[go: up one dir, main page]
More Web Proxy on the site http://driver.im/

Skeletal muscle (commonly referred to as muscle) is one of the three types of vertebrate muscle tissue, the other being cardiac muscle and smooth muscle. They are part of the voluntary muscular system[1] and typically are attached by tendons to bones of a skeleton.[2][3] The skeletal muscle cells are much longer than in the other types of muscle tissue, and are also known as muscle fibers.[4] The tissue of a skeletal muscle is striated – having a striped appearance due to the arrangement of the sarcomeres.

Skeletal muscle
Depiction of skeletal muscle
Details
SynonymsSkeletal striated muscle, striated voluntary muscle
SystemMuscular system
Identifiers
Latinmuscularis skeletalis
MeSHD018482
TA21976
THH2.00.05.2.00002
Anatomical terminology

A skeletal muscle contains multiple fascicles – bundles of muscle fibers. Each individual fiber, and each muscle is surrounded by a type of connective tissue layer of fascia. Muscle fibers are formed from the fusion of developmental myoblasts in a process known as myogenesis resulting in long multinucleated cells. In these cells the nuclei, termed myonuclei, are located along the inside of the cell membrane. Muscle fibers also have multiple mitochondria to meet energy needs.

Muscle fibers are in turn composed of myofibrils. The myofibrils are composed of actin and myosin filaments called myofilaments, repeated in units called sarcomeres, which are the basic functional, contractile units of the muscle fiber necessary for muscle contraction.[5] Muscles are predominantly powered by the oxidation of fats and carbohydrates, but anaerobic chemical reactions are also used, particularly by fast twitch fibers. These chemical reactions produce adenosine triphosphate (ATP) molecules that are used to power the movement of the myosin heads.[6]

Skeletal muscle comprises about 35% of the body of humans by weight.[7] The functions of skeletal muscle include producing movement, maintaining body posture, controlling body temperature, and stabilizing joints.[8] Skeletal muscle is also an endocrine organ.[9][10][11] Under different physiological conditions, subsets of 654 different proteins as well as lipids, amino acids, metabolites and small RNAs are found in the secretome of skeletal muscles.[12]

Skeletal muscles are substantially composed of multinucleated contractile muscle fibers (myocytes). However, considerable numbers of resident and infiltrating mononuclear cells are also present in skeletal muscles.[13] In terms of volume, myocytes make up the great majority of skeletal muscle. Skeletal muscle myocytes are usually very large, being about 2–3 cm long and 100 μm in diameter.[14] By comparison, the mononuclear cells in muscles are much smaller. Some of the mononuclear cells in muscles[15] are endothelial cells (which are about 50–70 μm long, 10–30 μm wide and 0.1–10 μm thick),[16] macrophages (21 μm in diameter) and neutrophils (12-15 μm in diameter).[17] However, in terms of nuclei present in skeletal muscle, myocyte nuclei may be only half of the nuclei present, while nuclei from resident and infiltrating mononuclear cells make up the other half.[13]

Considerable research on skeletal muscle is focused on the muscle fiber cells, the myocytes, as discussed in detail in the first sections, below. However, recently, interest has also focused on the different types of mononuclear cells of skeletal muscle, as well as on the endocrine functions of muscle, described subsequently, below.

Structure

edit

Gross anatomy

edit
Front and back views of the major skeletal muscles of the human body
Front view of major skeletal muscles
Back view of major skeletal muscles

There are more than 600 skeletal muscles in the human body, making up around 40% of body weight in healthy young adults.[18][19][20] In Western populations, men have on average around 61% more skeletal muscle than women.[21] Most muscles occur in bilaterally-placed pairs to serve both sides of the body. Muscles are often classed as groups of muscles that work together to carry out an action. In the torso there are several major muscle groups including the pectoral, and abdominal muscles; intrinsic and extrinsic muscles are subdivisions of muscle groups in the hand, foot, tongue, and extraocular muscles of the eye. Muscles are also grouped into compartments including four groups in the arm, and the four groups in the leg.

Apart from the contractile part of a muscle consisting of its fibers, a muscle contains a non-contractile part of dense fibrous connective tissue that makes up the tendon at each end. The tendons attach the muscles to bones to give skeletal movement. The length of a muscle includes the tendons. Connective tissue is present in all muscles as deep fascia. Deep fascia specialises within muscles to enclose each muscle fiber as endomysium; each muscle fascicle as perimysium, and each individual muscle as epimysium. Together these layers are called mysia. Deep fascia also separates the groups of muscles into muscle compartments.

Two types of sensory receptors found in muscles are muscle spindles, and Golgi tendon organs. Muscle spindles are stretch receptors located in the muscle belly. Golgi tendon organs are proprioceptors located at the myotendinous junction that inform of a muscle's tension.

Skeletal muscle cells

edit

Skeletal muscle cells are the individual contractile cells within a muscle, and are often termed as muscle fibers.[3] A single muscle such as the biceps in a young adult male contains around 253,000 muscle fibers.[22]

Skeletal muscle fibers are multinucleated with the nuclei often referred to as myonuclei. This occurs during myogenesis with the fusion of myoblasts each contributing a nucleus.[23] Fusion depends on muscle-specific proteins known as fusogens called myomaker and myomerger.[24]

Many nuclei are needed by the skeletal muscle cell for the large amounts of proteins and enzymes needed to be produced for the cell's normal functioning. A single muscle fiber can contain from hundreds to thousands of nuclei.[25] A muscle fiber for example in the human biceps with a length of 10 cm can have as many as 3,000 nuclei.[25] Unlike in a non-muscle cell where the nucleus is centrally positioned, the myonucleus is elongated and located close to the sarcolemma. The myonuclei are quite uniformly arranged along the fiber with each nucleus having its own myonuclear domain where it is responsible for supporting the volume of cytoplasm in that particular section of the myofiber.[24][25]

A group of muscle stem cells known as myosatellite cells, also satellite cells are found between the basement membrane and the sarcolemma of muscle fibers. These cells are normally quiescent but can be activated by exercise or pathology to provide additional myonuclei for muscle growth or repair.[26]

Attachment to tendons

edit

Muscles attach to tendons in a complex interface region known as the musculotendinous junction also known as the myotendinous junction, an area specialised for the primary transmission of force.[27] At the muscle-tendon interface, force is transmitted from the sarcomeres in the muscle cells to the tendon.[5] Muscles and tendons develop in close association, and after their joining at the myotendinous junction they constitute a dynamic unit for the transmission of force from muscle contraction to the skeletal system.[27]

Arrangement of muscle fibers

edit
 
Muscle types by fiber arrangement
 
Types of pennate muscle. A – unipennate; B – bipennate; C – multipennate

Muscle architecture refers to the arrangement of muscle fibers relative to the axis of force generation, which runs from a muscle's origin to its insertion. The usual arrangements are types of parallel, and types of pennate muscle. In parallel muscles, the fascicles run parallel to the axis of force generation, but the fascicles can vary in their relationship to one another, and to their tendons.[28] These variations are seen in fusiform, strap, and convergent muscles.[4] A convergent muscle has a triangular or fan-shape as the fibers converge at its insertion and are fanned out broadly at the origin.[28] A less common example of a parallel muscle is a circular muscle such as the orbicularis oculi, in which the fibers are longitudinally arranged, but create a circle from origin to insertion.[29] These different architectures, can cause variations in the tension that a muscle can create between its tendons.

The fibers in pennate muscles run at an angle to the axis of force generation.[29] This pennation angle reduces the effective force of any individual fiber, as it is effectively pulling off-axis. However, because of this angle, more fibers can be packed into the same muscle volume, increasing the physiological cross-sectional area (PCSA). This effect is known as fiber packing, and in terms of force generation, it more than overcomes the efficiency-loss of the off-axis orientation. The trade-off comes in overall speed of muscle shortening and in the total excursion. Overall muscle shortening speed is reduced compared to fiber shortening speed, as is the total distance of shortening.[29] All of these effects scale with pennation angle; greater angles lead to greater force due to increased fiber packing and PCSA, but with greater losses in shortening speed and excursion. Types of pennate muscle are unipennate, bipennate, and multipennate. A unipennate muscle has similarly angled fibers that are on one side of a tendon. A bipennate muscle has fibers on two sides of a tendon. Multipennate muscles have fibers that are oriented at multiple angles along the force-generating axis, and this is the most general and most common architecture.[29]

Muscle fiber growth

edit

Muscle fibers grow when exercised and shrink when not in use. This is due to the fact that exercise stimulates the increase in myofibrils which increase the overall size of muscle cells. Well exercised muscles can not only add more size but can also develop more mitochondria, myoglobin, glycogen and a higher density of capillaries. However, muscle cells cannot divide to produce new cells, and as a result there are fewer muscle cells in an adult than in a newborn.[30]

Muscle naming

edit

There are a number of terms used in the naming of muscles including those relating to size, shape, action, location, their orientation, and their number of heads.

By size
brevis means short; longus means long; longissimus means longest; magnus means large; major means larger; maximus means largest; minor means smaller, and minimus smallest; latissimus means widest, and vastus means huge.[31] These terms are often used after the particular muscle such as gluteus maximus, and gluteus minimus.[32]
By relative shape
deltoid means triangular; quadratus means having four sides; rhomboideus means having a rhomboid shape; teres means round or cylindrical, and trapezius means having a trapezoid shape;[32] serratus means saw-toothed; orbicularis means circular; pectinate means comblike; piriformis means pear-shaped; platys means flat and gracilis means slender.[31] Examples are the pronator teres, and the pronator quadratus.
By action
abductor moving away from the midline; adductor moving towards the midline; depressor moving downwards; elevator moving upwards; flexor moving that decreases an angle; extensor moving that increase an angle or straightens; pronator moving to face down; supinator moving to face upwards;[32] internal rotator rotating towards the body; external rotator rotating away from the body; sphincter decreases the size, and tensor gives tension to; fixator muscles serve to fix a joint in a given position by stabilizing the prime mover whilst other joints are moving.
By number of heads
biceps two; triceps three and quadriceps four.[32]
By location
named after the near main structure such as the temporal muscle (temporalis) near to the temporal bone.[31] Also supra- above; infra- below, and sub- under.[19]
By fascicle orientation
Relative to the midline, rectus means parallel to the midline; transverse means perpendicular to the midline, and oblique means diagonal to the midline.[31] Relative to the axis of the generation of force – types of parallel, and types of pennate muscles.

Fiber types

edit

Broadly there are two types of muscle fiber: Type I, which is slow, and Type II which are fast. Type II has two divisions of type IIA (oxidative), and type IIX (glycolytic), giving three main fiber types.[33] These fibers have relatively distinct metabolic, contractile, and motor unit properties. The table below differentiates these types of properties. These types of properties—while they are partly dependent on the properties of individual fibers—tend to be relevant and measured at the level of the motor unit, rather than individual fiber.[34]

Various Properties of Different Fiber Types[34]
Properties Type I fibers Type IIA fibers Type IIX fibers
Motor Unit Type Slow Oxidative (SO) Fast Oxidative/Glycolytic (FOG) Fast Glycolytic (FG)
Twitch speed Slow Fast Fast
Twitch force Small Medium Large
Resistance to fatigue High High Low
Glycogen content Low High High
Capillary supply Rich Rich Poor
Capillary density High Intermediate Low
Myoglobin High High Low
Red color Dark Dark Pale
Mitochondrial density High High Low
Oxidative enzyme capacity High Intermediate-high Low
Z-line width Intermediate Wide Narrow
Alkaline ATPase activity Low High High
Acidic ATPase activity High Medium-high Low

Slow oxidative (type I) fibers contract relatively slowly and use aerobic respiration to produce ATP. Fast oxidative (type IIA) fibers have fast contractions and primarily use aerobic respiration, but because they may switch to anaerobic respiration (glycolysis), can fatigue more quickly than slow oxidative fibers. Fast glycolytic (type IIX) fibers have fast contractions and primarily use anaerobic glycolysis. The FG fibers fatigue more quickly than the others. Most skeletal muscles in a human contain(s) all three types, although in varying proportions.[35]

Fiber color

edit

Traditionally, fibers were categorized depending on their varying color, which is a reflection of myoglobin content. Type I fibers appear red due to the high levels of myoglobin. Red muscle fibers tend to have more mitochondria and greater local capillary density. These fibers are more suited for endurance and are slow to fatigue because they use oxidative metabolism to generate ATP (adenosine triphosphate). Less oxidative Type II fibers are white due to relatively low myoglobin and a reliance on glycolytic enzymes.

