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First published online February 29, 2008
Journal of Experimental Biology 211, 837-843 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.014340
Quantitative analysis of neonatal skeletal muscle functional improvement in the mouse
1 Department of Bioengineering, University of California-San Diego and Veterans
Affairs Medical Center, La Jolla, CA 92093, USA
2 Department of Orthopaedic Surgery, University of California-San Diego and
Veterans Affairs Medical Center, La Jolla, CA 92093, USA
3 Department of Radiology, University of California-San Diego and Veterans
Affairs Medical Center, La Jolla, CA 92093, USA
* Author for correspondence (e-mail: rlieber{at}ucsd.edu)
Accepted 7 January 2008
 |
Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Key words: skeletal muscle, isometric stress, growth, maturation, myofibril, desmin
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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). Postnatal muscle growth is attributed primarily to muscle
fiber hypertrophy, which increases the diameter of existing fibers through
protein deposition and, synergistically, through the differentiation of
myogenic stem cells that synthesize new myotubes and establish new myonuclear
domains (Christ and Brand-Saberi,
2002; O'Connor et al.,
2007; White and Esser,
1989; Zammit et al.,
2006). However, during muscle growth, and specifically during the
perinatal period, muscle tissue dramatically increases its mechanical
abilities independently of size. In the mouse, muscle isometric stress
increases roughly tenfold, from 
25 kPa immediately after birth
(Bang et al., 2006) to 250
kPa by musculoskeletal maturity (Sam et
al., 2000). Clearly, a size-independent maturational process
occurs during postnatal muscle growth, but the underlying biochemical,
morphological and architectural factors that affect function during muscle
growth have not been defined.
When considering muscle function, the mechanical machinery may be
considered as the composite of the force-generating myofibrillar apparatus and
the lateral force transmission network. The principal thick filament
constituent of the myofibril is myosin heavy chain (MyHC), and developmental
heterogeneity across muscles arises in part from differences in the expression
of MyHC isoforms, which include at least two early developmental [embryonic
(EMB) and neonatal (NEO)] and four mature (I, IIA, IIX and IIB) isoforms
(Bottinelli, 2001;
Schiaffino and Reggiani,
1994). Postnatal transitions away from early developmental MyHC
isoforms and toward muscle-specific distributions of mature isoforms have been
observed in a number of mammalian species
(Agbulut et al., 2003;
Strbenc et al., 2006;
Wank et al., 2006). In the
lateral force transmission network, an important constituent is the
intermediate filament desmin, which is the first muscle-specific structural
protein to be expressed in the embryo
(Herrmann et al., 1989;
Mayo et al., 1992). Desmin is
essential for complete mechanocoupling from the myofibrillar Z-disk to the
sarcolemma, and, indirectly, to the extracellular matrix
(Li et al., 1997;
Sam et al., 2000;
Shah et al., 2004). However,
it remains unclear whether the maturation of the myofibrillar apparatus or the
lateral force transmission network contributes more to the postnatal
development of muscle stress.
The purpose of this study was to characterize postnatal skeletal muscle growth in mice during a 4-week postnatal time-course, thereby verifying the hypothesis that skeletal muscle undergoes size-independent functional maturation during growth. The goal was to define the time-courses of tissue morphology (muscle fiber size and packing of myofibrils), muscle architecture, biochemistry of relevant muscle structural proteins (MyHC isoforms and desmin), and size-independent muscle contractile function (maximum isometric stress). Stepwise multiple regression analysis determined the predictive capacity of each growth parameter on contractile function.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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Measurement of fiber cross-sectional area
To assess muscle fiber growth, fiber size was measured by laminin
immunohistochemistry and image analysis as described previously
(Minamoto et al., 2007).
Transverse TA sections (thickness: 10 µm) were quenched in
methanol:H2O2 (3:1) to block endogenous peroxidase
activity, and nonspecific binding was blocked with 1% bovine serum albumin
(BSA), followed by 1.5% normal goat serum to which 10% normal rat serum was
added. Sections were immunolabeled overnight with polyclonal anti-laminin
(1:1000; Sigma-Aldrich, St Louis, MO, USA) to label the basement membranes of
the muscle cells. Sections were then incubated for 1 h with Alexa Fluor
594-conjugated secondary goat anti-rabbit IgG (Invitrogen, Carlsbad, CA, USA).
