EC:3.6.1.3 - FACTA Search

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Query: EC:3.6.1.3 (ATPase)
65,361 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

1-5 of the epsilon-amino groups of myosin were trinitrophenylated by 2,4,6-trinitrobenzene sulphonate. The Mg2+-activated ATPase activity was found to increase twenty fold while the K+-activated ATPase was strongly inhibited as a result of this treatment. Myosin was dissociated by urea after trinitrophenylation and its heavy and light chains were isolated. Virtually all the introduced trinitrophenyl groups were found in the heavy chain indicating that the lysyl residues, the modification of which affects the ATPase activity, are located at the heavy core of the myosin molecule.
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PMID:Studies on the amino groups of myosin-ATPase. II. Localization of the amino groups. 12 97

Two types of canine cardiac myosins, from the free wall of the left ventricle and from the free wall of the right ventricle, were compared with canine skeletal muscle myosin from gastrocnemius. For K+ -activated myosin the Vmax values in mumoles of Pi/mg.min were: right ventricle, 0.57 +/- 0.02; left ventricle, 0.72 +/- 0.09; gastrocnemius, 0.92 +/- 0.04. For Ca++ -activated myosin the Vmax values were: right ventricle, 0.32 +/- 0.04; left ventricle, 0.42 +/- 0.03; gastrocnemius, 0.52 +/- 0.02; (p greater than 0.01 for all defferences). For all three types of tissues the Vmax values for NH4+ -activated myosin were the same (2.30 +/- 0.11). Corresponding to kinetic changes there were significant changes in the proportion and type of myosin subunits. In the two cardiac ventricles where heavy chains were immunologically identical, 81% of the total nitrogen of right ventricular myosin was present in the heavy chains whereas in left ventricular myosin 90% of the total nitrogen of myosin was present in the heavy chains. Quantifications were made on polyacrylamide gels were dye binding was directly related to nitrogen concentration for each of the myosin chains. In canine skeletal muscle gastrocnemius where the myosin heavy chains were immunologically nonidentical with those of cardiac myosin, 87% of the total nitrogen was present in the heavy chains. The data suggest that there are 2 moles of myosin light chains per mole of myosin heavy chains in right ventricular myosin where the adenosine triphosphatase (ATPase) activity is low and 1 mole of myosin light chains per mole of myosin heavy chains in left ventricula myosin where ATPase activity is elevated; for skeletal muscle myosin there were 1.5 moles of myosin light chains per mole of myosin heavy chains. Proportion of myosin light chain C1 to light chain C2 was the same in both left and right ventricular myosin. In skeletal muscle myosin the proportion of light chain C1 to light chain C2 was significantly different from that of cardiac tissue. It appears that the proportion of myosin light chain C1 to light chain C2 is directly related to the type of myosin heavy chain present since the immunologically identical heavy chains of cardiac tissue were immunologically nonidentical with those of skeletal muscle myosin.
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PMID:Comparative analyses of skeletal and cardiac myosins. 12 33

Mild pulmonic stenosis was performed in dogs to evaluate the effect of systolic pressures overloading on the activity and subunits of myosin in the early hypertrophied right ventricle. Three weeks following pulmonary constriction, six hypertrophied dogs were sacrificed and compared to six sham-operated dogs which served as controls. In the right ventricular free wall of hypertrophied right ventricles (HRV), the heart/body weight was 46% greater than that of normal right ventricles (NRV) (p less than 0.01). Myosin ATPase activity (Vmax values) in mumoles phosphate/mg/min, was elevated significantly in the stressed ventricle for both K+ and Ca++ activity in hypertrophied right ventricles. Associated with the increase in myosin activity, there was an increase in proportion of heavy to light chains in myosin from HRV. There were approximately 2 moles of myosin light chains per mole of myosin heavy chains in NRV and approximately 1 mole of myosin light chains per mole of myosin heavy chains in HRV. The proportion of light chain C1 to C2, did not change in myosin from NRV and HRV. Of the C1 light chains, according to two-dimensional gel electrophoresis, there was less C1d as compared to C1c in HRV as compared to NRV. Thus K+- and Ca++- activated myosin is elevated in early canine HRV by pressure overload. It is suggested taht the augmented myosin activity is due to a reduction of light chain inhibition of myosin ATPase activity, which appears to result from the slower turnover rate of myosin light chains relative to heavy chains. Furthermore, when myosin light chains are added to hypertrophied right ventricular myosin, the ATPase activity is lowered.
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PMID:Modulation of myosin in right ventricular hypertrophy. 12 38