Twitch speed

edit

Fibers can also be classified on their twitch capabilities, into fast and slow twitch. These traits largely, but not completely, overlap the classifications based on color, ATPase, or MHC (myosin heavy chain).

Some authors define a fast twitch fiber as one in which the myosin can split ATP very quickly. These mainly include the ATPase type II and MHC type II fibers. However, fast twitch fibers also demonstrate a higher capability for electrochemical transmission of action potentials and a rapid level of calcium release and uptake by the sarcoplasmic reticulum. The fast twitch fibers rely on a well-developed, anaerobic, short term, glycolytic system for energy transfer and can contract and develop tension at 2–3 times the rate of slow twitch fibers. Fast twitch muscles are much better at generating short bursts of strength or speed than slow muscles, and so fatigue more quickly.[36]

The slow twitch fibers generate energy for ATP re-synthesis by means of a long term system of aerobic energy transfer. These mainly include the ATPase type I and MHC type I fibers. They tend to have a low activity level of ATPase, a slower speed of contraction with a less well developed glycolytic capacity.[36] Fibers that become slow-twitch develop greater numbers of mitochondria and capillaries making them better for prolonged work.[37]

Type distribution

edit

Individual muscles tend to be a mixture of various fiber types, but their proportions vary depending on the actions of that muscle. For instance, in humans, the quadriceps muscles contain ~52% type I fibers, while the soleus is ~80% type I.[38] The orbicularis oculi muscle of the eye is only ~15% type I.[38] Motor units within the muscle, however, have minimal variation between the fibers of that unit. It is this fact that makes the size principal of motor unit recruitment viable.

The total number of skeletal muscle fibers has traditionally been thought not to change. It is believed there are no sex or age differences in fiber distribution; however, proportions of fiber types vary considerably from muscle to muscle and person to person.[citation needed] Among different species there is much variation in the proportions of muscle fiber types.[39]

Sedentary men and women (as well as young children) have 45% type II and 55% type I fibers.[citation needed] People at the higher end of any sport tend to demonstrate patterns of fiber distribution e.g. endurance athletes show a higher level of type I fibers. Sprint athletes, on the other hand, require large numbers of type IIX fibers. Middle-distance event athletes show approximately equal distribution of the two types. This is also often the case for power athletes such as throwers and jumpers. It has been suggested that various types of exercise can induce changes in the fibers of a skeletal muscle.[40]

It is thought that by performing endurance type events for a sustained period of time, some of the type IIX fibers transform into type IIA fibers. However, there is no consensus on the subject.[citation needed] It may well be that the type IIX fibers show enhancements of the oxidative capacity after high intensity endurance training which brings them to a level at which they are able to perform oxidative metabolism as effectively as slow twitch fibers of untrained subjects. This would be brought about by an increase in mitochondrial size and number and the associated related changes, not a change in fiber type.

Fiber typing methods

edit
 
ATPase staining of a muscle cross section. Type II fibers are dark, due to the alkaline pH of the preparation. In this example, the size of the type II fibers is considerably less than the type I fibers due to denervation atrophy.

There are numerous methods employed for fiber-typing, and confusion between the methods is common among non-experts. Two commonly confused methods are histochemical staining for myosin ATPase activity and immunohistochemical staining for myosin heavy chain (MHC) type. Myosin ATPase activity is commonly—and correctly—referred to as simply "fiber type", and results from the direct assaying of ATPase activity under various conditions (e.g. pH).[34] Myosin heavy chain staining is most accurately referred to as "MHC fiber type", e.g. "MHC IIa fibers", and results from determination of different MHC isoforms.[34] These methods are closely related physiologically, as the MHC type is the primary determinant of ATPase activity. However, neither of these typing methods is directly metabolic in nature; they do not directly address oxidative or glycolytic capacity of the fiber.

When "type I" or "type II" fibers are referred to generically, this most accurately refers to the sum of numerical fiber types (I vs. II) as assessed by myosin ATPase activity staining (e.g. "type II" fibers refers to type IIA + type IIAX + type IIXA ... etc.).

Below is a table showing the relationship between these two methods, limited to fiber types found in humans. Subtype capitalization is used in fiber typing vs. MHC typing, and some ATPase types actually contain multiple MHC types. Also, a subtype B or b is not expressed in humans by either method.[41] Early researchers believed humans to express a MHC IIb, which led to the ATPase classification of IIB. However, later research showed that the human MHC IIb was in fact IIx,[41] indicating that the IIB is better named IIX. IIb is expressed in other mammals, so is still accurately seen (along with IIB) in the literature. Non human fiber types include true IIb fibers, IIc, IId, etc.

ATPase Vs. MHC fiber types[34][42][43]
ATPase type MHC heavy chain(s)
Type I MHC Iβ
Type IC MHC Iβ > MHC IIa
Type IIC MHC IIa > MHC Iβ
Type IIA MHC IIa
Type IIAX MHC IIa > MHC IIx
Type IIXA MHC IIx > MHC IIa
Type IIX MHC IIx

Further fiber typing methods are less formally delineated, and exist on more of a spectrum. They tend to be focused more on metabolic and functional capacities (i.e., oxidative vs. glycolytic, fast vs. slow contraction time). As noted above, fiber typing by ATPase or MHC does not directly measure or dictate these parameters. However, many of the various methods are mechanistically linked, while others are correlated in vivo.[44][45] For instance, ATPase fiber type is related to contraction speed, because high ATPase activity allows faster crossbridge cycling.[34] While ATPase activity is only one component of contraction speed, Type I fibers are "slow", in part, because they have low speeds of ATPase activity in comparison to Type II fibers. However, measuring contraction speed is not the same as ATPase fiber typing.

Muscle fiber type evolution

edit

Almost all multicellular animals depend on muscles to move.[46] Generally, muscular systems of most multicellular animals comprise both slow-twitch and fast-twitch muscle fibers, though the proportions of each fiber type can vary across organisms and environments. The ability to shift their phenotypic fiber type proportions through training and responding to the environment has served organisms well when placed in changing environments either requiring short explosive movements (higher fast twitch proportion) or long duration of movement (higher slow twitch proportion) to survive.[47] Bodybuilding has shown that changes in muscle mass and force production can change in a matter of months.[48] Some examples of this variation are described below.[49]

Examples of muscle fiber variation in different animals

edit

Invertebrates

edit

American lobster, Homarus americanus, has three fiber types including fast twitch fibers, slow-twitch and slow-tonic fibers.[50] Slow-tonic is a slow twitch-fiber that can sustain longer contractions (tonic).[51][52]  In lobsters, muscles in different body parts vary in the muscle fiber type proportions based on the purpose of the muscle group.[50]

Vertebrates

edit

In the early development of vertebrate embryos, growth and formation of muscle happens in successive waves or phases of myogenesis. The myosin heavy chain isotype is a major determinant of the specific fiber type. In zebrafish embryos, the first muscle fibers to form are the slow twitch fibers. These cells will undergo migration from their original location to form a monolayer of slow twitch muscle fibers. These muscle fibers undergo further differentiation as the embryo matures.[53]

Reptiles

edit

In larger animals, different muscle groups will increasingly require different fiber type proportions within muscle for different purposes. Turtles, such as Trachemys scripta elegans, have complementary muscles within the neck that show a potential inverse trend of fiber type percentages (one muscle has high percentage of fast twitch, while the complementary muscle will have a higher percentage of slow twitch fibers). The complementary muscles of turtles had similar percentages of fiber types.[51]

Mammals

edit

Chimpanzee muscles are composed of 67% fast-twitch fibers and have a maximum dynamic force and power output 1.35 times higher than human muscles of similar size. Among mammals, there is a predominance of type II fibers utilizing glycolytic metabolism. Because of the discrepancy in fast twitch fibers compared to humans, chimpanzees outperform humans in power related tests. Humans, however, will do better at exercise in aerobic range requiring large metabolic costs such as walking (bipedalism).[54]

Genetic conservation versus functional conservation

edit

Across species, certain gene sequences have been preserved, but do not always have the same functional purpose. Within the zebrafish embryo, the Prdm1 gene down-regulates the formation of new slow twitch fibers through direct and indirect mechanisms such as Sox6 (indirect). In mice, the Prdm1 gene is present but does not control slow muscle genes in mice through Sox6.[55]

Plasticity

edit

In addition to having a genetic basis, the composition of muscle fiber types is flexible and can vary with a number of different environmental factors. This plasticity can, arguably, be the strongest evolutionary advantage among organisms with muscle.

In fish, different fiber types are expressed at different water temperatures.[53] Cold temperatures require more efficient metabolism within muscle and fatigue resistance is important. While in more tropical environments, fast powerful movements (from higher fast-twitch proportions) may prove more beneficial in the long run.[56]

In rodents such as rats, the transitory nature of their muscle is highly prevalent. They have high percentage of hybrid muscle fibers and have up to 60% in fast-to-slow transforming muscle.[48]

Environmental influences such as diet, exercise and lifestyle types have a pivotal role in proportions of fiber type in humans. Aerobic exercise will shift the proportions towards slow twitch fibers, while explosive powerlifting and sprinting will transition fibers towards fast twitch.[47] In animals, "exercise training" will look more like the need for long durations of movement or short explosive movements to escape predators or catch prey.[57]

Microanatomy

edit
 
Structure of muscle fibre showing a sarcomere under electron microscope with schematic explanation.
 
Diagram of sarcoplasmic reticulum with terminal cisternae and T-tubules.

Skeletal muscle exhibits a distinctive banding pattern when viewed under the microscope due to the arrangement of two contractile proteins myosin, and actin – that are two of the myofilaments in the myofibrils. The myosin forms the thick filaments, and actin forms the thin filaments, and are arranged in repeating units called sarcomeres. The interaction of both proteins results in muscle contraction.

The sarcomere is attached to other organelles such as the mitochondria by intermediate filaments in the cytoskeleton. The costamere attaches the sarcomere to the sarcolemma.[5]

Every single organelle and macromolecule of a muscle fiber is arranged to ensure that it meets desired functions. The cell membrane is called the sarcolemma with the cytoplasm known as the sarcoplasm. In the sarcoplasm are the myofibrils. The myofibrils are long protein bundles about one micrometer in diameter. Pressed against the inside of the sarcolemma are the unusual flattened myonuclei. Between the myofibrils are the mitochondria.

While the muscle fiber does not have smooth endoplasmic cisternae, it contains sarcoplasmic reticulum. The sarcoplasmic reticulum surrounds the myofibrils and holds a reserve of the calcium ions needed to cause a muscle contraction. Periodically, it has dilated end sacs known as terminal cisternae. These cross the muscle fiber from one side to the other. In between two terminal cisternae is a tubular infolding called a transverse tubule (T tubule). T tubules are the pathways for action potentials to signal the sarcoplasmic reticulum to release calcium, causing a muscle contraction. Together, two terminal cisternae and a transverse tubule form a triad.[58]

Development

edit
 
Human embryo showing somites labelled as primitive segments.