Sections were preserved in Vectashield mounting medium (Vector Laboratories,
Burlingame, CA, USA) and photographed at 10x magnification under a
fluorescence microscope. Images were processed in ImageJ
(http://rsb.info.nih.gov/ij/;
National Institutes of Health, Bethesda, MD, USA) using a custom-made macro
that performed image thresholding and computed areas enclosed by `rings' of
pericellular laminin. Filtering criteria were applied to ensure measurement of
actual muscle fibers, rejecting regions with cross-sectional areas <50
µm2 or >5600 µm2 to eliminate neurovascular
structures or `optically fused' fibers, respectively. In addition, incomplete
fibers along the edge of the image were excluded. Finally, regions with
circularity (defined as the ratio of the diameters of an ellipse) of <0.3
or >1.0 were excluded to avoid measuring fibers from oblique sections.
Measurement of area fraction of contractile material
Cross-sectional area fraction of contractile material was measured by actin
labeling and image analysis. Sections serial to those used for fiber
cross-sectional area measurements were fixed in 3.7% formaldehyde and blocked
in 1% BSA. Sections were incubated with Alexa Fluor 488-conjugated phalloidin
(Invitrogen) to label sarcomeric actin. Sections were preserved in Vectashield
and photographed at 40x magnification. Images were thresholded in ImageJ
using identical fluorescence intensity cutoff values for all images. The area
fraction of fluorescence was used as a measure of the cross-sectional area
fraction of contractile material.
Muscle functional assessment
Isometric contractile tests were performed on mouse pup hindlimbs as
previously described (Bang et al.,
2006). Hindlimbs were transected at the proximal femur, skinned,
and immersed in mammalian Ringer solution (137 mmol l–1 NaCl,
5 mmol l–1 KCl, 24 mmol l–1
NaH2PO4, 2 mmol l–1 CaCl2, 1
mmol l–1 MgSO4, 11 mmol l–1
glucose and 1 mg l–1 curare). Hindlimbs were transferred to a
customized muscle-testing chamber filled with Ringer solution
(Fig. 1). The fragility of
1-day-old muscle and tendons prevented direct muscle testing, and, therefore,
the muscle-tendon–bone complex associated with the TA muscle was used in
all experiments. To fix the hindlimb in the chamber, it was secured distal to
the TA by tying the ankle to a rigid post interfaced with a force transducer
(Model 300B, Aurora Scientific, Aurora, ON, Canada) using silk sutures passing
around the tibiotarsal joint space and around the ventral surface of the foot.
Proximal to the TA, the sharp end of an anodized stainless steel pin was
driven down the shaft of the femur until it protruded from the femoral
condyle. The blunt half was secured with a setscrew attached to a rigid frame.
The plantarflexors were then released at the Achilles tendon and carefully
resected. TA muscle length was measured using a dissecting microscope fitted
with an eyepiece crosshair reticule and translating the chamber under the
field of view from the TA origin to the myotendinous junction with a digital
micrometer. Maximum isometric tension in the dorsiflexors was imposed by
applying a 400 ms train of 0.3 ms pulses delivered at 100 Hz while maintaining
constant muscle length. This measurement was repeated twice at 2 min
intervals. After testing, TA muscles were dissected and weighed. A computer
algorithm written in LabVIEW (National Instruments, Austin, TX, USA) performed
all data acquisition and analysis of force-time records.
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Muscle architecture and isometric stress calculation
To determine the maximum isometric stress generated by each muscle,
isometric tension is typically normalized to physiological cross-sectional
area (PCSA), a metric of force-generating capacity
(Powell et al., 1984). In this
study, an adjusted PCSA* was used to account for variable
myofibrillar packing. Muscle mass (M, in mg), muscle density
(
=1.056, in g cm–3)
(Mendez and Keys, 1960), fiber
pennation angle (
=11.7°)
(Burkholder et al., 1994),
fiber length (Lf, in mm), and the cross-sectional area
fraction of contractile material (Xcsa, as measured
previously) were used to compute adjusted PCSA* (in
mm2), using the formula:
 | (1) |
).
