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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)

The proton circuit devised by Mitchell in the chemiosmotic theory was subjected to analysis using the formalism of irreversible thermodynamics. The phenomenological coefficients and the degree of coupling relating co-permeant flows were derived from anion/H+, substrate/H+, cation/H+ and anion/anion biporter models. Linearity and equality of the cross-coefficients in Onsager relations were always satisfied. Macroscopic flows leading to charges splitting, such as oxido-reduction, hydro-dehydratation and transhydrogenase, are driven by a composite thermodynamic force which includes the proton-motive component. Multiple coupling occurs in the circuit when it is assumed that the net inward flux of protons becomes zero, i.e. when the circulation of protons reaches a stationary state. Under these conditions, oxidative phosphorylation, ATPase- or respiration-linked transhydrogenase and uptake of anion or cation against their electrochemical gradient may be predicted, in agreement with known experimental evidence.
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PMID:A non-equilibrium thermodynamics analysis of active transport within the framework of the chemiosotic theory. 0 23

Net synthesis of adenosine 5'-triphosphate (ATP) in energy-depleted cells of Escherichia coli was observed when an inwardly directed protonmotive force was artificially imposed. In wild-type cells, ATP synthesis occurred whether the protonmotive force was dominated by the membrane potential (negative inside) or the pH gradient (alkaline inside). Formation of ATP did not occur unless the protonmotive force exceeded a value of 200 mV. Under these conditions, no ATP synthesis was found when cells were exposed to an inhibitor of the membrane-bound Ca2+- and Mg2+- stimulated adenosine triphosphatase (EC 3.6.1.3), dicyclohexylcarbodiimide, or to a proton conductor, carbonylcyanide-p-trifluoromethoxyphenyl-hydrazone. Adenosine triphosphatase-negative mutants failed to show ATP synthesis in response to either a membrane potential or a pH gradient. ATP synthesis driven by a protonmotive force was observed in a cytochrome-deficient mutant. These observations are consistent with the chemiosmotic hypothesis of Mitchell (1961, 1966, 1974).
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PMID:Protonmotive force as the source of energy for adenosine 5'-triphosphate synthesis in Escherichia coli. 0 27

31P nuclear magnetic resonance spectra at 145.7 MHZ were obtained of concentrated suspensions of E. coli cells. The position of the Pi resonance was used to determine the pH, and in most experiments it was possible to distinguish the intracellular (pHin) and extracellular (pHex) values. During respiration pHin approached 7.55, while pHex varied from 6.0 to 8.0. With succinate as a carbon source and in a N2 environment, pHin - pHex. Upon addition of glucose, pHin greater than pHex. In the presence of an ATPase (adenosinetriphosphatase; ATP phosphohydrolase; EC 3.6.1.3) inhibitor dicyclohexylcarbodiimide, pHin remained equal to pHex even in the presence of glucose. In other experiments, oxygenation brought pHin above pHex even in the presence of dicyclohexylcarbodiimide. These experiments are consistent with Mitchell's hypothesis that, first, delta pH can be created by the reversal of the ATPase reaction and, second, that protons are pumped outward during respiration. In addition to Pi, about 10 more resonances were resolved, several of which were assigned to different phosphate metabolites.
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PMID:High-resolution 31P nuclear magnetic resonance studies of metabolism in aerobic Escherichia coli cells. 1 57