All muscles are derived from paraxial mesoderm. During embryonic development in the process of somitogenesis the paraxial mesoderm is divided along the embryo's length to form somites, corresponding to the segmentation of the body most obviously seen in the vertebral column.[59] Each somite has three divisions, sclerotome (which forms vertebrae), dermatome (which forms skin), and myotome (which forms muscle). The myotome is divided into two sections, the epimere and hypomere, which form epaxial and hypaxial muscles, respectively. The only epaxial muscles in humans are the erector spinae and small vertebral muscles, and are innervated by the dorsal rami of the spinal nerves. All other muscles, including those of the limbs are hypaxial, and innervated by the ventral rami of the spinal nerves.[59]

During development, myoblasts (muscle progenitor cells) either remain in the somite to form muscles associated with the vertebral column or migrate out into the body to form all other muscles. Myoblast migration is preceded by the formation of connective tissue frameworks, usually formed from the somatic lateral plate mesoderm. Myoblasts follow chemical signals to the appropriate locations, where they fuse into elongated multinucleated skeletal muscle cells.[59]

Between the tenth and the eighteenth weeks of gestation, all muscle cells have fast myosin heavy chains; two myotube types become distinguished in the developing fetus – both expressing fast chains but one expressing fast and slow chains. Between 10 and 40 per cent of the fibers express the slow myosin chain.[60]

Fiber types are established during embryonic development and are remodelled later in the adult by neural and hormonal influences.[39] The population of satellite cells present underneath the basal lamina is necessary for the postnatal development of muscle cells.[61]

Function

edit

The primary function of muscle is contraction.[3] Following contraction, skeletal muscle functions as an endocrine organ by secreting myokines – a wide range of cytokines and other peptides that act as signalling molecules.[62] Myokines in turn are believed to mediate the health benefits of exercise.[63] Myokines are secreted into the bloodstream after muscle contraction. Interleukin 6 (IL-6) is the most studied myokine, other muscle contraction-induced myokines include BDNF, FGF21, and SPARC.[64]

Muscle also functions to produce body heat. Muscle contraction is responsible for producing 85% of the body's heat.[65] This heat produced is as a by-product of muscular activity, and is mostly wasted. As a homeostatic response to extreme cold, muscles are signaled to trigger contractions of shivering in order to generate heat.[66]

 
Classes of levers present in the human skeletal muscular system

Contraction

edit
 
When a sarcomere contracts, the Z lines move closer together, and the I band becomes smaller. The A band stays the same width. At full contraction, the thin and thick filaments overlap.
 
Contraction in more detail

Contraction is achieved by the muscle's structural unit, the muscle fiber, and by its functional unit, the motor unit.[4] Muscle fibers are excitable cells stimulated by motor neurons. The motor unit consists of a motor neuron and the many fibers that it makes contact with. A single muscle is stimulated by many motor units. Muscle fibers are subject to depolarization by the neurotransmitter acetylcholine, released by the motor neurons at the neuromuscular junctions.[67]

In addition to the actin and myosin myofilaments in the myofibrils that make up the contractile sarcomeres, there are two other important regulatory proteins – troponin and tropomyosin, that make muscle contraction possible. These proteins are associated with actin and cooperate to prevent its interaction with myosin. Once a cell is sufficiently stimulated, the cell's sarcoplasmic reticulum releases ionic calcium (Ca2+), which then interacts with the regulatory protein troponin. Calcium-bound troponin undergoes a conformational change that leads to the movement of tropomyosin, subsequently exposing the myosin-binding sites on actin. This allows for myosin and actin ATP-dependent cross-bridge cycling and shortening of the muscle.

Excitation-contraction coupling

edit

Excitation contraction coupling is the process by which a muscular action potential in the muscle fiber causes the myofibrils to contract. This process relies on a direct coupling between the sarcoplasmic reticulum calcium release channel RYR1 (ryanodine receptor 1), and voltage-gated L-type calcium channels (identified as dihydropyridine receptors, DHPRs). DHPRs are located on the sarcolemma (which includes the surface sarcolemma and the transverse tubules), while the RyRs reside across the SR membrane. The close apposition of a transverse tubule and two SR regions containing RyRs is described as a triad and is predominantly where excitation–contraction coupling takes place. Excitation–contraction coupling occurs when depolarization of skeletal muscle cell results in a muscle action potential, which spreads across the cell surface and into the muscle fiber's network of T-tubules, thereby depolarizing the inner portion of the muscle fiber. Depolarization of the inner portions activates dihydropyridine receptors in the terminal cisternae, which are close to ryanodine receptors in the adjacent sarcoplasmic reticulum. The activated dihydropyridine receptors physically interact with ryanodine receptors to activate them via foot processes (involving conformational changes that allosterically activates the ryanodine receptors). As the ryanodine receptors open, Ca2+
is released from the sarcoplasmic reticulum into the local junctional space and diffuses into the bulk cytoplasm to cause a calcium spark. The sarcoplasmic reticulum has a large calcium buffering capacity partially due to a calcium-binding protein called calsequestrin. The near synchronous activation of thousands of calcium sparks by the action potential causes a cell-wide increase in calcium giving rise to the upstroke of the calcium transient. The Ca2+
released into the cytosol binds to Troponin C by the actin filaments, to allow crossbridge cycling, producing force and, in some situations, motion. The sarco/endoplasmic reticulum calcium-ATPase (SERCA) actively pumps Ca2+
back into the sarcoplasmic reticulum. As Ca2+
declines back to resting levels, the force declines and relaxation occurs.[68]

Muscle movement

edit

The efferent leg of the peripheral nervous system is responsible for conveying commands to the muscles and glands, and is ultimately responsible for voluntary movement. Nerves move muscles in response to voluntary and autonomic (involuntary) signals from the brain. Deep muscles, superficial muscles, muscles of the face and internal muscles all correspond with dedicated regions in the primary motor cortex of the brain, directly anterior to the central sulcus that divides the frontal and parietal lobes.

In addition, muscles react to reflexive nerve stimuli that do not always send signals all the way to the brain. In this case, the signal from the afferent fiber does not reach the brain, but produces the reflexive movement by direct connections with the efferent nerves in the spine. However, the majority of muscle activity is volitional, and the result of complex interactions between various areas of the brain.

Nerves that control skeletal muscles in mammals correspond with neuron groups along the primary motor cortex of the brain's cerebral cortex. Commands are routed through the basal ganglia and are modified by input from the cerebellum before being relayed through the pyramidal tract to the spinal cord and from there to the motor end plate at the muscles. Along the way, feedback, such as that of the extrapyramidal system contribute signals to influence muscle tone and response.

Deeper muscles such as those involved in posture often are controlled from nuclei in the brain stem and basal ganglia.

Proprioception

edit

In skeletal muscles, muscle spindles convey information about the degree of muscle length and stretch to the central nervous system to assist in maintaining posture and joint position. The sense of where our bodies are in space is called proprioception, the perception of body awareness, the "unconscious" awareness of where the various regions of the body are located at any one time. Several areas in the brain coordinate movement and position with the feedback information gained from proprioception. The cerebellum and red nucleus in particular continuously sample position against movement and make minor corrections to assure smooth motion.[citation needed]

Energy consumption

edit
 
(a) Some ATP is stored in a resting muscle. As contraction starts, it is used up in seconds. More ATP is generated from creatine phosphate for about 15 seconds. (b) Each glucose molecule produces two ATP and two molecules of pyruvic acid, which can be used in aerobic respiration or converted to lactic acid. If oxygen is not available, pyruvic acid is converted to lactic acid, which may contribute to muscle fatigue. This occurs during strenuous exercise when high amounts of energy are needed but oxygen cannot be sufficiently delivered to muscle. (c) Aerobic respiration is the breakdown of glucose in the presence of oxygen (O2) to produce carbon dioxide, water, and ATP. Approximately 95 percent of the ATP required for resting or moderately active muscles is provided by aerobic respiration, which takes place in mitochondria.

Muscular activity accounts for much of the body's energy consumption. All muscle cells produce adenosine triphosphate (ATP) molecules which are used to power the movement of the myosin heads. Muscles have a short-term store of energy in the form of creatine phosphate which is generated from ATP and can regenerate ATP when needed with creatine kinase. Muscles also keep a storage form of glucose in the form of glycogen. Glycogen can be rapidly converted to glucose when energy is required for sustained, powerful contractions. Within the voluntary skeletal muscles, the glucose molecule can be metabolized anaerobically in a process called glycolysis which produces two ATP and two lactic acid molecules in the process (in aerobic conditions, lactate is not formed; instead pyruvate is formed and transmitted through the citric acid cycle). Muscle cells also contain globules of fat, which are used for energy during aerobic exercise. The aerobic energy systems take longer to produce the ATP and reach peak efficiency, and requires many more biochemical steps, but produces significantly more ATP than anaerobic glycolysis. Cardiac muscle on the other hand, can readily consume any of the three macronutrients (protein, glucose and fat) aerobically without a 'warm up' period and always extracts the maximum ATP yield from any molecule involved. The heart, liver and red blood cells will also consume lactic acid produced and excreted by skeletal muscles during exercise.

Skeletal muscle uses more calories than other organs.[69] At rest it consumes 54.4 kJ/kg (13.0 kcal/kg) per day. This is larger than adipose tissue (fat) at 18.8 kJ/kg (4.5 kcal/kg), and bone at 9.6 kJ/kg (2.3 kcal/kg).[70]

Efficiency

edit

The efficiency of human muscle has been measured (in the context of rowing and cycling) at 18% to 26%. The efficiency is defined as the ratio of mechanical work output to the total metabolic cost, as can be calculated from oxygen consumption. This low efficiency is the result of about 40% efficiency of generating ATP from food energy, losses in converting energy from ATP into mechanical work inside the muscle, and mechanical losses inside the body. The latter two losses are dependent on the type of exercise and the type of muscle fibers being used (fast-twitch or slow-twitch). For an overall efficiency of 20 percent, one watt of mechanical power is equivalent to 4.3 kcal per hour. For example, one manufacturer of rowing equipment calibrates its rowing ergometer to count burned calories as equal to four times the actual mechanical work, plus 300 kcal per hour, this amounts to about 20 percent efficiency at 250 watts of mechanical output. The mechanical energy output of a cyclic contraction can depend upon many factors, including activation timing, muscle strain trajectory, and rates of force rise & decay. These can be synthesized experimentally using work loop analysis.

Muscle strength

edit
Grading of muscle strength
Grade 0 No contraction
Grade 1 Trace of contraction, but no movement at the joint
Grade 2 Movement at the joint with gravity eliminated
Grade 3 Movement against gravity, but not against added resistance
Grade 4 Movement against external resistance, but less than normal
Grade 5 Normal strength

Muscle strength is a result of three overlapping factors: physiological strength (muscle size, cross sectional area, available crossbridging, responses to training), neurological strength (how strong or weak is the signal that tells the muscle to contract), and mechanical strength (muscle's force angle on the lever, moment arm length, joint capabilities).[citation needed]

Vertebrate muscle typically produces approximately 25–33 N (5.6–7.4 lbf) of force per square centimeter of muscle cross-sectional area when isometric and at optimal length.[71] Some invertebrate muscles, such as in crab claws, have much longer sarcomeres than vertebrates, resulting in many more sites for actin and myosin to bind and thus much greater force per square centimeter at the cost of much slower speed. The force generated by a contraction can be measured non-invasively using either mechanomyography or phonomyography, be measured in vivo using tendon strain (if a prominent tendon is present), or be measured directly using more invasive methods.

