differentiation of human myoblasts was induced by switching confluent
myoblasts cultures to FM containing either 2 or 5% horse serum for
48-80 h.
Cell Proliferation Assays
Human myoblasts (2 × 104) were plated in 24-well collagen-coated tissue culture plates in muscle growth medium. At 24-72 h after plating, the cells were pulsed with 1 µCi/ml [methyl-3H]thymidine (specific activity, 25 Ci/mmol) for 2 h at 37°C. DNA synthesis was assayed by measuring the amount of radioactivity incorporated into trichloroacetic acid-insoluble material. The cells were washed twice with cold PBS, treated with cold 20% trichloroacetic acid for 30 min at 37°C, and lysed for 10 min with 0.1 N NaOH and 0.1% SDS. The lysates were mixed with Scintisafe Econo1 scintillation fluid (Fisher, Pittsburgh, PA) and counted in a Beckmann-LS6000IC liquid scintillation counter. Triplicate wells were used to analyze each experimental condition.
Embryonic Myosin Heavy Expression
Human myoblasts were plated in six-well collagen-coated culture plates in muscle growth medium and grown to high density. High density myoblasts were preincubated in either vehicle or CSA for 24 h before switching to FM, and drug treatment was continued for another 48-80 h. Treatment time was determined by the length of time necessary to obtain extensive myotube formation in the vehicle-treated samples. This time varied depending on the lot number and percentage of serum. Duplicate wells for each condition were lysed in ice-cold RIPA-2 (50 mM Tris, pH 8.0, 150 mM NaCl, 1% NP-40, 0.5% deoxycholate, 0.1% SDS containing protease inhibitors [90 µg/ml phenylmethylsulfonylfluoride, 0.1 mM leupeptin, 0.2 trypsin inhibitor unit/ml aprotinin, 5 µg/ml pepstatin A, 0.2 mM sodium orthovanadate, and 50 µg/ml soybean trypsin inhibitor]). Insoluble material was pelleted by centrifugation.
Equal amounts of protein (10 µg) (Bradford, 1976) were loaded onto
SDS-polyacrylamide minigels consisting of a 7.5% separating gel with a
4% stacking gel (Laemmli, 1970) and electrophoresed at 150 V for 70 min. Proteins were transferred to an Immobilon membrane (Millipore,
Bedford, MA) using a Transblot apparatus (Bio-Rad, Richmond,CA) at 250 mA for 1 h as per the manufacturer's protocol. After nonspecific
binding was blocked by incubation of the membrane with 5% nonfat dry
milk in Tris-buffered saline (TBS), the membrane was incubated
overnight at 4°C with a mouse monoclonal antibody against embryonic
myosin heavy chain (EyMHC) (Cho et al., 1994). The EMyHC
antibody (F.1652) was used as an undiluted hybridoma supernatant. The
membranes were washed in TBS containing 0.1% Tween 20 and further
incubated with a 1:10,000 dilution of a peroxidase-conjugated
anti-mouse IgG in TBS containing 0.1% Tween 20 and 5% horse serum for
1 h at room temperature. After further washing, the membrane was
incubated with an ECL Western blotting detection kit (Amersham) as per
the manufacturer's directions, exposed to Hyperfilm-ECL x-ray film
(Amersham), and developed using an automatic film processor.
Densitometry of the films was performed using an optical scanner and
NIH Image software.
Creatine Kinase Assays
SJL mouse myoblasts were plated at 1.5 × 105
cells per well in 12-well plates in GM. After 4 h, vehicle or CSA
was added, and 12 h later, the GM was replaced with
Insulin-Transferrin-Selenium FM (DMEM, 1:100 dilution of
Insulin-Transferrin-Selenium Supplement [GIBCO BRL], 0.1% BSA, 200 U/ml penicillin G, 200 µg/ml streptomycin). Cells were lysed and
sonicated 24 h later in 0.05 M glycylglycine (pH 7.5), 1% NP-40,
0.1% 
-mercaptoethanol. Creatine kinase (CK) activity was determined
using Sigma Diagnostics procedure number DG147-UV and standardized to
protein levels (Bradford, 1976). Background, defined as
nondifferentiation-specific CK activity in myoblasts maintained in GM,
was subtracted from values determined in drug-treated samples
(mean = 14.5% of vehicle CK activity). Values are reported as
percent of vehicle CK activity (mU/mg protein). Triplicate samples were
analyzed for each concentration of CSA in three independent
experiments.