Growth of Halobacterium halobium under illumination with limiting aeration induces bacteriorhodopsin formation and renders the cells capable of photophosphorylation. Cells depleted of endogenous reserves by a starvation treatment were used to investigate the means by which energy is coupled to the active transport of [14C]proline, -leucine, and -histidine. Proline was readily accumulated by irradiated cells under anaerobiosis even when the photophosphorylation was abolished by the adenosine triphosphatase inhibitor N,N'-dicyclohexylcarbodimiide (DCCD). The uptake of proline in the dark was limited except when the cells were allowed to accumulate adenosine 5'-triphosphate (ATP) by prior light exposure or by the oxidation of glycerol. DCCD inhibited this dark uptake. These findings essentially support Mitchell's chemiosmotic theory of active transport. The driving force is apparently the proton-motive force developed when protons are extruded from irradiated bacteriorhodopsin or by the dydrolysis of ATP by membrane adenosine triphosphatase. Carbonylcyanide m-chlorophenylhydrazone (CCCP), a proton permeant known to abolish membrane potential, was a strong inhibitor of proline uptake. Leucine transport was also apparently driven by proton-motive force, although its kinetic properties differed from the proline system. Histidine transport is apparently not a chemiosmotic system. Dark- or light-exposed cells show comparable initial rats of histidine uptake, and these processes were only partially inhibited by DCCD or CCCP. The histidine system apparently does not utilize ATP per se since comparable rates of uptake were exhibited by cells of differing intracellular ATP levels. Irradiated cells did effect a greater total accumulation of histidine than dark-exposed cells. These findings suggest that ATP is needed for sustained transport.
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PMID:Energy coupling in the active transport of amino acids by bacteriohodopsin-containing cells of Halobacterium holobium. 12 52

Triphenylsulphonium ions inhibit mitochondrial oxidative phosphorylation and adenosine triphosphatase activity. The site of action is on the soluble F1 adenosine triphosphatase component. Triphenylsylphonium ions also inhibit electron transfer in the NAD-cytochrome b region of the respiratory chain. In both types of inhibition, triphenylsulphonium ions are effective at low concentrations, half-maximal inhibition being produced by a concentration of about 20-30 muM. These effects resemble the effects of alkylguanidines on mitochondria and are discussed in relation to the effects of alkylguanidines and other lipophilic cations such as ethidium and dibenzyldimethylammonium ions. A modification of the purification procedure for the soluble mitochondrial adenosine triphosphatase [Beechey, Hubbard, Linnett, Mitchell & Munn (1975) Biochem. J. 148, 533-537] IS DESCRIBED, WHICH YIELDS A PREPARATION WITH A HIGHER SPECIFIC ACTIVITY AND SHOWING FEWER BANDS IN GEL ELECTROPHORESIS.
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PMID:Effects of triphenylsulphonium ions on mitochondria. Inhibition of adenosine triphosphatase activity. 13 79

1. Soluble ATPase (adenosine triphosphatase) activity is released when rat liver submitochondrial particles are shaken with chloroform, provided that ATP or glycerol is present in the suspending medium. The extraction is very rapid and appears to be complete. 2. The ATPase of the chloroform extract is about 50% pure and can be readily purified to a specific activity of 60-70mumol/min per mg of protein by (NH(4))(2)SO(4) fractionation and column chromatography on Sephadex G-200. 3. The particulate and soluble ATPases have many similar properties, including their K(m) values for ATP, activation by various metal ions, hydrolytic activity with other nucleotides and stimulation by bicarbonate ions. 4. Unlike the particulate enzyme, the soluble enzyme is cold-labile and insensitive to oligomycin. 5. The molecular weight indicated by the mobility of the soluble ATPase on Sepharose 6B is 360000. 6. The soluble ATPase combines very readily with liver submitochondrial particles depleted of ATPase by salt extraction, and oligomycin-sensitivity is restored. Very little recombination of the enzyme occurs with chloroform-extracted particles. 7. The soluble enzyme contains orcinol-reactive material, suggesting that it may be a glycoprotein. The carbohydrate content was estimated to be 1-2% by weight. 8. It is concluded that the liver ATPase obtained by the chloroform extraction method of Beechey, Hubbard, Linnett, Mitchell & Munn [(1975) Biochem. J.148, 533-537] is similar to other preparations described previously and that this method is superior in simplicity and speed.
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PMID:Purification and properties of the adenosine triphosphatase released from the liver mitochondrial membrane by chloroform. 15 21