The strength of any given muscle, in terms of force exerted on the skeleton, depends upon length, shortening speed, cross sectional area, pennation, sarcomere length, myosin isoforms, and neural activation of motor units. Significant reductions in muscle strength can indicate underlying pathology, with the chart at right used as a guide.

The maximum holding time for a contracted muscle depends on its supply of energy and is stated by Rohmert's law to exponentially decay from the beginning of exertion.

The "strongest" human muscle

edit

Since three factors affect muscular strength simultaneously and muscles never work individually, it is misleading to compare strength in individual muscles, and state that one is the "strongest". But below are several muscles whose strength is noteworthy for different reasons.

  • In ordinary parlance, muscular "strength" usually refers to the ability to exert a force on an external object—for example, lifting a weight. By this definition, the masseter or jaw muscle is the strongest. The 1992 Guinness Book of Records records the achievement of a bite strength of 4,337 N (975 lbf) for 2 seconds. What distinguishes the masseter is not anything special about the muscle itself, but its advantage in working against a much shorter lever arm than other muscles.
  • If "strength" refers to the force exerted by the muscle itself, e.g., on the place where it inserts into a bone, then the strongest muscles are those with the largest cross-sectional area. This is because the tension exerted by an individual skeletal muscle fiber does not vary much. Each fiber can exert a force on the order of 0.3 micronewton. By this definition, the strongest muscle of the body is usually said to be the quadriceps femoris or the gluteus maximus.
  • Because muscle strength is determined by cross-sectional area, a shorter muscle will be stronger "pound for pound" (i.e., by weight) than a longer muscle of the same cross-sectional area. The myometrial layer of the uterus may be the strongest muscle by weight in the female body. At the time when an infant is delivered, the entire uterus weighs about 1.1 kg (40 oz). During childbirth, the uterus exerts 100 to 400 N (25 to 100 lbf) of downward force with each contraction.
  • The external muscles of the eye are conspicuously large and strong in relation to the small size and weight of the eyeball. It is frequently said that they are "the strongest muscles for the job they have to do" and are sometimes claimed to be "100 times stronger than they need to be." However, eye movements (particularly saccades used on facial scanning and reading) do require high speed movements, and eye muscles are exercised nightly during rapid eye movement sleep.
  • The statement that "the tongue is the strongest muscle in the body" appears frequently in lists of surprising facts, but it is difficult to find any definition of "strength" that would make this statement true. The tongue consists of eight muscles, not one.

Force generation

edit

Muscle force is proportional to physiological cross-sectional area (PCSA), and muscle velocity is proportional to muscle fiber length.[72] The torque around a joint, however, is determined by a number of biomechanical parameters, including the distance between muscle insertions and pivot points, muscle size and architectural gear ratio. Muscles are normally arranged in opposition so that when one group of muscles contracts, another group relaxes or lengthens.[73] Antagonism in the transmission of nerve impulses to the muscles means that it is impossible to fully stimulate the contraction of two antagonistic muscles at any one time. During ballistic motions such as throwing, the antagonist muscles act to 'brake' the agonist muscles throughout the contraction, particularly at the end of the motion. In the example of throwing, the chest and front of the shoulder (anterior deltoid) contract to pull the arm forward, while the muscles in the back and rear of the shoulder (posterior deltoid) also contract and undergo eccentric contraction to slow the motion down to avoid injury. Part of the training process is learning to relax the antagonist muscles to increase the force input of the chest and anterior shoulder.

Contracting muscles produce vibration and sound.[74] Slow twitch fibers produce 10 to 30 contractions per second (10 to 30 Hz). Fast twitch fibers produce 30 to 70 contractions per second (30 to 70 Hz).[75] The vibration can be witnessed and felt by highly tensing one's muscles, as when making a firm fist. The sound can be heard by pressing a highly tensed muscle against the ear, again a firm fist is a good example. The sound is usually described as a rumbling sound. Some individuals can voluntarily produce this rumbling sound by contracting the tensor tympani muscle of the middle ear. The rumbling sound can also be heard when the neck or jaw muscles are highly tensed.[citation needed]

Signal transduction pathways

edit

Skeletal muscle fiber-type phenotype in adult animals is regulated by several independent signaling pathways. These include pathways involved with the Ras/mitogen-activated protein kinase (MAPK) pathway, calcineurin, calcium/calmodulin-dependent protein kinase IV, and the peroxisome proliferator γ coactivator 1 (PGC-1). The Ras/MAPK signaling pathway links the motor neurons and signaling systems, coupling excitation and transcription regulation to promote the nerve-dependent induction of the slow program in regenerating muscle. Calcineurin, a Ca2+/calmodulin-activated phosphatase implicated in nerve activity-dependent fiber-type specification in skeletal muscle, directly controls the phosphorylation state of the transcription factor NFAT, allowing for its translocation to the nucleus and leading to the activation of slow-type muscle proteins in cooperation with myocyte enhancer factor 2 (MEF2) proteins and other regulatory proteins. Ca2+/calmodulin-dependent protein kinase activity is also upregulated by slow motor neuron activity, possibly because it amplifies the slow-type calcineurin-generated responses by promoting MEF2 transactivator functions and enhancing oxidative capacity through stimulation of mitochondrial biogenesis.

Contraction-induced changes in intracellular calcium or reactive oxygen species provide signals to diverse pathways that include the MAPKs, calcineurin and calcium/calmodulin-dependent protein kinase IV to activate transcription factors that regulate gene expression and enzyme activity in skeletal muscle.

 
Exercise-induced signaling pathways in skeletal muscle that determine specialized characteristics of slow- and fast-twitch muscle fibers

PGC1-α (PPARGC1A), a transcriptional coactivator of nuclear receptors important to the regulation of a number of mitochondrial genes involved in oxidative metabolism, directly interacts with MEF2 to synergistically activate selective slow twitch (ST) muscle genes and also serves as a target for calcineurin signaling. A peroxisome proliferator-activated receptor δ (PPARδ)-mediated transcriptional pathway is involved in the regulation of the skeletal muscle fiber phenotype. Mice that harbor an activated form of PPARδ display an "endurance" phenotype, with a coordinated increase in oxidative enzymes and mitochondrial biogenesis and an increased proportion of ST fibers. Thus—through functional genomics—calcineurin, calmodulin-dependent kinase, PGC-1α, and activated PPARδ form the basis of a signaling network that controls skeletal muscle fiber-type transformation and metabolic profiles that protect against insulin resistance and obesity.

The transition from aerobic to anaerobic metabolism during intense work requires that several systems are rapidly activated to ensure a constant supply of ATP for the working muscles. These include a switch from fat-based to carbohydrate-based fuels, a redistribution of blood flow from nonworking to exercising muscles, and the removal of several of the by-products of anaerobic metabolism, such as carbon dioxide and lactic acid. Some of these responses are governed by transcriptional control of the fast twitch (FT) glycolytic phenotype. For example, skeletal muscle reprogramming from an ST glycolytic phenotype to an FT glycolytic phenotype involves the Six1/Eya1 complex, composed of members of the Six protein family. Moreover, the hypoxia-inducible factor 1-α (HIF1A) has been identified as a master regulator for the expression of genes involved in essential hypoxic responses that maintain ATP levels in cells. Ablation of HIF-1α in skeletal muscle was associated with an increase in the activity of rate-limiting enzymes of the mitochondria, indicating that the citric acid cycle and increased fatty acid oxidation may be compensating for decreased flow through the glycolytic pathway in these animals. However, hypoxia-mediated HIF-1α responses are also linked to the regulation of mitochondrial dysfunction through the formation of excessive reactive oxygen species in mitochondria.

Other pathways also influence adult muscle character. For example, physical force inside a muscle fiber may release the transcription factor serum response factor from the structural protein titin, leading to altered muscle growth.

Exercise

edit
 
Jogging is one form of aerobic exercise.

Physical exercise is often recommended as a means of improving motor skills, fitness, muscle and bone strength, and joint function. Exercise has several effects upon muscles, connective tissue, bone, and the nerves that stimulate the muscles. One such effect is muscle hypertrophy, an increase in size of muscle due to an increase in the number of muscle fibers or cross-sectional area of myofibrils.[76] Muscle changes depend on the type of exercise used.

Generally, there are two types of exercise regimes, aerobic and anaerobic. Aerobic exercise (e.g. marathons) involves activities of low intensity but long duration, during which the muscles used are below their maximal contraction strength. Aerobic activities rely on aerobic respiration (i.e. citric acid cycle and electron transport chain) for metabolic energy by consuming fat, protein, carbohydrates, and oxygen. Muscles involved in aerobic exercises contain a higher percentage of Type I (or slow-twitch) muscle fibers, which primarily contain mitochondrial and oxidation enzymes associated with aerobic respiration.[77][78] On the contrary, anaerobic exercise is associated with activities of high intensity but short duration, such as sprinting or weight lifting. The anaerobic activities predominately use Type II, fast-twitch, muscle fibers.[79] Type II muscle fibers rely on glucogenesis for energy during anaerobic exercise.[80] During anaerobic exercise, type II fibers consume little oxygen, protein and fat, produce large amounts of lactic acid and are fatigable. Many exercises are partially aerobic and anaerobic; for example, soccer and rock climbing.

The presence of lactic acid has an inhibitory effect on ATP generation within the muscle. It can even stop ATP production if the intracellular concentration becomes too high. However, endurance training mitigates the buildup of lactic acid through increased capillarization and myoglobin.[81] This increases the ability to remove waste products, like lactic acid, out of the muscles in order to not impair muscle function. Once moved out of muscles, lactic acid can be used by other muscles or body tissues as a source of energy, or transported to the liver where it is converted back to pyruvate. In addition to increasing the level of lactic acid, strenuous exercise results in the loss of potassium ions in muscle. This may facilitate the recovery of muscle function by protecting against fatigue.[82]

Delayed onset muscle soreness is pain or discomfort that may be felt one to three days after exercising and generally subsides two to three days later. Once thought to be caused by lactic acid build-up, a more recent theory is that it is caused by tiny tears in the muscle fibers caused by eccentric contraction, or unaccustomed training levels. Since lactic acid disperses fairly rapidly, it could not explain pain experienced days after exercise.[83]

Clinical significance

edit

Muscle disease

edit

Diseases of skeletal muscle are termed myopathies, while diseases of nerves are called neuropathies. Both can affect muscle function or cause muscle pain, and fall under the umbrella of neuromuscular disease. The cause of many myopathies is attributed to mutations in the various associated muscle proteins.[5][84] Some inflammatory myopathies include polymyositis and inclusion body myositis

 
In muscular dystrophy, the affected tissues become disorganized and the concentration of dystrophin (green) is greatly reduced.

Neuromuscular diseases affect the muscles and their nervous control. In general, problems with nervous control can cause spasticity or paralysis, depending on the location and nature of the problem. A number of movement disorders are caused by neurological disorders such as Parkinson's disease and Huntington's disease where there is central nervous system dysfunction.[85]

Symptoms of muscle diseases may include weakness, spasticity, myoclonus and myalgia. Diagnostic procedures that may reveal muscular disorders include testing creatine kinase levels in the blood and electromyography (measuring electrical activity in muscles). In some cases, muscle biopsy may be done to identify a myopathy, as well as genetic testing to identify DNA abnormalities associated with specific myopathies and dystrophies.