SH group substitution by DTNB enabled natural actomyosin to split ATP (in the prescence of Mg2+) also in the absence of Ca2+, when assayed at low ionic strength. At higher KCl concentrations the ATPase activity of SH group substituted actomyosin was still Ca-dependent. Addition of unsubstituted myosin to natural actomyosin whose SH groups had been substituted increased the ATPase activity. This increase was Ca-insensitive indicating that SH group substitution of myosin in actomyosin can make the interaction of additional myosin molecules Ca-independent. In natural actomyosin Ca-insensitivity of ATPase activity was attained at a lower degree of SH group substitution when substitution was performed in the presence of EDTA. The part of ATPase activity which still remained Ca-sensitive after DTNB treatment could be activated by lower concentrations of free Ca2+ than the Ca-sensitive ATPase of untreated actomyosin. In reconstituted actomyosin the Ca-sensitivity of ATPase activity could more easily be reduced when the myosin-actin ratio was high. For demonstrating remaining Ca-sensitivity in SH group substituted reconstituted actomyosin more tropomyosin-troponin was needed than for sensitizing unsubstituted actomyosin to Ca2+. The similarities between the ATPase acitivity of SH group substituted actomyosin on the one hand and that of actomyosin at low concentrations of ATP on the other hand suggest that SH group substitution modifies actin-myosin interaction in a similar way as does nucleotide-free myosin (rigor myosin).
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PMID:Calcium sensitivity of actomyosin ATPase: its modification by substitution of myosin sulfhydryl groups. 12 88

Using myosin, heavy meromyosin, and subfragment-1 the steady state rate of Mg-modified adenosine triphosphatase (Mg-ATPase) was determined over a range of substrate concentrations between 10(-8) M and 5 X 10(-3)M, at 0.5 M and 0.05 M KC1 (pH 7.4 at 20 degrees C). At the substrate concentrations below 10(-5) M, myosin Mg-ATPase was observed to show that two active sites interact, as suggested by the analysis of transient kinetic studies (Walz, F. G., Jr.: J. Theor. Biol. 41, 357-373 (1973)). The increase in the activity at Mg-ATP concentrations higher than 10(-4) M corresponds to the binding of Mg-ATP to myosin sites not responsible for the catalytic action. With heavy meromyosin and subfragment-1, the activity was best expressed by the Michaelis equation. With heavy meromyonsin, the activation at high ATP concentrations is detectable, though not as pronounced as with myosin, but not with subfragment-1.
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PMID:The effects of substrate concentration on the Mg-adenosine triphosphatase activity of myosin. 13 Jan 98

Experimentally-induced ischaemia in the dog heart was produced by ligating the left circumflex artery. Myosin B isolated from the ischaemic portion of the myocardium differed from myosin B isolated from control tissue in its diminished response to the calcium chelator ethyleneglycol bis (beta-amino-ethylether)-N, N'-tetraacetic acid (EGTA). In the presence of EGTA, ischaemic myosin B required 2.5 +/- 0.5 min for completion of superprecipitation, whereas control myosin B required 6.6 +/- 2.5 min. Likewise, the Mg++ -activated ATPase activity of ischaemic myosin B was inhibited by EGTA to a lesser degree than control myosin B. Experiments with reconstituted myosin B using desensitized control myosin B and regulatory proteins suggest that ischaemia induces changes in the regulatory proteins (troponin and tropomyosin).
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PMID:Biochemical and morphological correlates of cardiac ischaemia: Contractile proteins. 13 Feb 6