Induced Regeneration of Skeletal Muscle and Histological Analyses
C3H/HEN mice were anesthetized with an i.p. injection of a cocktail of 35 mg/kg ketamine and 5 mg/kg xylazine, and an incision of ~3 mm was made overlying the tibialis anterior muscles. Muscle damage was induced by direct application of a small piece of dry ice to the surface of the exposed muscle for 5 s. Groups of two to three animals received either PBS or 45 mg/kg CSA i.p daily and were killed 10 d after damage. The muscles were removed, embedded in OCT mounting medium, and frozen in isopentane cooled in liquid nitrogen. Serial cross-sections were collected onto gelatin-coated slides at 400- to 500-µm intervals along the entire length of the muscle and analyzed histologically by hematoxylin and eosin staining.
Retroviral Reporter Plasmids
The retroviral NF-AT-responsive plasmid (pKA7) contains a
luciferase coding sequence under the control of a minimal human IL-2
promoter with an upstream triplex of the distal IL-2 gene NF-AT
response element (Northrop et al., 1993). The control
plasmid (pKA9) is missing the NF-AT response elements, but contains the minimal IL-2 promoter. Both plasmids confer neomycin resistance and
were created by modifications (Boss et al., 1998) to the
retroviral plasmid pLNCX (Miller et al., 1993).
Retroviral Production and Infection
Retroviruses were prepared by transient transfection of
helper-virus free amphotropic producer cells (Pear et al.,
1993) with the plasmids pKA7 or pKA9. The Bing-CAK8 producer cells were
grown in producer growth media (PGM) consisting of DMEM, 4.5 µg/ml
glucose, 10% FBS in a humidified 5% CO2 atmosphere at
37°C. To produce infectious retroviral supernatants, cultured cells
at 50-80% confluence in 100-mm diameter dishes were transfected with
the retroviral plasmids using CaPO4 and 25 µM chloroquine
for 6-12 h before refeeding with 20 ml PGM. Twenty hours after the
start of the transfections, the PGM was aspirated and replaced with 9 ml fresh PGM before the dishes were placed in a humidified 5%
CO2 atmosphere at 32°C to enhance the retroviral titer
(Kotani et al., 1994). Supernatants containing infectious
retroviruses were collected at 48, 60, and 72 h after transfection
refeeding with 9 ml of PGM each time, filtered through a 0.45-µm
syringe tip cellulose acetate filter, aliquoted, snap frozen in liquid
nitrogen, and stored at 
80°C.
SJL myoblasts in multiwell plates were infected by adding retroviral
supernatant supplemented with 10% FBS, 5 ng/ml bFGF, and 4 µg/ml
polybrene and spinning at 2500 rpm for 30 min at 32°C in a Beckman
model GS-6R centrifuge in a swinging bucket rotor (Springer and Blau,
1997). The retroviral supernatant was aspirated, and the cells were
refed with GM and returned to the incubator. The infection protocol was
repeated once more 8-12 h later. Forty-eight hours after the last
infection, the cells were fed with GM containing 50 µg/ml G418. After
3-5 d of selection, the surviving cells were expanded and used for
experiments through approximately 10 more passages. The efficiency of
the two rounds of retroviral infections was estimated at >90% as
little cell death occurred during drug selection.
Drug Treatments and Luciferase Assays
Retrovirally infected SJL myoblasts were plated at 4-7 × 104 cells per well of 24-well collagen-coated plates and used in assays as indicated. Drugs were added to muscle cultures and incubated for 6-7 h at 37°C. The cells were washed with PBS, and 75 µl of lysis buffer (1% Triton X-100, 4 mM EGTA, 25 mM Tris/phosphate, 10% glycerol, 2 mM dithiothreitol) were added to each well and incubated for 10 min at room temperature. The cell lysates were centrifuged at 13,100 × g for 5 min at room temperature, and the supernatants were removed. Luciferase assays were performed by combining 50 µl of supernatant, 350 µl of assay buffer (25 mM Tris/phosphate, 40 mM MgSO4, 4 mM EGTA, 2 mM ATP, 1 mM dithiothreitol), and 100 µl of 0.75 mM D-luciferin. Light output was measured after a 5-s delay over a 10-s window using a Turner TD-20e luminometer (Turner Designs, Sunnyvale, CA).
