Novel Sensors of the Regulatory Switch on the Regulatory Light Chain of Smooth Muscle Myosin

Mazhari, Sam; Selser, Curtis T.; Cremo, Christine R.

doi:10.1074/jbc.m407062200

Cited by 21 publications

(26 citation statements)

References 60 publications

(60 reference statements)

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“…Studies with calcium-regulated scallop HMM show similar trends induced by calcium binding (12). The two RLC can be cross-linked in the unphosphorylated, but not phosphorylated smooth HMM (13), and phosphorylation causes a large structural rearrangement of the RLC Nterminus (14) to a more exposed and nonpolar environment (15) consistent with recent EPR studies (16). Cryo-EM image reconstructions of nucleotide-bound smooth HMM ordered on a lipid monolayer have visualized contacts between the two CDs that are abolished upon phosphorylation (17,18).…”

supporting

confidence: 74%

“…But it is clear that nucleotide at the active site biases the structure more toward an OFF state. Mazhari et al (15) showed that the environment of the RLC N-terminus (phosphorylated or not) in the absence of nucleotides was intermediate between the nucleotide bound unphosphorylated and phosphorylated states in HMM. The fact that we see little effect of phosphorylation on the dynamics in the absence of nucleotides is consistent with the general trend of the Mazhari et al data (15).…”

Section: Structural Models Of Heavy Meromyosin: Implications Of Dynammentioning

confidence: 99%

“…Mazhari et al (15) showed that the environment of the RLC N-terminus (phosphorylated or not) in the absence of nucleotides was intermediate between the nucleotide bound unphosphorylated and phosphorylated states in HMM. The fact that we see little effect of phosphorylation on the dynamics in the absence of nucleotides is consistent with the general trend of the Mazhari et al data (15). Therefore, the Taylor model (17,18) may represent a state that is more biased toward the OFF structure than the state that we are measuring in the absence of nucleotides.…”

Section: Structural Models Of Heavy Meromyosin: Implications Of Dynammentioning

confidence: 99%

“…Nucleotides have little effect upon the distribution of the relative head-to-head positions of both phosphorylated and unphosphorylated SMM at low ionic strength as determined by atomic force microscopy (11). Large structural differences between the conformation of the RLC N-terminal domain are observed in the absence of nucleotides (15,16), although nucleotide binding can enhance the structural differences (15). Two measures that are consistent with partial release of cross-bridges from the vertebrate skMM filament surface by phosphorylation, the phosphorylation-induced decrease in the chemical cross-linking rate between the S2 and the filament surface and the increase in the proteolytic susceptibility of the HMM-LMM junction, are observed without nucleotides (26).…”

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confidence: 99%

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Regulatory and Catalytic Domain Dynamics of Smooth Muscle Myosin Filaments

Song

Salzameda

et al. 2006

Biochemistry

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Domain dynamics of the chicken gizzard smooth muscle myosin catalytic domain (heavy chain Cys-717) and regulatory domain (regulatory light chain Cys-108) were determined in the absence of nucleotides using saturation-transfer electron paramagnetic resonance. In unphosphorylated synthetic filaments, the effective rotational correlation times, τ r , were 24 ± 6 μs and 441 ± 79 μs for the catalytic and regulatory domains, respectively. The corresponding amplitudes of motion were 42 ± 4° and 24 ± 9° as determined from steady-state phosphorescence anisotropy. These results suggest that the two domains have independent mobility due to a hinge between the two domains. Although a similar hinge was observed for skeletal myosin (Adhikari and Fajer (1997) Proc. Natl. Acad. Sci. U.S. A. 94, 9643-9647. Brown et al. (2001) Biochemistry 40,[8283][8284][8285][8286][8287][8288][8289][8290][8291], the latter displayed higher regulatory domain mobility, τ r = 40 ± 3 μs, suggesting a smooth muscle specific mechanism of constraining regulatory domain dynamics. In the myosin monomers the correlation times for both domains were the same (~4 μs) for both smooth and skeletal myosin, suggesting that the motional difference between the two isoforms in the filaments was not due to intrinsic variation of hinge stiffness. Heavy chain/regulatory light chain chimeras of smooth and skeletal myosin pinpointed the origin of the restriction to the heavy chain and established correlation between the regulatory domain dynamics with the ability of myosin to switch off but not to switch on the ATPase and the actin sliding velocity. Phosphorylation of smooth muscle myosin filaments caused a small increase in the amplitude of motion of the regulatory domain (from 24 ± 4° to 36 ± 7°) but did not significantly affect the rotational correlation time of the regulatory domain (441 to 408 μs) or the catalytic domain (24 to 17 μs). These data are not consistent with a stable interaction between the two catalytic domains in unphosphorylated smooth muscle myosin filaments in the absence of nucleotides. † This material is based upon work supported by the National Science Foundation under Grant No. 0346650, the AHA GIA 0455236B to P.G.F., and NIH AR40917 to C.R.C. and TCMRC 90103 to H.-C.L. L.S. is a recipient of American Heart Graduate Fellowship. *Author to whom correspondence should be addressed. Mailing address: Inst. Molecular Biophysics, Florida State University, Tallahassee, FL 32306. Tel: 850-645-1335. Fax: 850-644-1366. fajer@magnet.fsu.edu. ‡ Florida State University. § Tzu-Chi University. || These authors contributed equally. ⊥ University of Nevada School of Medicine. HHS Public Access Author Manuscript Author ManuscriptAuthor Manuscript Author ManuscriptMyosins are a superfamily of motor proteins that convert the chemical energy derived from ATP hydrolysis to mechanical energy by generating movement or force. Myosin II, the major protein from muscle, consists of two globular head domains and a coiled-coil tail or rod domain. At physiological...