A non-invasive elastography technique that measures muscle noise is undergoing experimentation to provide a way of monitoring neuromuscular disease. The sound produced by a muscle comes from the shortening of actomyosin filaments along the axis of the muscle. During contraction, the muscle shortens along its length and expands across its width, producing vibrations at the surface.[86]

Hypertrophy

edit

Independent of strength and performance measures, muscles can be induced to grow larger by a number of factors, including hormone signaling, developmental factors, strength training, and disease. Contrary to popular belief, the number of muscle fibres cannot be increased through exercise. Instead, muscles grow larger through a combination of muscle cell growth as new protein filaments are added along with additional mass provided by undifferentiated satellite cells alongside the existing muscle cells.[87]

Biological factors such as age and hormone levels can affect muscle hypertrophy. During puberty in males, hypertrophy occurs at an accelerated rate as the levels of growth-stimulating hormones produced by the body increase. Natural hypertrophy normally stops at full growth in the late teens. As testosterone is one of the body's major growth hormones, on average, men find hypertrophy much easier to achieve than women. Taking additional testosterone or other anabolic steroids will increase muscular hypertrophy.

Muscular, spinal and neural factors all affect muscle building. Sometimes a person may notice an increase in strength in a given muscle even though only its opposite has been subject to exercise, such as when a bodybuilder finds her left biceps stronger after completing a regimen focusing only on the right biceps. This phenomenon is called cross education.[citation needed]

Atrophy

edit
 
Prisoner of war exhibiting muscle loss as a result of malnutrition.

Every day between one and two percent of muscle is broken down and rebuilt. Inactivity, malnutrition, disease, and aging can increase the breakdown leading to muscle atrophy or sarcopenia. Sarcopenia is commonly an age-related process that can cause frailty and its consequences.[88] A decrease in muscle mass may be accompanied by a smaller number and size of the muscle cells as well as lower protein content.[89]

Human spaceflight, involving prolonged periods of immobilization and weightlessness is known to result in muscle weakening and atrophy resulting in a loss of as much as 30% of mass in some muscles.[90][91] Such consequences are also noted in some mammals following hibernation.[92]

Many diseases and conditions including cancer, AIDS, and heart failure can cause muscle loss known as cachexia.[93]

Research

edit

Myopathies have been modeled with cell culture systems of muscle from healthy or diseased tissue biopsies. Another source of skeletal muscle and progenitors is provided by the directed differentiation of pluripotent stem cells.[94]

Research on skeletal muscle properties uses many techniques. Electrical muscle stimulation is used to determine force and contraction speed at different frequencies related to fiber-type composition and mix within an individual muscle group. In vitro muscle testing is used for more complete characterization of muscle properties.

The electrical activity associated with muscle contraction is measured via electromyography (EMG). Skeletal muscle has two physiological responses: relaxation and contraction. The mechanisms for which these responses occur generate electrical activity measured by EMG. Specifically, EMG can measure the action potential of a skeletal muscle, which occurs from the hyperpolarization of the motor axons from nerve impulses sent to the muscle. EMG is used in research for determining if the skeletal muscle of interest is being activated, the amount of force generated, and an indicator of muscle fatigue.[95] The two types of EMG are intra-muscular EMG and the most common, surface EMG. The EMG signals are much greater when a skeletal muscle is contracting verses relaxing. However, for smaller and deeper skeletal muscles the EMG signals are reduced and therefore are viewed as a less valued technique for measuring the activation.[96] In research using EMG, a maximal voluntary contraction (MVC) is commonly performed on the skeletal muscle of interest, to have reference data for the rest of the EMG recordings during the main experimental testing for that same skeletal muscle.[97]

Research into the development of artificial muscles includes the use of electroactive polymers.

 
Skeletal muscle cell types include: very large multinuclear muscle fiber cells; small endothelial cells that line the inside of capillary blood vessels; small fibro-adipogenic progenitor cells (FAPs) which are muscle-fiber-adjacent multipotent mesenchymal stem cells that under different conditions can differentiate into adipocytes, fibroblasts or osteocytes. Also shown are pericytes situated on the outer surface of blood capillaries where they interact with the underlying endothelial cells. In addition, satellite cells are shown that can fuse with muscle fibers and contribute new myonuclei to muscle fibers, grow into new myocytes, or support focal membrane damage repair.[98]

Mononuclear cells of skeletal muscle

edit

Nuclei present in skeletal muscle are about 50% myocyte nuclei and 50% mononuclear cell nuclei.[13] Mononuclear cells found in skeletal muscle tissue samples from mice and humans[15][99][98] can be identified by messenger RNA transcription of cell type markers. Cameron et al.[98] identified nine cell types. They include endothelial cells that line capillaries (45% of cells), fibro-adipogenic progenitors (FAPs)(20%),[100] pericytes (14%) and endothelial-like pericytes (4%). Another 9% of mononuclear cells are muscle stem cells, adjacent to muscle fiber cells. Types of lymphoid cells (such as B-cells and T-cells) (3%) and myeloid cells such as macrophages (2%) made up most of the remaining mononuclear cells of skeletal muscle.[98] In addition, Cameron et al.[98] also identified two types of myocyte cells, Type I and Type II. Each of the different types of cells in skeletal muscle was found to express different sets of genes. The median number of genes expressed in each of the nine different cell types was 1,331 genes. When a biopsy is taken from a thigh muscle, however, the biopsy contains all the different cell types. Mixed together, in a biopsy of human thigh skeletal muscle, there are 13,026 to 13,108 genes with detected expression.[101][102]

Endocrine functions of skeletal muscle

edit

As pointed out in the Introduction to this article, under different physiological conditions, subsets of 654 different proteins as well as lipids, amino acids, metabolites and small RNAs occur in the secretome of skeletal muscles.[12] As described in the Wikipedia article "List of human endocrine organs and actions", skeletal muscle is identified as an endocrine organ due to its secretion of cytokines and other peptides produced by skeletal muscle as signaling molecules. Iizuka et al.,[9] indicated that skeletal muscle is an endocrine organ because it "synthesizes and secretes multiple factors, and these muscle derived-factors exert beneficial effects on peripheral and remote organs." The altered secretomes after endurance training or resistance training as well as the secretome of sedentary muscle appear to have many effects on distant tissues.

Sedentary skeletal muscle mass affects executive mental function

edit

A study in Canada tested the effect of muscle mass on mental functions during aging. An expectation of the study was that the endocrine components of the secretome specific to skeletal muscle could protect cognitive functions. The skeletal muscle mass of arms and legs of 8,279 Canadians over the age of 65 and in average health was measured at baseline and after three years.[103] Of these individuals, 1,605 participants (19.4%) were considered to have a low skeletal muscle mass at baseline, with less than 7.30 kg/m2 for males, and less than 5.42 kg/m2 for females (levels defined as sarcopenia in Canada).

Executive mental function, memory and psychomotor speed were each measured at baseline and after three years. Executive mental function was measured with standard tests, including the ability to say the sequence 1-A, 2-B, 3-C…, to name a number of animals in one minute, and with the Stroop test.[103] The study found that those individuals with lower skeletal muscle mass at the start of the study declined in their executive mental function considerably more sharply than those with higher muscle mass. Memory, as well as psychomotor speed, on the other hand, did not correlate with skeletal muscle mass.[103] Thus, larger muscle mass, with a concomitantly larger secretome, appeared to have the endocrine function of protecting the executive mental function of individuals over the age of 65.

Walking, using skeletal muscles, affects mortality

edit

Paluch et al.[104] compared the average number of steps walked per day to the risk of mortality, both for adults over 60 years old and for adults under 60 years old. The study was a meta-analysis of 15 studies, which, combined, evaluated 47,471 adults over a period of 7 years. Individuals were divided into approximately equal quartiles. The lowest quartile averaged 3,553 steps/day, the second quartile 5,801 steps/day, the third quartile 7,842 steps/day and the fourth quartile 10,901 steps/day. The briskness of walking, adjusted for the volume of walking, did not affect mortality. However, the number of steps/day was clearly related to mortality. When risk of mortality for those over 60 years old was set at 1.0 for the lowest quartile of steps/day, the relative risk of mortality for the second, third and fourth quartiles were 0.56, 0.45, and 0.35, respectively. For those under 60 years of age, the results were less pronounced. For those under 60 years of age, with the first quartile risk of mortality set at 1.0, the second, third and fourth quartile relative risks of mortality were 0.57, 0.42 and 0.53, respectively. Thus, use of skeletal muscles in walking has a large effect, especially among older individuals, on mortality.

Skeletal muscle secretome alters with exercise

edit

Williams et al.[102] obtained biopsies of a thigh skeletal muscle (vastus lateralis muscle) of eight 23-year old, originally sedentary, Caucasian males. Biopsies were taken both before and after a six-week long endurance exercise training program. The exercise consisted of riding a stationary bicycle for one hour, five days a week for six weeks.

Of the 13,108 genes with detected expression in the muscle biopsies, 641 genes were upregulated after endurance training and 176 genes were downregulated. Of the 817 total altered genes, 531 were identified as being in the secretome by either or both of Uniprot or Exocarta, or else by studies investigating the secretome of muscle cells. Because many of the exercise-regulated genes are identified as secreted, this indicates that much of the effect of exercise has an endocrine rather than metabolic function.[102] The main pathways found to be affected by secreted exercise-regulated proteins were related to cardiac, cognitive, kidney and platelet functions.

Exercise-trained effects are mediated by epigenetic mechanisms

edit

Between 2012 and 2019, at least 25 reports indicated a major role of epigenetic mechanisms in skeletal muscle responses to exercise.[105] Epigenetic alterations often occur by adding methyl groups to cytosines in the DNA or removing methyl groups from the cytosines of DNA, especially at CpG sites. Methylations of cytosines can cause the DNA to be compacted into heterochromatin, thus inhibiting access of other molecules to the DNA.[106] Epigenetic alterations also often occur through acetylations or deacetylations of the histone tails within chromatin. DNA in the nucleus generally consists of segments of 146 base pairs of DNA wrapped around eight tightly connected histones (and each histone also has a loose tail) in a structure called a nucleosome and one segment of DNA is connected to an adjacent DNA segment on a nucleosome by linker DNA. When histone tails are acetylated, they usually cause loosening of the DNA around the nucleosome, leading to increased accessibility of the DNA.

Exercise-induced regulation of genes in muscles

edit
 
Regulation of transcription in mammals. An active enhancer regulatory region is enabled to interact with the promoter region of its target gene by formation of a chromosome loop. This can allow initiation of messenger RNA (mRNA) synthesis by RNA polymerase II (RNAP II) bound to the promoter at the transcription start site of the gene. The loop is stabilized by one architectural protein anchored to the enhancer and one anchored to the promoter, and these proteins are joined together to form a dimer (red zigzags). Specific regulatory transcription factors bind to DNA sequence motifs on the enhancer. General transcription factors bind to the promoter. When a transcription factor is activated by a signal (here indicated as phosphorylation shown by a small red star on a transcription factor on the enhancer), the enhancer is activated and can now activate its target promoter. The active enhancer is transcribed on each strand of DNA in opposite directions by bound RNAP IIs. Mediator (a complex consisting of about 26 proteins in an interacting structure) communicates regulatory signals from the enhancer DNA-bound transcription factors to the promoter.

Gene expression in muscle is largely regulated, as in tissues generally, by regulatory DNA sequences, especially enhancers. Enhancers are non-coding sequences in the genome that activate the expression of distant target genes,[107] by looping around and interacting with the promoters of their target genes[108] (see Figure "Regulation of transcription in mammals"). As reported by Williams et al.,[102] the average distance in the loop between the connected enhancers and promoters of genes is 239,000 nucleotide bases.