Immunoblotting of NF-AT Proteins
SJL mouse muscle cells were lysed in RIPA-2 containing protease inhibitors (Complete Mini, Boehringer-Mannheim, Indianapolis, IN). Cellular proteins at 100 µg/lane for NF-ATc and NF-AT4/x/c3 analyses and 50 µg/lane for NF-ATp analysis were separated using SDS-PAGE. Immunoblots were processed as described for F.1652 detection except a peroxidase-conjugated anti-rabbit IgG was used for detection of NF-ATp and NF-AT4/x/c3. Specificity of the antibodies for NF-AT isoforms in immunoblots of muscle proteins was determined by preabsorbing the individual antibodies with extracts from HEK cells transfected with expression plasmids for NF-ATc(pSH107c), NF-AT4/x/c3 (pSH250A), or NF-ATp (pSH210) or control HEK extracts.
Immunohistochemistry
Human myoblasts were plated at approximately 30% confluency in GM. Myoblasts were assayed at high density (80-90% confluency). To induce the formation of multinucleated myotubes, myoblasts were grown to near confluence and switched to FM. Myotubes were assayed at two stages: nascent (24 h in FM) and mature (75-80 h in FM). Cultures were treated with vehicle (0.01% DMSO) or thapsigargin (10 nM) for 10 min at 37°C. In some experiments, CSA (1 µM) was added 10 min before the addition of thapsigargin.
Immediately after the drug treatments, the cells were fixed in 20°C
methanol for 5 min. To block nonspecific protein binding, the cells
were first incubated in blocking buffer (PBS, 2% horse serum, 0.5%
Triton X-100) for 30 min. All antibodies were diluted in this blocking
solution. The cells were further incubated with either a 1:1000
dilution of the anti-NF-ATc monoclonal antibody, a 1:500 dilution of
the anti-NF-ATp monoclonal antibody, or a 1:1500 dilution of the
anti-NF-AT4/x/c3 antibody for 1 h. After three washes, the cells
were incubated with a 1:1000 dilution of either biotinylated anti-mouse
IgG (for NF-ATc and NF-ATp antibodies) or biotinylated anti-rabbit IgG
(for NF-AT4/x/c3) for 30 min. After washing, antibody binding was
detected using TSA-Green according to the manufacturer's directions,
but with a 1:200 dilution of the streptavidin-conjugated horseradish
peroxidase. Specific staining was tested by replacing the primary
monoclonal antibodies with normal ascites or with normal rabbit serum
in the case of the polyclonal NF-AT4/x/c3 antibody or by omitting the
primary antibody. Further specificity was demonstrated by preabsorbing
the NF-ATc and NF-AT4/x/c3 antibodies with extracts from HEK cells
transfected with expression plasmids for these isoforms or control HEK
extracts. Specificity of the NF-ATp antibody was shown by staining of
muscle cultures derived from NF-ATp null mice. All analyses and
photography were performed on a Axiovert microscope (Carl Zeiss,
Thornwood, NY) equipped with a video camera (Optronics Engineering,
Goleta, CA) and Scion Image software (Scion, Frederick, MD).
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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CSA Inhibits Differentiation of Skeletal Muscle
Myogenesis requires growth and differentiation of myoblasts.
Myoblasts are proliferating mononucleated muscle precursor cells that
can be induced to withdraw from the cell cycle and fuse with one
another to form myotubes upon attaining high density in vitro and by a
decrease in growth factors. Myotubes are multinucleated, postmitotic
cells that express proteins characteristic of differentiated myofibers
in vivo. To determine the consequences of CSA on skeletal muscle
myogenesis, both growth and differentiation assays were performed.
First, the effect of CSA on myoblast proliferation was measured.
Myoblasts were treated with different doses of CSA for 24-72 h, and
the cells were then pulse labeled with 3H-thymidine to
quantitate DNA synthesis. As shown in Figure
1A, CSA minimally inhibits myoblast
proliferation. We next determined the effect of CSA on the biochemical
and histological differentiation of myoblasts into myotubes. Cultures
of high-density myoblasts were treated with different doses of CSA in a
low mitogen medium. Differentiation was assayed either by
immunoblots using an antibody to embryonic myosin heavy
chain (EMyHC) or enzymatic assays for CK activity. Both these assays
reveal that biochemical differentiation of myoblasts is inhibited in a
dose-dependent manner. Inhibition of differentiation is indicated by a
decrease in EMyHC expression (Figure 1B) or CK activity (Figure 1C).
Both these markers of differentiated myotubes are inhibited over a
similar range of CSA doses. At the highest dose of CSA tested,
biochemical differentiation is inhibited approximately 75-90%
depending on the specific marker that was assayed. Histological
analyses demonstrate that CSA also inhibits myoblast fusion as
indicated by the few multinucleated differentiated myotubes in the
drug-treated cultures (Figure 1D, panels A and B) in accordance with
the studies by Hardiman et al. (1993).
