Stability of Segments of Rabbit a-Tropomyosin

Woods, E. F.

doi:10.1071/bi9770527

Cited by 24 publications

(20 citation statements)

References 26 publications

(46 reference statements)

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“…Fluorescence probe studies with the label at Cys 190 have indicated that the probe responds to the unfolding in the pretransition temperature region (12, 13, 33). The main transition at 47°C is due to unfolding of the C-terminal region and the transition at about 54°C is due to unfolding in the N-terminal region (25, 26, 32). The relative areas under the derivative curves in Fig.…”

Section: Discussionmentioning

confidence: 99%

Long-Range Effects of Familial Hypertrophic Cardiomyopathy Mutations E180G and D175N on the Properties of Tropomyosin

Lehrer

2012

Biochemistry

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Cardiac α-tropomyosin (Tm) single site mutations, D175N and E180G, cause familial hypertrophic cardiomyopathy (FHC). Previous studies have shown that these mutations increase both Ca2+-sensitivity and residual contractile activity at low Ca2+, which causes incomplete relaxation during diastole resulting in hypertrophy and sarcomeric disarray. However, the molecular basis for the cause and the difference in severity of the manifested phenotypes of disease is not known. In this work we have: 1) used ATPase studies on reconstituted thin filaments in solution to show that these FHC mutants result in an increase in Ca2+-sensitivity and increased residual ATPase; 2) shown that both FHC mutants increase the rate of cleavage at R133, about 45 residues N-terminal to the mutations, when free and bound to actin; 3) shown that for Tm-E180G, the increase in the rate of cleavage is greater than for D175N; 4) shown that for E180G, cleavage also occurs at a new site 53 residues C-terminal to E180G, in parallel with cleavage at R133. The long-range decreases in dynamic stability due to these two single site mutations, suggests increases in flexibility that may decrease the ability of Tm to inhibit activity at low Ca2+ for D175N and to a greater degree for E180G, which may contribute to differences in the severity of FHC.

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Section: Discussionmentioning

confidence: 99%

Long-Range Effects of Familial Hypertrophic Cardiomyopathy Mutations E180G and D175N on the Properties of Tropomyosin

Lehrer

2012

Biochemistry

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“…The length of coiled-coil regions is likely to be greater in the native keratin since the potential number of residues which can take up this conformation is 103 and 100 respectively for the two types of polypeptide chains involved (Fraser et al 1976) (~94 % ex-helix and a potential length of 15 nm). Fragments of the ex-helical muscle protein, a-tropomyosin, obtained by either chemical splitting or limited proteolysis (Woods 1977;Pato et al 1981) all show a lower ex-helix content than the parent protein. The molecular weight of 50200 for the helix-rich particle excludes the similar three subunit structure 'of Crewther and Dowling (1971), Crewther (1976) in favour of a four-chain particle.…”

Section: General Discussion and Conclusionmentioning

confidence: 99%

Structural Studies on the Microfibrillar Proteins of Wool: Characterization of the a-Helix-Rich Particle Produced by Chymotryptic Digestion

Woods¹,

Gruen²

1981

Aust. Jnl. Of Bio. Sci.

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The oc-helix-rich particle produced bychymotryptic digestion of the reduced and alkylated microfibrillar proteins of wool was characterized by physicochemical methods. The preparations were homogeneous with respect to size and the particle molecular weight was found to be 50200 ± 2 000.Hydrodynamic methods indicated a length of about 20 nm for the particle. The properties of the particle, derived from two methods of isolation of the microfibrillar proteins, were identical and were also independent of the type of wool used. From a consideration of the molecular weight in denaturing solvents and from cross-linking experiments with dimethyl suberimidate a four-chain structure, consisting of a pair of double-stranded oc-helices, is proposed for the particle.

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“…The molecule unfolds, with increasing temperature or concentration of denaturant, in two distinct stages (Woods, 1969;Pont & Woods, 1971;Satoh & Mihashi, 1972). The first stage, the pretransition, appears to involve unfolding of the C-terminal half of the molecule, and the second stage, the main transition, involves the complete unfolding of the molecule (Chao & Holtzer, 1975;Woods, 1977;Betcher-Lange & Lehrer, 1978;Lehrer, 1978;Pato & Smillie, 1978;Potekhin & Privalov, 1978). Woods (1976) has described this as an equilibrium between the native molecule, N, a partially unfolded (in the C-terminal half) intermediate state, X, and the completely denatured tropomyosin, D; Le., N F= X D. Studies of the fluorescence of probes attached to cysteine-190 (Graceffa & Lehrer, 1980;Betteridge & Lehrer, 1983), of the N M R of histidine-153 (Edwards & Sykes, 1980), and of differential scanning calorimetry of tropomyosin (Williams & Swenson, 1981;Potekhin & Privalov, 1982) have provided more direct evidence for multistate thermal equilibria.…”

Section: Dynamic Equilibrium Between the Two Conformational States Ofmentioning

confidence: 99%

Dynamic equilibrium between the two conformational states of spin-labeled tropomyosin

Graceffa¹,

Lehrer²

1984

Biochemistry

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Tropomyosin was labeled with a maleimide nitroxide spin-label attached to cysteine-190 via a succinimido ring which was subsequently opened by incubation at alkaline pH. Electron spin resonance (ESR) spectra showed a temperature-dependent equilibrium, below the main unfolding transition of tropomyosin, between labels which were restricted in their motion (strongly immobilized), predominating at low temperatures, and those which were highly mobile (weakly immobilized), predominating at higher temperatures. These label states were associated with two protein states from a comparison of the ESR spectral changes with the thermal unfolding profile of tropomyosin. The strongly immobilized labels were associated with the completely folded molded and the weakly immobilized labels with a partially unfolded (in the cysteine-190 region) state which is an intermediate in the thermal unfolding of tropomyosin. A spectral subtraction technique was used to measure the concentration ratio of strongly and weakly immobilized labels from which an equilibrium constant, K, was determined at different temperatures. A linear van't Hoff plot was obtained, indicating that the spin-labeled protein is in thermal equilibrium between these two conformational states with delta H = 17 kcal/mol, delta S = 56 cal/(deg X mol), and K = 1.0 at 34 degrees C. An upper limit of 10(7) s-1 for the conformational fluctuation was estimated from the shapes and separation of the two ESR spectral components. In contrast to the label with the opened succinimido ring, the spin-label with an intact succinimido ring remained strongly immobilized on the protein, indicating that in the partially unfolded state the molecule retains structure in the cysteine-190 region.

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Stability of Segments of Rabbit a-Tropomyosin

Cited by 24 publications

References 26 publications

Long-Range Effects of Familial Hypertrophic Cardiomyopathy Mutations E180G and D175N on the Properties of Tropomyosin

Long-Range Effects of Familial Hypertrophic Cardiomyopathy Mutations E180G and D175N on the Properties of Tropomyosin

Structural Studies on the Microfibrillar Proteins of Wool: Characterization of the a-Helix-Rich Particle Produced by Chymotryptic Digestion

Dynamic equilibrium between the two conformational states of spin-labeled tropomyosin

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