Analysis of muscle stress instead of force allowed comparison of intrinsic
muscle contractility independent of muscle size.
Validation of muscle functional assessment
A pilot experiment was performed in which dorsiflexors from adult mice were
isometrically tested either without (N=4) or with (N=4)
transection of the tibia to eliminate ankle joint torque. Isometric stresses
in both groups were statistically indistinguishable (203±10 kPa without
transection, 227±20 kPa with transection; P>0.1),
indicating that force redirection due to ankle rotation did not occur in the
experimental apparatus. In addition, laser diffraction was to used to measure
sarcomere length in 12 mouse TA muscles, each formalin-fixed at a 90°
ankle angle, which was identical to the ankle angle at which TA muscles were
tested in the experimental apparatus (Fig.
1). The sarcomere length was 2.32±0.08 µm, indicating
that functional experiments were performed near the plateau of the
length-tension curve of the TA.
Gel electrophoresis of myosin heavy chain isoforms
MyHC isoform distributions were determined by adapting the gel
electrophoresis technique previously described
(Talmadge and Roy, 1993).
Muscles were homogenized, and the myofibril-rich pellet was washed and
resuspended in buffer supplemented with protease cocktail (5 µl of 100 mmol
l–1 PMSF, 10 µg µl–1 leupeptin and 10
µg µl–1 pepstatin A). Protein was then diluted in
sample buffer to a concentration of 0.125 mg ml–1 across all
muscle homogenates regardless of initial muscle size. Separation of MyHC
isoforms was performed with SDS–PAGE on polyacrylamide gels (16
cmx22 cm, thickness: 0.75 mm) for 22 h of migration at 275 V at 4°C.
Stacking and resolving gels were 4% and 8% polyacrylamide, respectively. After
migration, gels were silver stained according to the manufacturer's
instructions (Bio-Rad, Hercules, CA, USA). The positions of MyHC isoforms were
determined by their relative electrophoretic mobilities, which have been
characterized previously (Agbulut et al.,
2003; Schiaffino et al.,
1989). Densitometry was performed to compute band intensities
(Quantity One, Bio-Rad) and resultant MyHC isoform distributions.
|
Statistics
The effect of postnatal day on morphological, functional and biochemical
parameters was assessed by one-way analysis of variance (ANOVA) with
post-hoc Fisher's PLSD comparisons. For architectural or biochemical
parameters, linear regression was used to analyze relationships between those
parameters and isometric stress. To determine the relative contributions of
each parameter, the data were reanalyzed with stepwise multiple regression. A
P value of <0.05 was considered statistically significant, and
data are presented as mean ± standard error (s.e.m.).
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RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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1000
µm2 (Barash et al.,
2007; Hamalainen and Pette,
1993; Sartorius et al.,
1998). Strikingly, the packing of myofibrils was very low at P1,
with only 48.1±5.5% of the cross-sectional area occupied by contractile
material (Fig. 2B). In
incompletely filled fibers, accumulation of myofibrils began in the
subsarcolemmal region and moved inward, resulting in the appearance of
`hollow' muscle fibers lacking contractile material near their central axes
(Fig. 2B). Myofibrillar packing
at P28 had reached approximately adult levels, with 92.5±0.9% of the
cross-sectional area filled by myofibrils
(Fig. 2D). Such a robust
increase in myofibrillar packing indicated a near-total filling of the
intracellular space by contractile protein by P28
(Fig. 2F). Morphological maturation occurred synchronously with functional enhancement. The maximum isometric force generated by successive isometric contractions deviated by less than 1%, indicating that hindlimbs did not loosen from the testing apparatus or experience fatigue effects (data not shown). Maximum isometric force increased by approx. fivefold during the experimental time-course, from 1.7±0.1 g at P1 to 8.5±0.4 g by P28. However, since force increase largely arose from an increase in muscle size, stress was preferred as the metric for intrinsic mechanical function. Isometric stress exhibited an approx. sixfold increase from 27±3 kPa at P1 to 169±10 kPa by P28 (Fig. 3E), defining the size-independent increase in mechanical quality during postnatal growth.