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To study the effect of CSA in skeletal muscle in vivo, we produced a
localized damage within a limb muscle and then treated groups of
animals with either vehicle or 45 mg/kg CSA i.p. on a daily basis for
10 d. The dose of CSA used in these experiments has previously
been demonstrated to be immunosuppressive in C3H mice (Pavlath et
al., 1994). Limb muscle completely regenerates in 12-14 d after
local damage (Pavlath et al., 1998). As shown in Figure 1D,
control muscles at day 10 (bottom panel, C) are characterized by
centrally nucleated regenerating muscle fibers of various sizes.
Centrally nucleated muscle fibers are a hallmark of muscle regeneration
(Karpati et al., 1988). In contrast, at the same time point,
the muscles of CSA-treated animals (Figure 1D, bottom panel, D) are
greatly deficient in regenerated muscle fibers. Taken together, these
results demonstrate that CSA has profound effects on myogenesis in
skeletal muscle cells.
Functionally Active NF-AT Proteins Exist in Multinucleated Skeletal Muscle Cells
The principal effect of CSA in lymphocytes is to inhibit
NF-AT-mediated transcription. To determine whether skeletal muscle cells express functionally active NF-AT proteins, an NF-AT-responsive luciferase reporter in a retroviral vector (Boss et al.,
1998) was introduced into primary mouse myoblasts in vitro. A
retrovirus-based system was necessary for these studies because
primary myoblasts typically transfect with very low efficiency.
However, with the retroviral method of gene transfer, nearly 99% of
primary myoblasts can be stably transduced with the gene of interest
(Springer and Blau, 1997). This NF-AT responsive reporter contains a
very well characterized mimimal promoter and NF-AT enhancer (Northrop
et al., 1993) and works with the same fidelity as has been
observed in plasmids (Boss et al., 1996) (Boss et
al., 1998).
NF-AT-mediated transcription in lymphocytes is dependent on
simultaneous activation of calcineurin and MAP kinase signaling. Under
basal conditions, NF-AT exists as a phosphorylated form in the
cytoplasm, but translocates to the nucleus upon dephosphorylation in
response to increased intracellular calcium levels and activation of
the phosphatase, calcineurin. CSA blocks the action of calcineurin. The
MAP kinase pathway is dependent on activation of protein kinase c,
which leads to an induction of AP-1 family members. In the nucleus,
NF-AT forms complexes with AP-1 family members on enhancer elements of
specific genes leading to transcriptional activation. To determine
whether differentiated skeletal muscle cells contain functionally
active NF-AT proteins, high-density cultures of myoblasts containing
the NF-AT responsive reporter were allowed to form multinucleated
myotubes. Myotubes were treated with ionomycin, a calcium ionophore, to
induce nuclear translocation of NF-AT and phorbol myristate acetate
(PMA), a protein kinase c activator, to induce AP-1 family members.
Myotubes were treated for 6 h with an optimal dose of PMA or
ionomycin (I) alone, or together in the absence or presence of CSA.
NF-AT- mediated transcription is observed in myotubes containing the
NF-AT responsive luciferase construct (Figure
2A, 
). Both PMA or ionomycin alone
induce luciferase expression, yet a marked synergistic effect is
obtained in the presence of both drugs as expected for an
NF-AT-mediated transcriptional response. This transcriptional response
is blocked by CSA, further indicating that it is an NF-AT-mediated
response. No luciferase activity is present in myotubes containing a
control vector lacking the NF-AT response element (Figure 2A, 
).
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Two other drugs that increase intracellular calcium
levels, but differ in their mechanism of action from ionomycin, were
also tested to determine whether the induction of NF-AT-mediated
transcription in myotubes is specific for ionomycin. Thapsigargin
increases calcium levels by specifically inhibiting the sarcoplasmic
reticulum Ca2+-ATPase (Thastrup et al., 1990),
whereas ryanodine, in the micromolar range, stimulates ryanodine
receptors involved in calcium release from the sarcoplasmic reticulum
(Dulhunty et al., 1996). In the presence of PMA, both
thapsigargin (Figure 2B, panel A) and ryanodine (Figure 2B, panel B)
induce NF-AT-mediated transcription in a dose- dependent manner in
myotubes as measured by the NF-AT responsive reporter plasmid (Figure
2B, 
). The dose-response curve for ionomycin in the presence of PMA
is shown for comparison in Figure 2B, panel C. CSA blocks the
transcriptional responses obtained with all three drugs (Figure 2B,
). Together these results indicate that multinucleated myotubes
contain NF-AT proteins that are functionally active in response to
known pharmacologic inducers of NF-AT-mediated transcription in T
cells.