Exercise-induced alteration to gene expression by DNA methylation or demethylation

edit

Endurance muscle training alters muscle gene expression by epigenetic DNA methylation or de-methylation of CpG sites within enhancers.[109]

In a study by Lindholm et al.,[109] twenty-three individuals who were about 27 years old and sedentary volunteered to have endurance training on only one leg during 3 months. The other leg was used as an untrained control leg. The training consisted of one-legged knee extension training for 3 month (45 min, 4 sessions per week). Skeletal muscle biopsies from the vastus lateralis (a thigh muscle) were taken both before training began and 24 hours after the last training session from each of the legs. The endurance-trained leg, compared to the untrained leg, had significant DNA methylation changes at 4,919 sites across the genome. The sites of altered DNA methylation were predominantly in enhancers. Transcriptional analysis, using RNA sequencing, identified 4,076 differentially expressed genes.

The transcriptionally upregulated genes were associated with enhancers that had a significant decrease in DNA methylation, while transcriptionally downregulated genes were associated with enhancers that had increased DNA methylation. Increased methylation was mainly associated with genes involved in structural remodeling of the muscle and glucose metabolism. Enhancers with decreased methylation were associated with genes functioning in inflammatory or immunological processes and in transcriptional regulation.

Exercise-induced long-term alteration of gene expression by histone acetylation or deacetylation

edit
 
A nucleosome with histone tails set for transcriptional activation....DNA in the nucleus generally consists of segments of 146 base pairs of DNA wrapped around nucleosomes connected to adjacent nucleosomes by linker DNA. Nucleosomes consist of four pairs of histone proteins in a tightly assembled core region plus up to 30% of each histone remaining in a loosely organized polypeptide tail (only one tail of each pair is shown). The pairs of histones, H2A, H2B, H3 and H4, each have lysines (K) in their tails, some of which are subject to post-translational modifications consisting, usually, of acetylations [Ac] and methylations {me}. The lysines (K) are designated with a number showing their position as, for instance, (K4), indicating lysine as the 4th amino acid from the amino (N) end of the tail in the histone protein. The particular acetylations [Ac] and methylations {Me} shown are those that occur on nucleosomes close to, or at, some DNA regions undergoing transcriptional activation of the DNA wrapped around the nucleosome.

As indicated above, after exercise, epigenetic alterations to enhancers alter long-term expression of hundreds of muscle genes.[102] This includes genes producing proteins secreted into the systemic circulation, many of which may act as endocrine messengers.[102] Six sedentary, about 23 years old, Caucasian males provided vastus lateralis (a thigh muscle) biopsies before entering an exercise program (six weeks of 60-minute sessions of riding a stationary cycle, five days per week). Four days after this exercise program was completed, the expression of many genes was persistently epigentically altered. The alterations altered acetylations and deacetylations of the histone tails located in the enhancers controlling the genes with altered expression.[102]

Up-regulated genes were associated with epigenetic acetylations added at histone 3 lysine 27 (H3K27ac) of nucleosomes located at their enhancers. Down-regulated genes were associated with the removal of epigenetic acetylations at H3K27 in nucleosomes located at their enhancers (see Figure "A nucleosome with histone tails set for transcriptional activation"). Biopsies of the vastus lateralis muscle showed expression of 13,108 genes at baseline before the exercise training program. Four days after the exercise program was completed, biopsies of the same muscles showed altered gene expression, with 641 genes up-regulated and 176 genes down-regulated.[102] Williams et al. identified 599 enhancer-gene interactions, covering 491 enhancers and 268 genes (multiple enhancers were found connected to some genes), where both the enhancer and the connected target gene were coordinately either upregulated or downregulated after exercise training.[102]