Certain architectural parameters followed growth time-courses similar to the morphological parameters and correlated well with isometric stress. For example, muscle mass increased an approx. fourfold from P1 to P28 (Fig. 3B). Similarly, Lf increased approx. fivefold across the experimental time-course (Fig. 3C). Muscle PCSA* did not increase as vigorously, as indicated by a 50% increase from P1 to P28 (Fig. 3D). By ungrouping the samples from postnatal day, it was revealed that both muscle mass (P<0.001; Fig. 3F) and Lf (P<0.0001; Fig. 3G) exhibited significant positive correlations with isometric stress. On the other hand, PCSA* exhibited no significant correlation with isometric stress (P>0.1, Fig. 3H). Both muscle mass and Lf served as proxies for animal age, so their significant correlations with stress were not surprising.
As expected (Agbulut et al.,
2003; Strbenc et al.,
2006), postnatal levels of MyHC isoforms EMB and NEO declined to
0% while expression of isoforms IIX and IIB increased to approximately adult
values (33.7±3.4% IIX and 63.0±1.2% IIB) by P28
(Fig. 4A). Maximum isometric
stress was negatively correlated with levels of EMB and NEO
(P<0.001 for each; Fig.
4B,C) but positively correlated with levels of IIX and IIB
(P<0.001 for each; Fig.
4F,G). That both IIX and IIB isoforms were predictors of
contractile function was of particular interest because they are the principal
thick filament constituents of the mature mouse TA. Low levels of isoforms I
and IIA were observed but did not correlate with contractile function
(P>0.05 for each; Fig.
4D,E), which is appropriate given that neither I nor IIA are
substantially present in the mature mouse TA. Desmin levels increased
immediately postnatally but quickly plateaued by P7
(Fig. 5A), indicating that
adult levels of desmin were achieved before that time-point. Desmin levels
exhibited a weak but statistically significant correlation with isometric
stress (P<0.05; Fig.
5B). These regressions indicate that MyHC composition explained
more of the variance in isometric stress than desmin.
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Stepwise multiple regression analysis was used to determine which architectural and/or biochemical parameter(s) were the best predictors of isometric stress. Using a critical F-to-enter of 4, three regression steps were necessary: (1) the first step of the multiple regression identified Lf as the strongest predictor of isometric stress (F-to-enter=171.8); (2) the second step identified PCSA (F-to-enter=8.9); and (3) the third step identified EMB (F-to-enter=6.3). Because architectural variables depend on muscle size, stepwise regression was performed again using only biochemical parameters. This time, one regression step was necessary because the first step identified NEO as the strongest predictor of isometric stress (F-to-enter=99.8). Together, these data indicate that the decline in early developmental MyHC isoforms was the best size-independent predictor of isometric stress. However, none of these variables are entirely `independent' and probably co-vary during development.
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DISCUSSION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONReferences |
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48%) filling of P1
muscle, compared to the near-total (92%) filling of P28 muscle, is one
basis for the severely impaired stress-generation capacity of newborn mouse
muscle.
In this study, the isometric stress observed at P28 (170 kPa) is still
considerably less than the isometric stress of 250 kPa observed in mature
mouse muscles (Sam et al.,
2000). Assuming that functional quality continues to improve into
weeks beyond the terminal 4-week time-point used in this study, it may be
useful to locate the time-point when mature stress generation is achieved.
While 4 postnatal weeks is sufficient for skeletal maturity, additional time
is necessary for muscular maturity, and the age at which mouse muscles can
generate 250 kPa of isometric stress may define true musculoskeletal
maturity.
Because the fragility and small size of neonatal muscles prevented direct
isometric testing, whole-hindlimb preparations were used instead to measure
tetanic forces in the dorsiflexors. This system is prone to several sources of
error, especially in the PCSA calculation in
Eqn 1. For example, forces were
normalized to the PCSA of the TA muscle alone and neglected the
cross-sectional area contributions of the other ankle dorsiflexors, such as
the extensor digitorum longus (EDL) and extensor hallucis longus (EHL).