Induction of NF-AT-mediated Transcription Varies with the Stage of Myogenesis
To determine whether the induction of NF-AT-mediated transcription is restricted to a particular stage of myogenesis, primary mouse muscle cells were assayed either as myoblasts or myotubes. To discriminate more finely among muscle cells during specific stages of myogenesis, these experiments were performed on cells at three stages: myoblasts (80-90% confluent), nascent myotubes (24 h in fusion medium), and mature myotubes (48 h in fusion medium). Mature myotubes are distinguished from nascent myotubes by increased cell size and nuclear number. Muscle cells with the NF-AT responsive reporter plasmid at these three stages of myogenesis were treated for 6 h with an optimal dose of PMA and ionomycin and assayed for luciferase (Figure 3A). NF-AT-mediated transcription is detected at low levels in myoblasts, and these levels progressively increase as myotubes form. The highest level of induction is observed in mature myotubes. Similar differences between human myoblasts and myotubes were obtained.
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To rule out that the increase in NF-AT-mediated transcription observed
as muscle cells become more differentiated is due solely to an increase
in the amount of NF-AT proteins, immunoblots were performed. Since three isoforms of NF-AT are expressed in skeletal muscle tissue as assessed from mRNA studies (Hoey et al.,
1995), isoform-specific antibodies to NF-ATc, NF-ATp, and NF-AT4/x/c3 were used. The sizes of the NF-AT proteins in skeletal muscle cells
(Figure 3B) are similar to those obtained in lymphoid cells (Timmerman
et al., 1997). Furthermore, muscle differentiation is not
accompanied by an increase in the level of any of the three NF-AT
isoforms, indicating that protein content alone cannot account for the
increase in NF-AT-mediated transcription with differentiation. Rather,
NF-AT-mediated transcription is influenced by the developmental state
of the muscle cells. It is most prominently associated with myotubes,
but can occur in myoblasts at ~10-fold lower level.
Nuclear Translocation of each NF-AT Isoform Occurs Only at Specific Stages of Myogenesis
To determine whether muscle cells selectively activate individual
NF-AT isoforms at specific stages of myogenesis, we next performed
immunohistochemical analyses of cultured human muscle cells using
isoform-specific antibodies to NF-ATc, NF-ATp, and NF-AT4/x/c3. Human
muscle cells were used in these experiments rather than mouse cells
because human myotubes are larger and flatter, facilitating their use
in subsequent immunohistochemical analyses. The reported
specificity of these antibodies (Timmerman et al., 1997) was
verified using our immunohistochemical protocols by immunostaining of
HEK293 cells transfected with expression plasmids for each of the
individual isoforms (our unpublished results). In addition, we show
that these antibodies are specific for NF-AT isoforms expressed in
muscle cells (Figure 4). The nuclear staining obtained with the NF-AT4/x/c3 (Figure 4, A and B) and NF-ATc
(Figure 4, C and D) antibodies in thapsigargin-treated skeletal muscle
cells is eliminated by preabsorbing the antibodies with extracts
prepared by transfection of HEK cells with the appropriate NF-AT
expression plasmid (Figure 4, B and D). The specificity of the NF-ATp
antibody in muscle cells is shown by intense cytoplasmic staining of
wild-type (Figure 4E) but not NF-ATp null muscle cells (Figure 4F).