See also

edit

References

edit
  1. ^ Birbrair, Alexander; Zhang, Tan; Wang, Zhong-Min; Messi, Maria Laura; Enikolopov, Grigori N.; Mintz, Akiva; Delbono, Osvaldo (21 March 2013). "Role of Pericytes in Skeletal Muscle Regeneration and Fat Accumulation". Stem Cells and Development. 22 (16): 2298–2314. doi:10.1089/scd.2012.0647. ISSN 1547-3287. PMC 3730538. PMID 23517218.
  2. ^ Betts, J. Gordon; Young, Kelly A.; Wise, James A.; Johnson, Eddie; Poe, Brandon; Kruse, Dean H.; Korol, Oksana; Johnson, Jody E.; Womble, Mark; Desaix, Peter (6 March 2013). "Interactions of Skeletal Muscles, Their Fascicle Arrangement, and Their Lever Systems". Interactions of skeletal muscles. OpenStax. Archived from the original on 23 March 2022. Retrieved 24 May 2021.
  3. ^ a b c "Structure of Skeletal Muscle | SEER Training". training.seer.cancer.gov.
  4. ^ a b c Moore, Keith L. (2018). Clinically oriented anatomy (Eighth ed.). Philadelphia: Wolters Kluwer. pp. 30–33. ISBN 9781496347213.
  5. ^ a b c d Henderson, CA; Gomez, CG; Novak, SM; Mi-Mi, L; Gregorio, CC (18 June 2017). "Overview of the Muscle Cytoskeleton". Comprehensive Physiology. 7 (3): 891–944. doi:10.1002/cphy.c160033. PMC 5890934. PMID 28640448.
  6. ^ Brainard, Jean; Gray-Wilson, Niamh; Harwood, Jessica; Karasov, Corliss; Kraus, Dors; Willan, Jane (2011). CK-12 Life Science Honors for Middle School. CK-12 Foundation. p. 451. Retrieved 18 April 2015.
  7. ^ Janssen I, Heymsfield SB, Wang ZM, Ross R (July 2000). "Skeletal muscle mass and distribution in 468 men and women aged 18-88 yr". J Appl Physiol. 89 (1): 81–8. doi:10.1152/jappl.2000.89.1.81. PMID 10904038. S2CID 9232367.
  8. ^ McCuller C, Jessu R, Callahan AL (January 2022) [Updated 25 Mar 2022]. Physiology, Skeletal Muscle. Treasure Island, FL: StatPearls Publishing. PMID 30725824. NBK537139 – via StatPearls [Internet].
  9. ^ a b Iizuka K, Machida T, Hirafuji M (2014). "Skeletal muscle is an endocrine organ". J Pharmacol Sci. 125 (2): 125–31. doi:10.1254/jphs.14r02cp. PMID 24859778.
  10. ^ Hoffmann C, Weigert C (November 2017). "Skeletal Muscle as an Endocrine Organ: The Role of Myokines in Exercise Adaptations". Cold Spring Harb Perspect Med. 7 (11): a029793. doi:10.1101/cshperspect.a029793. PMC 5666622. PMID 28389517.
  11. ^ Severinsen MC, Pedersen BK (August 2020). "Muscle-Organ Crosstalk: The Emerging Roles of Myokines". Endocr Rev. 41 (4): 594–609. doi:10.1210/endrev/bnaa016. PMC 7288608. PMID 32393961.
  12. ^ a b Florin A, Lambert C, Sanchez C, Zappia J, Durieux N, Tieppo AM, Mobasheri A, Henrotin Y (March 2020). "The secretome of skeletal muscle cells: A systematic review". Osteoarthr Cartil Open. 2 (1): 100019. doi:10.1016/j.ocarto.2019.100019. PMC 9718214. PMID 36474563.
  13. ^ a b c Von Walden F, Rea M, Mobley CB, Fondufe-Mittendorf Y, McCarthy JJ, Peterson CA, Murach KA (November 2020). "The myonuclear DNA methylome in response to an acute hypertrophic stimulus". Epigenetics. 15 (11): 1151–1162. doi:10.1080/15592294.2020.1755581. PMC 7595631. PMID 32281477.
  14. ^ Alberts, Bruce; Johnson, Alexander; Lewis, Julian; Raff, Martin; Roberts, Keith; Walter, Peter (2002). Genesis, Modulation, and Regeneration of Skeletal Muscle. Garland Science.
  15. ^ a b Giordani L, He GJ, Negroni E, Sakai H, Law JY, Siu MM, Wan R, Corneau A, Tajbakhsh S, Cheung TH, Le Grand F (May 2019). "High-Dimensional Single-Cell Cartography Reveals Novel Skeletal Muscle-Resident Cell Populations". Mol Cell. 74 (3): 609–621.e6. doi:10.1016/j.molcel.2019.02.026. PMID 30922843.
  16. ^ Introduction. Morgan & Claypool Life Sciences. 2011.
  17. ^ Tigner, A.; Ibrahim, S. A.; Murray, I. (2022). "Histology, White Blood Cell". StatPearls. PMID 33085295.
  18. ^ Ying Ji; Dympna Gallagher (2014). "3. Body composition assessment of the critically ill patient". In Faber, Peter; Siervo, Mario (eds.). Nutrition in Critical Care. New York: Cambridge University Press. p. 22. ISBN 978-1-107-66901-7. Retrieved 17 February 2023.
  19. ^ a b "Muscle Groups | SEER Training". training.seer.cancer.gov. Retrieved 17 May 2021.
  20. ^ "What is the strongest muscle in the human body?". Library of Congress. Retrieved 17 May 2021.
  21. ^ Muller, Martin N.; Wrangham, Richard W.; Pilbeam, David R., eds. (2017). "11. The Evolution of the Human Mating System". Chimpanzees and Human Evolution. Cambridge, Massachusetts: Harvard University Press. p. 397. ISBN 9780674967953. Retrieved 17 February 2023.
  22. ^ Klein, CS; Marsh, GD; Petrella, RJ; Rice, CL (July 2003). "Muscle fiber number in the biceps brachii muscle of young and old men". Muscle & Nerve. 28 (1): 62–8. doi:10.1002/mus.10386. PMID 12811774. S2CID 20508198.
  23. ^ Cho, CH; Lee, KJ; Lee, EH (August 2018). "With the greatest care, stromal interaction molecule (STIM) proteins verify what skeletal muscle is doing". BMB Reports. 51 (8): 378–387. doi:10.5483/bmbrep.2018.51.8.128. PMC 6130827. PMID 29898810.
  24. ^ a b Prasad, V; Millay, DP (8 May 2021). "Skeletal muscle fibers count on nuclear numbers for growth". Seminars in Cell & Developmental Biology. 119: 3–10. doi:10.1016/j.semcdb.2021.04.015. PMC 9070318. PMID 33972174. S2CID 234362466.
  25. ^ a b c Snijders, T; Aussieker, T; Holwerda, A; Parise, G; van Loon, LJC; Verdijk, LB (July 2020). "The concept of skeletal muscle memory: Evidence from animal and human studies". Acta Physiologica. 229 (3): e13465. doi:10.1111/apha.13465. PMC 7317456. PMID 32175681.
  26. ^ Quarta, M; Cromie, M; Chacon, R (20 June 2017). "Bioengineered constructs combined with exercise enhance stem cell-mediated treatment of volumetric muscle loss". Nature Communications. 8: 15613. Bibcode:2017NatCo...815613Q. doi:10.1038/ncomms15613. PMC 5481841. PMID 28631758.
  27. ^ a b Charvet, B; Ruggiero, F; Le Guellec, D (April 2012). "The development of the myotendinous junction. A review". Muscles, Ligaments and Tendons Journal. 2 (2): 53–63. PMC 3666507. PMID 23738275.
  28. ^ a b Martini, Frederic H.; Timmons, Michael J.; Tallitsch, Robert B. (2008). Human Anatomy (6 ed.). Benjamin Cummings. pp. 251–252. ISBN 978-0-321-50042-7.
  29. ^ a b c d Lieber, Richard L. (2002) Skeletal muscle structure, function, and plasticity. Wolters Kluwer Health.
  30. ^ Ziser, Stephen. "&Muscle Cell Anatomy & Function" (PDF). www.austincc.edu. Archived (PDF) from the original on 23 September 2015. Retrieved 12 February 2015.
  31. ^ a b c d Tortora, Gerard J. (2012). Principles of anatomy & physiology (13th ed.). Hoboken, NJ: Wiley. p. 372. ISBN 9780470646083.
  32. ^ a b c d Saladin, Kenneth S. (2011). Human anatomy (3rd ed.). New York: McGraw-Hill. p. 265. ISBN 9780071222075.
  33. ^ Betts, J. Gordon; Young, Kelly A.; Wise, James A.; Johnson, Eddie; Poe, Brandon; Kruse, Dean H.; Korol, Oksana; Johnson, Jody E.; Womble, Mark; Desaix, Peter (6 March 2013). Types of muscle fibers. OpenStax. Retrieved 17 June 2021.
  34. ^ a b c d e f MacIntosh, Brian R.; Gardiner, Phillip F.; McComas, Alan J. (2006). Skeletal Muscle: Form and Function. Human Kinetics. ISBN 978-0-7360-4517-9.
  35. ^   This article incorporates text available under the CC BY 4.0 license. Betts, J Gordon; Desaix, Peter; Johnson, Eddie; Johnson, Jody E; Korol, Oksana; Kruse, Dean; Poe, Brandon; Wise, James; Womble, Mark D; Young, Kelly A (14 May 2023). Anatomy & Physiology. Houston: OpenStax CNX. 10.5 Types of muscle fibres. ISBN 978-1-947172-04-3.
  36. ^ a b "Muscle fiber type". About.com. Sports Medicine. Archived from the original on 21 November 2007. Retrieved 27 November 2007.
  37. ^ MacIntosh, Brian R. (2006). Skeletal muscle : form and function (2nd ed.). Champaign, IL: Human Kinetics. p. 274. ISBN 978-0-7360-4517-9.
  38. ^ a b Johnson, M.A.; Polgar, J.; Weightman, D.; Appleton, D. (1973). "Data on the distribution of fibre types in thirty-six human muscles. An autopsy study". Journal of the Neurological Sciences. 18 (1): 111–129. doi:10.1016/0022-510x(73)90023-3. PMID 4120482.
  39. ^ a b Schiaffino, S; Reggiani, C (October 2011). "Fiber types in mammalian skeletal muscles". Physiological Reviews. 91 (4): 1447–531. doi:10.1152/physrev.00031.2010. hdl:11577/2526092. PMID 22013216.
  40. ^ Michael Yessis (2006). Build A Better Athlete. Ultimate Athlete Concepts. ISBN 978-1-930546-78-3.
  41. ^ a b Smerdu V, Karsch-Mizrachi I, Campione M, Leinwand L, Schiaffino, S (December 1994). "Type IIx myosin heavy chain transcripts are expressed in type IIb fibers of human skeletal muscle". The American Journal of Physiology. 267 (6 Pt 1): C1723–8. doi:10.1152/ajpcell.1994.267.6.C1723. PMID 7545970.
  42. ^ Pette, D; Staron, RS (15 September 2000). "Myosin isoforms, muscle fiber types, and transitions". Microscopy Research and Technique. 50 (6): 500–9. doi:10.1002/1097-0029(20000915)50:6<500::AID-JEMT7>3.0.CO;2-7. PMID 10998639. S2CID 7820419.
  43. ^ Staron, Robert S.; Johnson, Peter (November 1993). "Myosin polymorphism and differential expression in adult human skeletal muscle". Comparative Biochemistry and Physiology B. 106 (3): 463–475. doi:10.1016/0305-0491(93)90120-T. PMID 8281747.
  44. ^ Buchthal, F.; Schmalbruch, H. (August 1970). "Contraction times and fibre types in intact human muscle". Acta Physiologica Scandinavica. 79 (4): 435–452. doi:10.1111/j.1748-1716.1970.tb04744.x. PMID 5472111.
  45. ^ Garnett, R.A.; O'Donovan, M.J.; Stephens, J.A.; Taylor, A. (February 1979). "Motor unit organization of human medial gastrocnemius". The Journal of Physiology. 287 (1): 33–43. doi:10.1113/jphysiol.1979.sp012643. PMC 1281479. PMID 430414.[permanent dead link]
  46. ^ Magazine, Viviane Callier, Quanta. "Too Small for Big Muscles, Tiny Animals Use Springs". Scientific American. Retrieved 13 December 2022.{{cite web}}: CS1 maint: multiple names: authors list (link)
  47. ^ a b Simoneau, Jean-Aimé; Bouchard, Claude (August 1995). "Genetic determinism of fiber type proportion in human skeletal muscle". The FASEB Journal. 9 (11): 1091–1095. doi:10.1096/fasebj.9.11.7649409. ISSN 0892-6638. PMID 7649409. S2CID 9613549.
  48. ^ a b Sieck, Gary C. (1 January 2001). "Highlighted Topics series: Plasticity in Skeletal, Cardiac, and Smooth Muscle". Journal of Applied Physiology. 90 (1): 1. doi:10.1152/jappl.2001.90.1.1. ISSN 8750-7587.
  49. ^ Hamilton, Marc T.; Booth, Frank W. (1 January 2000). "Skeletal muscle adaptation to exercise: a century of progress". Journal of Applied Physiology. 88 (1): 327–331. doi:10.1152/jappl.2000.88.1.327. ISSN 8750-7587. PMID 10642397. S2CID 7024153.
  50. ^ a b "Fiber polymorphism in skeletal muscles of the American lobster, Homarus americanus: continuum between slow-twitch (S1) and slow-tonic (S2) fibers". journals.biologists.com. Retrieved 13 December 2022.
  51. ^ a b Callister, Robert J.; Pierce, Patricia A.; McDonagh, Jennifer C.; Stuart, Douglas G. (April 2005). "Slow-tonic muscle fibers and their potential innervation in the turtle, Pseudemys (Trachemys)scripta elegans". Journal of Morphology. 264 (1): 62–74. doi:10.1002/jmor.10318. ISSN 0362-2525. PMID 15732049. S2CID 36961922.
  52. ^ Sokoloff, Alan J.; Li, Haiyan; Burkholder, Thomas J. (August 2007). "Limited expression of slow tonic myosin heavy chain in human cranial muscles". Muscle & Nerve. 36 (2): 183–189. doi:10.1002/mus.20797. PMC 3816747. PMID 17486578.
  53. ^ a b "Expression of multiple slow myosin heavy chain genes reveals a diversity of zebrafish slow twitch muscle fibres with differing requirements for Hedgehog and Prdm1 activity". journals.biologists.com. Retrieved 13 December 2022.
  54. ^ O'Neill, Matthew C.; Umberger, Brian R.; Holowka, Nicholas B.; Larson, Susan G.; Reiser, Peter J. (11 July 2017). "Chimpanzee super strength and human skeletal muscle evolution". Proceedings of the National Academy of Sciences. 114 (28): 7343–7348. Bibcode:2017PNAS..114.7343O. doi:10.1073/pnas.1619071114. ISSN 0027-8424. PMC 5514706. PMID 28652350.
  55. ^ "Non Conservation of Function for the Evolutionarily Conserved Prdm1 Protein in the Control of the Slow Twitch Myogenic Program in the Mouse Embryo". academic.oup.com. Retrieved 13 December 2022.
  56. ^ Ronnestad, H.V (2020). "Effects of temperature on feeding and digestive processes in fish". Temperature Medical Physiology and Beyond. 7 (4): 307–320. doi:10.1080/23328940.2020.1765950. PMC 7678922. PMID 33251280.
  57. ^ McDougall, Christopher (2009). Born to Run: a hidden tribe, superathletes, and the Greatest Race Never Seen.