Therefore, the PCSAs used here were systematically too low, resulting in
stress values that were systematically high. A previous architectural study in
adult mice (Burkholder et al.,
1994) has shown that the PCSAs of the EDL (1.8±1.6
cm2) and EHL (0.2±0.1 cm2) relative to the TA
(5.3±0.6 cm2) occupy 27% of the cross-sectional area of
the dorsiflexion musculature, suggesting that the impact of this effect is
significant but difficult to quantify without knowledge of the relative muscle
PCSAs in neonatal mice. In addition, PCSA calculations assumed constant muscle
density regardless of age. This assumption is imperfect, especially since the
morphological data showed enhanced myofibrillar packing that might result in
an age-dependent increase in muscle density. However, the error produced by
this assumption is probably small, since mature mouse muscle density (1.056 g
cm–3) is very close to that of water, and the myofibril-free
volume fraction of immature muscle tissue contains mostly water.
Interestingly, early developmental isoforms of MyHC (EMB and NEO) were the
strongest predictors of isometric stress as determined by the stepwise
regression analysis, which is reasonable considering that their dramatic
postnatal reductions occur almost exactly during the 4-week experimental
time-course used here. However, this result is strictly correlative and does
not suggest a causal relationship between reduced EMB or NEO expression and
enhanced mechanical function. Rather, the progressive displacement of EMB and
NEO by mature isoforms IIX and IIB is a more likely cause, with early
developmental isoforms playing placeholder roles for mature isoforms during
development. Gradual reconstruction of the thick filament occurs during
developmental remodeling of muscle through a process mediated by thyroid
hormone, probably resulting in the transient existence of hybrid thick
filaments (Butler-Browne and Whalen,
1984; Butler-Browne et al.,
1987; Adams et al.,
1999). The biomechanical effects of thick filament reconstruction
and MyHC isoform heterogeneity during development remain unknown.
Western blotting for desmin indicated that the lateral force transmission network contributes to the postnatal enhancement of contractile function but not as robustly as MyHC. Therefore, it is likely that the lateral force transmission network is secondary to the myofibrillar apparatus in the postnatal development of muscle stress. While age-dependent changes in desmin levels were less striking than the maturation of MyHC, the western blots used here were limited in that they could not detect possible maturation of desmin cytoskeletal architecture (e.g. enhanced attachment to costameres and/or myofibrillar Z-disks). It is also likely that maturation occurs in other muscle-specific but non-myofibrillar molecular systems that were not explored in this study, such as neuromuscular junction specification, calcium handling and costamere assembly. Maturation of these systems would result in improved muscle contractility independent of either the myofibrillar apparatus or the lateral force transmission network.
The mechanical, morphological and biochemical data all support the notion of size-independent increases in muscle contractile function during growth. Therefore, the bipartite model of muscle growth, incorporating fiber hypertrophy and myogenic differentiation, is incomplete. A third aspect – intrinsic functional enhancement – needs to be considered as well. Together, these aspects of muscle growth may define a three-dimensional `growth space' through which muscles pass during their progression from immature to mature stages of postnatal development. It is likely that muscles follow distinct trajectories through the growth space depending on their anatomical geometries and functional demands. The growth space trajectory of a muscle may serve as a type of developmental fingerprint for its native function.
The structural and functional data regarding neonatal skeletal muscle
presented here provide a secondary benefit to investigators researching the
physiology of muscle-specific proteins. Specifically, these data are necessary
to serve as a reference for studying certain muscle-specific proteins whose
knockout is neonatal-lethal in mouse models. Examples of such proteins include
Myf5, a transcription factor mediating myogenic commitment
(Braun et al., 1992), nebulin,
a regulator of thin filament assembly (Bang
et al., 2006; Witt et al.,
2006), and Cypher, a Z-disk stabilizer
(Zhou et al., 2001). In these
models, severe postnatal myofibrillar degeneration and muscle fiber necrosis
occur secondarily to the gene deletion and render invalid any comparison with
age-matched or mature wild-type controls. Therefore, comparison with immature
wild-type controls at neonatal time-points is preferred.
|
Acknowledgments |
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