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Immunohistochemical experiments were performed on muscle cells at three stages: myoblasts (80-90% confluent), nascent myotubes (24 h in fusion medium), and mature myotubes (75-80 h in fusion medium) in order again to finely discriminate among different stages of myogenesis. All three NF-AT isoforms are present in both myoblasts and myotubes in agreement with the immunoblot results (Figure 3B). Under basal culture conditions, the three NF-AT isoforms exist in the cytoplasm. Low amounts of the NF-AT isoforms may exist also in the nucleus but are undetectable by the immunochemical methods employed. Striking differences were observed among muscle cells in the calcium-induced nuclear translocation of NF-AT isoforms at all stages of myogenesis tested. Each isoform of NF-AT undergoes calcium-induced nuclear translocation only at specific stages of myogenesis. In myoblasts, calcium-induced, CSA-sensitive nuclear translocation of NF-AT 4/x/c3 is observed (Figure 5, A-C), but not of NF-ATc (Figure 5, D-F) or NF-ATp (Figure 5, G-I). Further selectivity among NF-AT isoforms in calcium-induced nuclear translocation was observed in multinucleated myotubes. Unlike myoblasts, nuclear translocation of NF-AT4/x/c3 is not observed in either nascent or mature myotube cultures (data not shown). Rather, NF-ATp and NF-ATc undergo nuclear translocation in multinucleated myotubes, but with clear differences. Only in 50-60% of nascent myotubes does NF-ATp undergo calcium-induced nuclear translocation (Figure 6B), which occurs to all nuclei within a multinucleated cell and is inhibited by CSA (Figure 6C). In contrast, NF-ATc undergoes calcium-induced nuclear translocation in 90-95% of both nascent and mature myotubes (Figure 7, B-D) that is CSA-sensitive (Figure 7E). Furthermore, in a population of myotubes, thapsigargin induces translocation of NF-ATc to all nuclei within the multinucleated cell (Figure 7B), but in another smaller population of myotubes in the same cultures (10-20%), NF-ATc translocates preferentially to some nuclei within the same cell and not to others (Figure 7, C and D). A nonrandom pattern in nuclear translocation is always observed: positive nuclei are clustered together in a region either at the end of a chain of nuclei (Figure 7C) or within an larger grouping of nuclei (Figure 7D). The frequency of myotubes with such nuclear selectivity is not influenced by the length of thapsigargin treatment. In addition, the number of nuclei contained within a myotube does not appear to influence whether such nuclear selectivity is present. The calcium-induced nuclear translocation of NF-AT isoforms at different stages of muscle development is summarized in Table 1. Together, these results indicate that nuclear translocation of individual NF-AT isoforms in response to calcium varies greatly and is influenced by the differentiation state of muscle.
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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In lymphocytes, the general role of NF-AT proteins in the
induction of early gene expression in response to antigen receptor engagement is well defined (for review, see Rao et al.,
1997). These early response genes include those coding for cytokines and cell surface receptors. Northern analyses suggest that mRNAs for
various NF-AT isoforms exist also in nonlymphoid tissues (Hoey et
al., 1995). NF-AT proteins are present in such diverse cell types
as PC12 (Boss et al., 1996), smooth muscle (Boss et
al., 1998), and endothelium (Cockerill et al., 1995).
In these nonlymphoid cells, little is known about the role of NF-AT
proteins in general or of individual isoforms.
In this study, we demonstrate that CSA, a widely used
immunosuppressant and a well characterized inhibitor of NF-AT-mediated transcription, blocks the differentiation of skeletal muscle cells, suggesting a functional role for NF-AT proteins in skeletal muscle physiology. We hypothesize that the action of CSA is due to inhibition of a critical NF-AT activation event at some specific stage of differentiation. This work confirms and extends the in vitro findings of Hardiman (Hardiman et al., 1993) on CSA effects on
morphological differentiation by demonstrating that muscle regeneration
after induced trauma is inhibited at immunosuppressive doses of CSA. In
addition, we used a combination of functional and immunohistochemical assays to demonstrate the activation and cellular localization of
native NF-AT proteins in skeletal muscle cells in response to known
pharmacological inducers in lymphoid cells. Differences were observed
among developmental stages of muscle, among NF-AT isoforms and even
among nuclei in multinucleated muscle cells. These results indicate
complexity in the regulation of NF-AT in skeletal muscle cells compared
with lymphoid cells.
Developmental Specificity
NF-AT proteins are expressed by skeletal muscle cells at all three
stages of myogenesis tested: myoblasts and nascent and mature myotubes.
The highest levels of NF-AT-mediated transcription in response to
pharmacological stimulators of intracellular calcium and AP-1 are
associated with mature myotubes. Several mechanisms acting alone or in
combination could account for the differences between myoblasts and
differentiated myotubes in the level of NF-AT-mediated transcription
achieved with these drugs. First, different developmental stages of
muscle may differ to the degree to which either intracellular calcium
or AP-1 can be elevated. Second, we have shown that NF-AT 4/x/c3 is the
only isoform in high-density myoblasts that undergoes nuclear
translocation in response to a stimulator of intracellular calcium. The
low levels of NF-AT-mediated transcription in myoblasts, therefore,
may reflect the lower affinity of the NF-AT 4/x/c3 isoform for the
NF-AT response element that was derived from the IL-2 promoter (Ho
et al., 1995; Timmerman et al., 1997) and used in
the reporter construct. Third, in myoblasts, NF-AT4/x/c3 may form
transcriptional complexes with nuclear proteins other than AP-1.
Finally, activation of JNK, a member of the MAP kinase family, has been
recently shown to block nuclear accumulation of recombinant NFAT4/x/c3
in BHK cells (Chow et al., 1997). Drugs, such as PMA, that
induce the expression of AP-1 serve to activate the MAP kinase pathway
in cells.
