Myosin concentration, muscle

In addition to the displacement of caldesmon, smooth muscle cell contraction requires kinase-induced phosphorylation of myosin. Smooth muscle has a unique type of myosin filament called p-light chains which are the target (substrate) for MLCK, but MLCK is only active when complexed with CaCM. Myosin light chain phosphatase reverses the PKA-mediated process and when cytosolic calcium ion concentration falls, CDM is released from CaCM and re-associates with the actin. The central role of calcium-calmodulin in smooth muscle contraction is shown in Figure 7.4. 

In either case, a reservoir of a solution with a higher concentration of precipitant is present in the same compartment. Water evaporates from the samples into the larger reservoir, concentrating the protein and causing its crystallization. Crystals grow slightly better in a spacecraft than on Earth. ° ° Some proteins, notably myosin from muscle, crystallize well only after reductive methylation of all lysine side chains to dimethyllysine with formaldehyde and sodium borohydride (Eq. 3-34). ... 

Estimates of the levels of the major protein components of smooth and skeletal muscles have been compiled by Hartshorne (1987). The concentrations of myosin, actin, and TM for arterial and nonarterial smooth muscles are estimated to be approximately 56 xM, 1.6 mM, 0.27 mM and 56 jjlM, 0.87 mM, 0.15 mM, respectively. In skeletal muscle, the corresponding concentrations are approximately 0.18, 0.7, and 0.1 mM. Thus in smooth muscles the myosin concentration is significantly reduced, whereas the actin and TM concentrations are elevated relative to those of skeletal muscle. In the present context the important point is that the molar ratio ( 1.2 7) of TM to actin monomers is more than adequate to fully saturate the available TM binding sites on F-actin (one per seven actin monomers). 

The organisation of thick and thin filaments in the smooth muscle cells differs markedly from that in the skeletal muscle. The myosin concentration in smooth muscle is about 20% of that in skeletal muscle (Murphy et al. 1974) and based on electron microscopy the thick myosin filaments appear to be surrounded by approximately 15 actin filaments (Devine and Somlyo 1971, Somlyo 1980). At present no sarcomere" equivalents have been identified in smooth muscle, but in order to enable shortening over... 

In the presence of calcium, the primary contractile protein, myosin, is phosphorylated by the myosin light-chain kinase initiating the subsequent actin-activation of the myosin adenosine triphosphate activity and resulting in muscle contraction. Removal of calcium inactivates the kinase and allows the myosin light chain to dephosphorylate myosin which results in muscle relaxation. Therefore the general biochemical mechanism for the muscle contractile process is dependent on the avaUabUity of a sufficient intraceUular calcium concentration. 

The major relaxing transmitters are those that elevate the cAMP or cGMP concentration (Fig. 3). Adenosine stimulates the activity of cAMP kinase. The next step is not clear, but evidence has been accumulated that cAMP kinase decreases the calcium sensitivity of the contractile machinery. In vitro, cAMP kinase phosphorylated MLCK and decreased thereby the affinity of MLCK for calcium-calmodulin. However, this regulation does not occur in intact smooth muscle. Possible other substrate candidates for cAMP kinase are the heat stable protein HSP 20, (A heat stable protein of 20 kDa that is phosphorylated by cGMP kinase. It has been postulated that phospho-HSP 20 interferes with the interaction between actin and myosin allowing thereby smooth muscle relaxation without dephosphorylation of the rMLC.) Rho A and MLCP that are phosphorylated also by cGMP kinase I (Fig. 3). 

The regulation of smooth muscle and nonmuscle myosin-II is substantially different from the mechanism described above for two important reasons. First, there is no troponin in smooth muscle and nonmuscle cells. Second, although the rate of hydrolysis of ATP by these myosins is low in the presence of physiological concentrations of Mg % the addition of actin does not necessarily result in the stimulation of ATP hydrolysis by smooth muscle or nonmuscle myosin-II. These observations suggest the presence of a unique mechanism for Ca " regulation in smooth and nonmuscle cells, and that these myosins require an activation process before actin can stimulate ATP hydrolysis. 

In resting muscle the high concentration of ADP does not decrease the proton gradient effectively and the high membrane potential slows electron transport. ADP, formed when ATP is hydrolyzed by myosin ATPase during contraction, may stimulate electron transport. However, the concentration of ATP (largely as its Mg salt) is buffered by its readily reversible formation from creatine phosphate catalyzed in the intermembrane space, and in other cell compartments, by the various isoenzymes of creatine kinase (reviewed by Walliman et al., 1992). 