  58. ^ Saladin, Kenneth S. (2010). Anatomy and Physiology (3rd ed.). New York: Watnick. pp. 405–406. ISBN 9780072943689.
  59. ^ a b c Sweeney, Lauren (1997). Basic Concepts in Embryology: A Student's Survival Guide (1st Paperback ed.). McGraw-Hill Professional.
  60. ^ MacIntosh, Brian R. (2006). Skeletal muscle : form and function (2nd ed.). Champaign, IL: Human Kinetics. pp. 63–64. ISBN 978-0-7360-4517-9.
  61. ^ Murach, KA; Fry, CS; Kirby, TJ; Jackson, JR; Lee, JD; White, SH; Dupont-Versteegden, EE; McCarthy, JJ; Peterson, CA (1 January 2018). "Starring or Supporting Role? Satellite Cells and Skeletal Muscle Fiber Size Regulation". Physiology. 33 (1): 26–38. doi:10.1152/physiol.00019.2017. PMC 5866409. PMID 29212890.
  62. ^ Grube, L; Dellen, R; Kruse, F (2 February 2018). "Mining the Secretome of C2C12 Muscle Cells: Data Dependent Experimental Approach To Analyze Protein Secretion Using Label-Free Quantification and Peptide Based Analysis". Journal of Proteome Research. 17 (2): 879–890. doi:10.1021/acs.jproteome.7b00684. PMID 29322779.
  63. ^ Pedersen, B. K. (2013). "Muscle as a Secretory Organ". Comprehensive Physiology. Vol. 3. pp. 1337–62. doi:10.1002/cphy.c120033. ISBN 9780470650714. PMID 23897689.
  64. ^ Lee, JH; Jun, HS (2019). "Role of Myokines in Regulating Skeletal Muscle Mass and Function". Frontiers in Physiology. 10: 42. doi:10.3389/fphys.2019.00042. PMC 6363662. PMID 30761018.
  65. ^ "Introduction to the Muscular System | SEER Training". training.seer.cancer.gov.
  66. ^ "1.5 Homeostasis - Anatomy and Physiology | OpenStax". openstax.org. 25 April 2013. Retrieved 25 June 2021.
  67. ^ Costanzo, Linda S. (2002). Physiology (2nd ed.). Philadelphia: Saunders. p. 23. ISBN 0-7216-9549-3.
  68. ^ Calderón, Juan C.; Bolaños, Pura; Caputo, Carlo (24 January 2014). "The excitation–contraction coupling mechanism in skeletal muscle". Biophysical Reviews. 6 (1): 133–160. doi:10.1007/s12551-013-0135-x. ISSN 1867-2450. PMC 5425715. PMID 28509964.
  69. ^ Heydemann, A (20 June 2018). "Skeletal Muscle Metabolism in Duchenne and Becker Muscular Dystrophy-Implications for Therapies". Nutrients. 10 (6): 796. doi:10.3390/nu10060796. PMC 6024668. PMID 29925809.
  70. ^ Heymsfield, SB; Gallagher, D; Kotler, DP; Wang, Z; Allison, DB; Heshka, S (2002). "Body-size dependence of resting energy expenditure can be attributed to nonenergetic homogeneity of fat-free mass". American Journal of Physiology. Endocrinology and Metabolism. 282 (1): E132–E138. doi:10.1152/ajpendo.2002.282.1.e132. PMID 11739093. S2CID 10257328.
  71. ^ McGinnis, Peter M. (2013). Biomechanics of Sport and Exercise (3rd ed.). Champaign, IL: Human Kinetics. ISBN 978-0-7360-7966-2.
  72. ^ Quoted from National Skeletal Muscle Research Center; UCSD, Muscle Physiology Home Page – Skeletal Muscle Architecture Archived 18 July 2014 at the Wayback Machine, Effect of Muscle Architecture on Muscle Function
  73. ^ "9.6 Forces and Torques in Muscles and Joints - College Physics | OpenStax". openstax.org. 21 June 2012. Retrieved 15 May 2021.
  74. ^ Barry, D. T. (1992). "Vibrations and sounds from evoked muscle twitches". Electromyogr Clin Neurophysiol. 32 (1–2): 35–40. PMID 1541245.
  75. ^ [1], Peak Performance – Endurance training: understanding your slow twitch muscle fibers will boost performance
  76. ^ Gonyea WJ, Sale DG, Gonyea FB, Mikesky A (1986). "Exercise induced increases in muscle fiber number". Eur J Appl Physiol Occup Physiol. 55 (2): 137–141. doi:10.1007/BF00714995. PMID 3698999. S2CID 29191826.
  77. ^ Jansson E, Kaijser L (July 1977). "Muscle adaptation to extreme endurance training in man". Acta Physiol. Scand. 100 (3): 315–24. doi:10.1111/j.1748-1716.1977.tb05956.x. PMID 144412.
  78. ^ Gollnick PD, Armstrong RB, Saubert CW, Piehl K, Saltin B (September 1972). "Enzyme activity and fiber composition in skeletal muscle of untrained and trained men". J Appl Physiol. 33 (3): 312–9. doi:10.1152/jappl.1972.33.3.312. PMID 4403464.
  79. ^ Schantz P, Henriksson J, Jansson E (April 1983). "Adaptation of human skeletal muscle to endurance training of long duration". Clinical Physiology. 3 (2): 141–51. doi:10.1111/j.1475-097x.1983.tb00685.x. PMID 6682735.
  80. ^ Monster AW, Chan H, O'Connor D (April 1978). "Activity patterns of human skeletal muscles: relation to muscle fiber type composition". Science. 200 (4339): 314–7. doi:10.1126/science.635587. PMID 635587.
  81. ^ Pattengale PK, Holloszy JO (September 1967). "Augmentation of skeletal muscle myoglobin by a program of treadmill running". Am. J. Physiol. 213 (3): 783–5. doi:10.1152/ajplegacy.1967.213.3.783. PMID 6036801.
  82. ^ Nielsen, OB; Paoli, F; Overgaard, K (2001). "Protective effects of lactic acid on force production in rat skeletal muscle". Journal of Physiology. 536 (1): 161–166. doi:10.1111/j.1469-7793.2001.t01-1-00161.x. PMC 2278832. PMID 11579166.
  83. ^ Robergs, R; Ghiasvand, F; Parker, D (2004). "Biochemistry of exercise-induced metabolic acidosis". Am J Physiol Regul Integr Comp Physiol. 287 (3): R502–516. doi:10.1152/ajpregu.00114.2004. PMID 15308499. S2CID 2745168.
  84. ^ Wang, Y; Jardine, MJ (November 2011). "Benefits of exercise training in patients receiving haemodialysis: a systematic review and meta-analysis". British Journal of Sports Medicine. 45 (14): 1165–6. doi:10.1136/bjsports-2011-090558. PMID 21989854. S2CID 27583398.
  85. ^ "Overview of Movement Disorders - Brain, Spinal Cord, and Nerve Disorders". MSD Manual Consumer Version. Retrieved 24 June 2021.
  86. ^ Dumé, Belle (18 May 2007). "'Muscle noise' could reveal diseases' progression". NewScientist.com news service.
  87. ^ Poole, RM, ed. (1986). The Incredible Machine. Washington, DC: National Geographic Society. pp. 307–311. ISBN 978-0-87044-621-4.
  88. ^ Cruz-Jentoft, AJ; Sayer, AA (29 June 2019). "Sarcopenia". Lancet. 393 (10191): 2636–2646. doi:10.1016/S0140-6736(19)31138-9. PMID 31171417. S2CID 208792618.
  89. ^ Fuster G, Busquets S, Almendro V, López-Soriano FJ, Argilés JM (2007). "Antiproteolytic effects of plasma from hibernating bears: a new approach for muscle wasting therapy?". Clin Nutr. 26 (5): 658–661. doi:10.1016/j.clnu.2007.07.003. PMID 17904252.
  90. ^ Roy RR, Baldwin KM, Edgerton VR (1996). "Response of the neuromuscular unit to spaceflight: What has been learned from the rat model". Exerc. Sport Sci. Rev. 24: 399–425. doi:10.1249/00003677-199600240-00015. PMID 8744257. S2CID 44574997.
  91. ^ "NASA Muscle Atrophy Research (MARES) Website". Archived from the original on 4 May 2010.
  92. ^ Lohuis TD, Harlow HJ, Beck TD (2007). "Hibernating black bears (Ursus americanus) experience skeletal muscle protein balance during winter anorexia". Comp. Biochem. Physiol. B. 147 (1): 20–28. doi:10.1016/j.cbpb.2006.12.020. PMID 17307375.
  93. ^ Ebner N, Springer J, Kalantar-Zadeh K, Lainscak M, Doehner W, Anker SD, von Haehling S (July 2013). "Mechanism and novel therapeutic approaches to wasting in chronic disease". Maturitas. 75 (3): 199–206. doi:10.1016/j.maturitas.2013.03.014. PMID 23664695. S2CID 42148927.[permanent dead link]
  94. ^ Chal J, Oginuma M, Al Tanoury Z, Gobert B, Sumara O, Hick A, Bousson F, Zidouni Y, Mursch C, Moncuquet P, Tassy O, Vincent S, Miyanari A, Bera A, Garnier JM, Guevara G, Hestin M, Kennedy L, Hayashi S, Drayton B, Cherrier T, Gayraud-Morel B, Gussoni E, Relaix F, Tajbakhsh S, Pourquié O (August 2015). "Differentiation of pluripotent stem cells to muscle fiber to model Duchenne muscular dystrophy". Nature Biotechnology. 33 (9): 962–969. doi:10.1038/nbt.3297. PMID 26237517. S2CID 21241434. Closed access icon 
  95. ^ Cè, E; Rampichini, S; Limonta, E; Esposito, F (10 December 2013). "Fatigue effects on the electromechanical delay components during the relaxation phase after isometric contraction". Acta Physiologica. 211 (1): 82–96. doi:10.1111/apha.12212. PMID 24319999. S2CID 34744926.
  96. ^ Xu, Q; Quan, Y; Yang, L; He, J (January 2013). "An adaptive algorithm for the determination of the onset and offset of muscle contraction by EMG signal processing". IEEE Transactions on Neural Systems and Rehabilitation Engineering. 21 (1): 65–73. doi:10.1109/TNSRE.2012.2226916. PMID 23193462. S2CID 25169061.
  97. ^ Milder, DA; Sutherland, EJ; Gandevia, SC; McNulty, PA (2014). "Sustained maximal voluntary contraction produces independent changes in human motor axons and the muscle they innervate". PLOS ONE. 9 (3): e91754. Bibcode:2014PLoSO...991754M. doi:10.1371/journal.pone.0091754. PMC 3951451. PMID 24622330.
  98. ^ a b c d e Cameron A, Wakelin G, Gaulton N, Young LV, Wotherspoon S, Hodson N, Lees MJ, Moore DR, Johnston AP (December 2022). "Identification of underexplored mesenchymal and vascular-related cell populations in human skeletal muscle". Am J Physiol Cell Physiol. 323 (6): C1586–C1600. doi:10.1152/ajpcell.00364.2022. PMID 36342160. S2CID 253383236.
  99. ^ Rubenstein AB, Smith GR, Raue U, Begue G, Minchev K, Ruf-Zamojski F, Nair VD, Wang X, Zhou L, Zaslavsky E, Trappe TA, Trappe S, Sealfon SC (January 2020). "Single-cell transcriptional profiles in human skeletal muscle". Sci Rep. 10 (1): 229. Bibcode:2020NatSR..10..229R. doi:10.1038/s41598-019-57110-6. PMC 6959232. PMID 31937892.
  100. ^ Biferali B, Proietti D, Mozzetta C, Madaro L (2019). "Fibro-Adipogenic Progenitors Cross-Talk in Skeletal Muscle: The Social Network". Front Physiol. 10: 1074. doi:10.3389/fphys.2019.01074. PMC 6713247. PMID 31496956.
  101. ^ "The skeletal muscle-specific proteome". The Human Protein Atlas.
  102. ^ a b c d e f g h i Williams K, Carrasquilla GD, Ingerslev LR, Hochreuter MY, Hansson S, Pillon NJ, Donkin I, Versteyhe S, Zierath JR, Kilpeläinen TO, Barrès R (November 2021). "Epigenetic rewiring of skeletal muscle enhancers after exercise training supports a role in whole-body function and human health". Mol Metab. 53: 101290. doi:10.1016/j.molmet.2021.101290. PMC 8355925. PMID 34252634.
  103. ^ a b c Tessier AJ, Wing SS, Rahme E, Morais JA, Chevalier S (July 2022). "Association of Low Muscle Mass With Cognitive Function During a 3-Year Follow-up Among Adults Aged 65 to 86 Years in the Canadian Longitudinal Study on Aging". JAMA Netw Open. 5 (7): e2219926. doi:10.1001/jamanetworkopen.2022.19926. PMC 9250053. PMID 35796211.
  104. ^ Paluch AE, Bajpai S, Bassett DR, Carnethon MR, Ekelund U, Evenson KR, Galuska DA, Jefferis BJ, Kraus WE, Lee IM, Matthews CE, Omura JD, Patel AV, Pieper CF, Rees-Punia E, Dallmeier D, Klenk J, Whincup PH, Dooley EE, Pettee Gabriel K, Palta P, Pompeii LA, Chernofsky A, Larson MG, Vasan RS, Spartano N, Ballin M, Nordström P, Nordström A, Anderssen SA, Hansen BH, Cochrane JA, Dwyer T, Wang J, Ferrucci L, Liu F, Schrack J, Urbanek J, Saint-Maurice PF, Yamamoto N, Yoshitake Y, Newton RL Jr, Yang S, Shiroma EJ, Fulton JE, et al. (Steps for Health Collaborative) (March 2022). "Daily steps and all-cause mortality: a meta-analysis of 15 international cohorts". Lancet Public Health. 7 (3): e219–e228. doi:10.1016/S2468-2667(21)00302-9. PMC 9289978. PMID 35247352.
  105. ^ Widmann M, Nieß AM, Munz B (April 2019). "Physical Exercise and Epigenetic Modifications in Skeletal Muscle". Sports Med. 49 (4): 509–523. doi:10.1007/s40279-019-01070-4. PMID 30778851. S2CID 73481438.
  106. ^ Rose NR, Klose RJ (December 2014). "Understanding the relationship between DNA methylation and histone lysine methylation". Biochimica et Biophysica Acta (BBA) - Gene Regulatory Mechanisms. 1839 (12): 1362–1372. doi:10.1016/j.bbagrm.2014.02.007. PMC 4316174. PMID 24560929.
  107. ^ Panigrahi A, O'Malley BW (April 2021). "Mechanisms of enhancer action: the known and the unknown". Genome Biol. 22 (1): 108. doi:10.1186/s13059-021-02322-1. PMC 8051032. PMID 33858480.
  108. ^ Marsman J, Horsfield JA (2012). "Long distance relationships: enhancer-promoter communication and dynamic gene transcription". Biochim Biophys Acta. 1819 (11–12): 1217–27. doi:10.1016/j.bbagrm.2012.10.008. PMID 23124110.
  109. ^ a b Lindholm ME, Marabita F, Gomez-Cabrero D, Rundqvist H, Ekström TJ, Tegnér J, Sundberg CJ (December 2014). "An integrative analysis reveals coordinated reprogramming of the epigenome and the transcriptome in human skeletal muscle after training". Epigenetics. 9 (12): 1557–69. doi:10.4161/15592294.2014.982445. PMC 4622000. PMID 25484259.