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supporting

confidence: 74%

Section: Structural Models Of Heavy Meromyosin: Implications Of Dynammentioning

confidence: 99%

Section: Structural Models Of Heavy Meromyosin: Implications Of Dynammentioning

confidence: 99%

mentioning

confidence: 99%

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Regulatory and Catalytic Domain Dynamics of Smooth Muscle Myosin Filaments

Song

Salzameda

et al. 2006

Biochemistry

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“…27) versus HMM (used here), and (iii) a large structural transition in the N-terminal domain from disordered to ordered helix was found in HMM (without ATP), but not in S1 (27). Yet another study has shown that fluorophores on the RLC N-terminal domain sense changes in solvent exposure upon ATP binding and phosphorylation but only in regulated constructs HMM but not S1 (29). Therefore it is likely that backbone conformational heterogeneity in the N-terminal domain contributes to the heterogeneity in the RLC-RLC distances, consistent with the variation of the distance distribution widths measured here.…”

Section: Discussionmentioning

confidence: 82%

Broad disorder and the allosteric mechanism of myosin II regulation by phosphorylation

Vileno

Chamoun

Liang

et al. 2011

Proc. Natl. Acad. Sci. U.S.A.

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Double electron electron resonance EPR methods was used to measure the effects of the allosteric modulators, phosphorylation, and ATP, on the distances and distance distributions between the two regulatory light chain of myosin (RLC). Three different states of smooth muscle myosin (SMM) were studied: monomers, the shorttailed subfragment heavy meromyosin, and SMM filaments. We reconstituted myosin with nine single cysteine spin-labeled RLC. For all mutants we found a broad distribution of distances that could not be explained by spin-label rotamer diversity. For SMM and heavy meromyosin, several sites showed two heterogeneous populations in the unphosphorylated samples, whereas only one was observed after phosphorylation. The data were consistent with the presence of two coexisting heterogeneous populations of structures in the unphosphorylated samples. The two populations were attributed to an on and off state by comparing data from unphosphorylated and phosphorylated samples. Models of these two states were generated using a rigid body docking approach derived from EM [Wendt T, Taylor D, Trybus KM, Taylor K (2001) Proc Natl Acad Sci USA 98:4361-4366] (PNAS, 2001, 98:4361-4366), but our data revealed a new feature of the offstate, which is heterogeneity in the orientation of the two RLC. Our average off-state structure was very similar to the Wendt model reveal a new feature of the off state, which is heterogeneity in the orientations of the two RLC. As found previously in the EM study, our on-state structure was completely different from the off-state structure. The heads are splayed out and there is even more heterogeneity in the orientations of the two RLC.computational modeling | structural biology M yosin II is a motor protein that can transduce chemical energy from ATP hydrolysis into mechanical work. This process involves cyclic interactions between actin in thin and myosin in thick filaments causing relative filament sliding. Smooth muscle myosin (SMM), which contains two heads, each with a motor domain (MD) and regulatory domain (RD), connected by a long coiled-coil tail domain is an example of a large multisubunit protein that is allosterically regulated by phosphorylation (for review, see ref. 1). Phosphorylation of a single serine on each regulatory light chain (RLC), which are about 100 Å distant from the active sites, is sufficient to transform the protein from a state in which the ATPase activity is weakly actin-activated to one in which it is strongly actin-activated by controlling the rate of Pi release (2). Because phosphorylation modulates the rate of ADP release (3) and also alters the attitude of the lever arm domain with respect to the MD (4), it is likely that phosphorylation modulates strain between the two heads (5).The structural basis for the allosteric regulation has been a topic of intense study. It is a difficult problem because regulation by phosphorylation requires the presence of both head domains. Cryogenic EM studies of double-headed constructs (6-9) have incorporated data fr...

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Smooth-Muscle Myosin II

Cremo

Hartshorne

Proteins and Cell Regulation

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Novel Sensors of the Regulatory Switch on the Regulatory Light Chain of Smooth Muscle Myosin

Cited by 21 publications

References 60 publications

Regulatory and Catalytic Domain Dynamics of Smooth Muscle Myosin Filaments

Regulatory and Catalytic Domain Dynamics of Smooth Muscle Myosin Filaments

Broad disorder and the allosteric mechanism of myosin II regulation by phosphorylation

Smooth-Muscle Myosin II

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