Isoform Specificity
Three isoforms of NF-AT (p, c, and 4/c3/x) are expressed by muscle
cells at all stages of myogenesis studied. Since all the cells in the
population express each isoform, this implies that each individual cell
must coexpress all three isoforms, as do lymphocytes (Timmerman
et al., 1997). However, in lymphocytes each isoform
undergoes nuclear translocation with the same kinetics in response to a
given stimulus. In contrast, in skeletal muscle cells each isoform
undergoes nuclear translocation only at specific stages of myogenesis.
The ability of individual NF-AT isoforms to undergo calcium-induced
nuclear translocation at only specific stages of myogenesis suggests
that individual NF-AT isoforms may regulate distinct subsets of genes
necessary for muscle cell physiology. The genes that are regulated by
NF-AT in skeletal muscle cells are unknown but currently under
investigation.
The role of individual isoforms of NF-AT in regulating expression of
specific genes in lymphoid cells is unclear. Two lines of evidence
suggest that each NF-AT family member may regulate distinct subsets of
genes. First, in NF-ATp null mice, the expression of some cytokines is
greatly affected, whereas the expression of others is minimally or not
at all affected (Hodge et al., 1996). Second, differences
exist among isoforms in the ability to form transcriptional complexes
on the NF-AT-binding sites in the enhancers of several early response
genes (Timmerman et al., 1997).
The differential ability of natively expressed NF-AT isoforms to
undergo nuclear translocation during muscle development suggests specificity in the activation of NF-AT beyond simply that of the amplitude and duration of changes in intracellular calcium (Dolmetsch et al., 1997). Such specificity may occur at the level of
dephosphorylation of NF-AT isoforms by calcineurin or in the subsequent
nuclear import or export of NF-AT isoforms (Chow et al.,
1997). Possibly, individual isoforms of NF-AT exist in different
subcellular compartments that differ in accessibility to calcium
(Thomas et al., 1996) or downstream effectors.
Nuclear Specificity
Differences were noted among the ability of NF-ATp and NF-ATc to
translocate to individual nuclei within a multinucleated myotube. In
all cases, NF-ATp underwent translocation to all nuclei within a single
multinucleated myotube. In contrast, NF-ATc could preferentially
translocate to only a subset of nuclei within a single multinucleated
myotube in some cases. Calcium-induced nuclear translocation of a
transcription factor to specific nuclei of a multinucleated muscle cell
may be a mechanism for localization of gene products to nuclear domains
or specialized regions of muscle cells (Hall and Ralston, 1989; Pavlath
et al., 1989). Nuclei in the synaptic region of adult muscle
fibers are transcriptionally distinct from other myofiber nuclei
(Changeux, 1991; Moscoso et al., 1995). The nuclei of
myotubes in culture are also not transcriptionally equivalent; some
genes are expressed by a subset of nuclei, whereas other genes are
transcribed by all nuclei equivalently under both aneural (Harris
et al., 1989; Berman et al., 1990; Tsim et
al., 1992; Dutton et al., 1993; Su et al.,
1995) or neural-like (Chu et al., 1995; Grubic et
al., 1995) conditions. How transcriptional differences between
nuclei in myotubes are established is unknown, but appears to be
controlled by a program already active before myoblast fusion (Su
et al., 1995). Thus, gene transcription in multinucleated
cells is regulated not only by classic cis and trans-acting elements, and chromatin structure, but also, as
suggested in this study, by nuclear selectivity in the translocation of transcription factors.
In summary, studies of native NF-AT isoforms in skeletal muscle reveal similiar pharmacological properties to those found in lymphocytes but identify additional complexities in the regulation of individual isoforms. The study of muscle cells isolated from mice genetically deficient in individual NF-AT isoforms will help define the role of specific isoforms in myogenesis. Future studies will delineate the genes that are regulated by NF-AT in skeletal muscle cells and how signal transduction via such NF-AT-regulated pathways contributes to muscle development and function.
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ACKNOWLEDGMENTS |
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We thank Dr. Gerald Crabtree for the antibodies against NF-ATp and NF-AT 4/x/c3, as well as the expression plasmids for each NF-AT isoform, and Dr. Laurie Glimcher for the NF-ATp null mice. T.J.M. is an Established Investigator of the American Heart Association. Supported by grants from the NIH (T.J.M.) and NIH grant AR-43410, Muscular Dystrophy Association, and Emory University Research Council (G.K.P.).