Frozen sections of equine musculus semitendinosus were examined for myosin adenosine triphosphatase (ATPase) and reduced nicotinamide adenine dinucleotide-tetrazolium reductase (NADH-TR), using standard histochemical procedures, and the proportions of the various fiber types and average fiber sectional size were determined. With ATPase staining, approximately 70% of the fibers were classified as alpha fibers (ATPase positive), and 30%, as beta fibers (ATPase negative). In addition, 2 populations of alpha fibers could be readily distinguished on the basis of the intensity of the ATPase reaction, and these were designated alpha positive and alpha intermediate. The relationship of this difference in ATPase reaction to contraction speed of the fibers is not known. With NADH-TR staining, fibers were classified as either red fibers (positive) having aerobic metabolism or white fibers (negative) having primarily anaerobic metabolism. All beta fibers were red by NADH-TR; thus, they conformed to the criteria for beta R fibers. All alpha positive fibers were white by NADH-TR, as were most of the alpha intermediate fibers, and would be classified alpha W. Some of the alpha intermediate fibers gave an intermediate reaction with NADH-TR and could be classified as alpha R fibers which have not transformed to alpha W fibers. The alpha positive fibers were 7 to 10 mum larger in diameter than either beta or alpha intermediate fibers.
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PMID:Fiber types and size in equine skeletal muscle. 13 Aug 14

If we select for consideration any reaction M1 in equilibrium M2 in the myosin-ATPase cycle, the question arises as to the relations between the rate constants for (1) M1 equilibrium M2, (2) AM1 in equilibrium AM2 (A = actin), (3) A + M1 in equilibrium AM1, and (4) A + M2 equilibrium AM2, with actin and myosin either (a) in solution or (b) in the myofilament structure. It is shown here, by means of examples, that a single so-called potential of mean force, W, and structural free energy, Am, suffice to determine the reaction free energy surfaces for all of these transitions (W for the solution case, W + Am for the structured case). In fact, Am is the same for all reactions in the myosin-ATPase cycle. Of course, though indispensable as the starting point and adequate for qualitative understanding, the reaction free energy surface does not provide (without additional theory) the actual values of the rate constants or of the corresponding basic free energy changes in the myosin states involved. These rate constants and free energies are discussed, in a preliminary way, in two other papers.
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PMID:Reaction free energy surfaces in myosin-actin-ATP systems. 13 77

A study of myosin extracted from dog's cardiac muscle at different stages of chronic heart failure (from 1 week to 1 year) was carried out. A decrease of UV-luminescence intensity, flow birefringence and ATPase activity (to 70%) was observed. The electron microscopic investigation of myosin and LMM structure shows the loss of ability to form typical paracrystals by LMM, the electron microscopic appearance of the whole myosin being unchanged.
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PMID:[Structural and functional changes in myosin in chronic coronary insufficiency]. 13 86

A contractile protein closely resembling natural actomyosin (myosin B) of rabbit skeletal muscle was extracted from plasmodia of the slime mold, Physarum polycephalum, by protecting the SH-groups with beta-mercaptoethanol or dithiothreitol. Superprecipitation of the protein induced by Mg2+-ATP at low ionic strength was observed only in the presence of very low concentrations of free Ca2+ ions, and the Mg2+-ATPase [EC 3.6.1.3] reaction was activated 2- to 6-fold by 1 muM of free Ca2+ ions. Crude myosin and actin fractions were separated by centrifuging plasmodium myosin B in the presence of Mg2+-PPi at high ionic strength. The crude myosin showed both EDTA- and Ca2+-activated ATPase activities. The Mg2+-ATPase activity of crude myosin from plasmodia was markedly activated by the addition of pure F-actin from rabbit skeletal muscle. Addition of the F-action-regulatory protein complex prepared from rabbit skeletal muscle as well as the actin fraction of plasmodium caused the same degree of activation as the addition of pure F-actin only in the presence of very low concentrations of Ca2+ ion
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PMID:Ca2+-sensitivity of actomyosin ATPase purified from Physarum polycephalum. 13 90

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