The structure of the contractile apparatus of smooth muscle at the next higher level is also characteristically different from other muscles. The concentrations of actin and myosin in smooth muscle are about three times higher for actin and four times lower for myosin than in skeletal muscle. Correspondingly, in smooth muscle the ratio of the numbers of moles of actin to moles of myosin, and the ratio of the number of actin filaments to those of myosin filaments, are about 12 times larger than for other muscles. Thus, the arrangements of the two sets of filaments are bound to be quite different just on the basis of numbers of actin and myosin... 

Of the several kinase activities which are important in smooth muscle, myosin light chain kinase, MLCK, is the one responsible for activation of the actin-myosin system to in vivo levels. MLCK is present in the other nonmuscle cell types which have the actin-myosin contractile system and all of these are probably activated in a manner similar to smooth muscle rather than by way of the Ca -troponin mechanism of striated muscle. MLCK from smooth muscle is about 130 kDa and is rather variable in shape. It is present in smooth muscle in 1-4 pM concentrations and binds with an equally high affinity to both myosin and actin. Thus, most MLCK molecules are bound to actin. Myosin light chain serine-19 is the primary target of smooth muscle myosin light chain kinase. 

One should note overall, that while some of these suggested mechanisms may in the future prove to have a role in the control of smooth muscle contraction, in chemically skinned preparations maximum force development follows activation by the MLCK active subunit in extremely low Ca " ion concentrations. The conclusion can hardly be avoided that phosphorylation alone is sufficient for activation, and if another mechanism is involved, it is not necessary for the initial genesis of force. If such mechanisms are operative, then they might be expected to run in parallel or consequent to myosin phosphorylation. A possible example of this category of effect is that a GTP-dependent process (G-protein) shifts the force vs. Ca ion concentration relationship to lower Ca ion concentrations. This kind of mechanism calls attention to the divergence of signals along the intracellular control pathways. 

There is nothing in Equations 1-8 which is an all-or-none situation. There are no positive feedback loops which might cause some kind of flip-flop of states of operation of the system. There are some possibilities for saturation phenomena but all relationships are graded. Overall, transient or steady-state, the changes of concentration of P-myosin are continuous, monotonic functions of the intracellular Ca ion concentration. On this basis it is more appropriate to say that smooth muscle contraction is modulated rather than triggered by Ca ion. 

Once the intracellular Ca " concentration begins to rise, calmodulin-calcium binding also rises and MLCK, which is dependent on calmodulin activation, rises in turn. The next step in this cascade is the phosphorylation of myosin. Finally, the phosphorylation of myosin results in the activation of the crossbridges and the accompanying transduction of ATP energy into mechanical work. Despite its differences in regulation, smooth muscle behaves mechanically much like other muscles. 

All these experiments were carried out with actin and myosin in solution, either using moderate ionic strength and low actin concentrations (Lymn and Taylor, 1971) or using low ionic strength and high actin concentrations (Stem et al., 1979). However, in muscle both the actin concentration and the ionic strength are high. To confirm these models, these same experiments need to be carried out in muscle fibers. 

In the absence of ATP, myosin crossbridges are unable to release the actin. As a result, the sarcomeres, and therefore the muscle, remain contracted. This phenomenon is referred to as rigor mortis. Following death, the concentration of intracellular calcium increases. This calcium allows the... 

It simulates the activity of myosin ATPase, which results in contraction of the muscle (i.e. increased cross-bridge cycling). This increases the rate of utilisation of ATP and hence increases the concentration of ADP. 

Figure 9.25 Control of the Krebs q/cle and myosin-ATPase by direct effects of Ccf ions and the resultant effects on electron transfer and oxidative phosphorylation in muscle. The stimulation of the Krebs cycle by ions results in an increase in the NADH/NAD concentration ratio, which stimulates electron transfer. The stimulation of myosin-ATPase by Ca lowers the ATP/ADP concentration ratio, which also stimulates electron transfer. The Ca ions are released from the sarcoplasmic reticulum in muscle in response to nervous stimulation. In addition, generation of ADP by myosin ATPase increases the ADP concentration, which stimulates the cycle. Note that a lack of oxygen will prevent generation of ATP (Chapter 13).

These messengers also play a role in regulating contraction of myometrium, which consists of smooth muscle fibres. Contraction is controlled by increases in the concentration of cytosolic Ca ions. Prostaglandins activate Ca ion channels in the plasma membrane of the fibres oxytocin activates release of Ca from intracellular stores. The increase in concentration of Ca ions leads to activation of myosin light-chain kinase which leads to crossbridge cycling and contraction (as described in Chapter 22 Figure 22.12). 

---