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FOOTNOTES |
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Corresponding author.
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ABBREVIATIONS |
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Abbreviations used: bFGF, basic fibroblast growth factor; CK, creatine kinase; CSA, cyclosporine A; EMyHC, embryonic myosin heavy chain; FBS, fetal bovine serum; FM, fusion medium; GM, growth medium; MEF2, myocyte enhancer factor 2; MRF, myogenic regulatory factor; NF-AT, nuclear factor of activated T Cells; PGM, producer growth medium; PMA, phorbol myristate acetate; TBS, Tris-buffered saline.
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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I. Johnston, H. McLay, M Abercromby, and D Robins Early thermal experience has different effects on growth and muscle fibre recruitment in spring- and autumn-running Atlantic salmon populations J. Exp. Biol., January 9, 2000; 203(17): 2553 - 2564. [Abstract] [PDF]
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D. Thaloor, K. J. Miller, J. Gephart, P. O. Mitchell, and G. K. Pavlath Systemic administration of the NF-kappa B inhibitor curcumin stimulates muscle regeneration after traumatic injury Am J Physiol Cell Physiol, August 1, 1999; 277(2): C320 - C329. [Abstract] [Full Text] [PDF]
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S. E. Dunn, J. L. Burns, and R. N. Michel Calcineurin Is Required for Skeletal Muscle Hypertrophy J. Biol. Chem., July 30, 1999; 274(31): 21908 - 21912. [Abstract] [Full Text] [PDF]
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T. T. Tran, W. Dai, and H. K. Sarkar Cyclosporin A Inhibits Creatine Uptake by Altering Surface Expression of the Creatine Transporter J. Biol. Chem., November 10, 2000; 275(46): 35708 - 35714. [Abstract] [Full Text] [PDF]
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S. Plyte, M. Boncristiano, E. Fattori, F. Galvagni, S. R. Paccani, M. B. Majolini, S. Oliviero, G. Ciliberto, J. L. Telford, and C. T. Baldari Identification and Characterization of a Novel Nuclear Factor of Activated T-cells-1 Isoform Expressed in Mouse Brain J. Biol. Chem., April 20, 2001; 276(17): 14350 - 14358. [Abstract] [Full Text] [PDF]
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S. E. Dunn, A. R. Simard, R. Bassel-Duby, R. S. Williams, and R. N. Michel Nerve Activity-dependent Modulation of Calcineurin Signaling in Adult Fast and Slow Skeletal Muscle Fibers J. Biol. Chem., November 21, 2001; 276(48): 45243 - 45254. [Abstract] [Full Text] [PDF]
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A. L. Serrano, M. Murgia, G. Pallafacchina, E. Calabria, P. Coniglio, T. Lomo, and S. Schiaffino Calcineurin controls nerve activity-dependent specification of slow skeletal muscle fibers but not muscle growth PNAS, November 6, 2001; 98(23): 13108 - 13113. [Abstract] [Full Text] [PDF]
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V. Horsley and G. K. Pavlath Nfat: ubiquitous regulator of cell differentiation and adaptation J. Cell Biol., March 4, 2002; 156(5): 771 - 774. [Abstract] [Full Text] [PDF]
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E. E. Dupont-Versteegden, M. Knox, C. M. Gurley, J. D. Houle, and C. A. Peterson Maintenance of muscle mass is not dependent on the calcineurin-NFAT pathway Am J Physiol Cell Physiol, June 1, 2002; 282(6): C1387 - C1395. [Abstract] [Full Text] [PDF]
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P. O. Mitchell, S. T. Mills, and G. K. Pavlath Calcineurin differentially regulates maintenance and growth of phenotypically distinct muscles Am J Physiol Cell Physiol, May 1, 2002; 282(5): C984 - C992. [Abstract] [Full Text] [PDF]
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6 M CSA (panel B) for 24 h in
ITS fusion medium. Few multinucleated myotubes are present in
CSA-treated cultures. Bar, 20 µm. Bottom panels, CSA inhibits muscle
regeneration in vivo. Localized damage was induced in the tibialis
anterior muscles of mice. Groups of mice were either treated with
vehicle (panel C) or 45 mg/kg CSA i.p. (panel D) daily for 10 d.
Muscle from vehicle-treated animals is characterized by centrally
nucleated muscle fibers of various sizes as expected at this timepoint.
Centrally nucleated muscle fibers are a hallmark of muscle
regeneration. Muscle from CSA-treated animals is greatly deficient in
regenerated muscle fibers. Cryostat sections of muscle in cross-section
stained with hematoxylin and eosin are shown.