The active transport of organic anions through the plasma membrane of the proximal tubules of frog kidney was studied. For this purpose a marker anion, fluorescein, was used, its flow into the tubules registered by the increase of fluorescense. The kinetics of transport was measured as function of time, concentration of substrate, concentration of a competing acid (p-aminohippuric acid) and temperature. The process is inhibited by strophantin, a specific poison for (Na++K+)-dependent ATPase. These data show that fluorescein transport is effected with the participation of a charged carrier, probably by the downfield mechanism postulated by Mitchell. To confirm this mechanism, a passive flow of K+ was created inwards across the membrane of the proximal tubules by means of valinomycin. It led to the discharge of the membrane and to the inhibition of fluorescein transport. Anions are transported downfield across the membrane, probably in a state of complexes with two Na+ ions. A magnetic field of 10000-28000 oersted inhibits the fluorescein transport strongly. This can be regarded as a proof of the liquid-crystalline structure of biological membranes and demonstrates the importance of this structure for active transport.
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PMID:Structure and active transport in the plasma membrane of the tubules of frog kidney. 108 Oct 4

After the proposal of the chemiosmotic theory by Mitchell (1966, 1979) it has been recognized that different membrane-bound enzymes are able to use the energy derived from ionic gradients for the synthesis of ATP. These include the F1-ATPases of mitochondria and chloroplasts, the Ca2+-dependent ATPase of sarcoplasmic reticulum and the (Na+,K+)-ATPase of plasma membrane. In these systems the process of energy transduction is fully reversible. The enzyme can use the energy derived from the hydrolysis of ATP to build up a concentration gradient of ions across the membrane and, in the reverse process, use the energy derived from the gradient to synthesize ATP. Another interesting system in which these forms of energy are interconverted is found in photosynthetic bacteria. In chromatophores of Rhodospirillum rubrum there is a membrane-bound pyrophosphatase that, like the transport ATPases, catalyses the synthesis of pyrophosphate from Pi when a light-dependent proton gradient is formed across the chromatophore membrane. Like F1-ATPase, this enzyme is also able to generate an electrochemical potential gradient of protons at the expense of pyrophosphate hydrolysis. The mechanism by which the energy derived from a gradient is used by membrane-bound enzymes to catalyse the synthesis of high-energy phosphate compounds is still far from understood. Among the different enzymes studied, Ca2+-dependent ATPase is probably the system in which most is known about the mechanism of energy transduction. We now know of experimental conditions which allow us to move the different intermediary steps of the catalytic cycle of the enzyme in the direction of ATP synthesis. Thus, ATP synthesis can be attained after a single catalytic cycle in the absence of a transmembrane Ca2+ gradient. The net synthesis of ATP can be promoted by a variety of perturbations, including Ca2+, pH and water activity. These experiments indicate that during the catalytic cycle different forms of energy are interconverted by the Ca2+-dependent ATPase. The ultimate step of the cycle seems to be a change of water activity within the catalytic site of the ATPase. A common feature of all membrane-bound enzymes mentioned above is that during the catalytic cycle there are steps in which the hydrolysis of a phosphate compound (ATP, pyrophosphate or an acyl phosphate residue) is accompanied by only a small change in free energy. In conditions similar to those found in the cytosol, the hydrolysis of these phosphate compounds is accompanied by a much larger change in free energy.(ABSTRACT TRUNCATED AT 400 WORDS)
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PMID:Role of water in processes of energy transduction: Ca2+-transport ATPase and inorganic pyrophosphatase. 242 74

It is argued that a proton concentration difference and/or a membrane potential is not the form into which the free energy of the oxidation-reduction reactions of the mitochondrial respiratory chain is first transduced. It is suggested that the search for a chemical intermediate should be continued in spite of the conclusion by some investigators that the chemical hypothesis is untenable. It is asked whether pH changes when measured in solutions containing mitochondria can be interpreted as evidence for H+ movements, also, whether there is a continuous, renewable and stable electrochemical proton concentration difference (delta mu H+) across the mitochondrial membrane, and whether in fact the delta mu H+ is a necessary intermediate in the synthesis of ATP. The four postulates of Mitchell's chemiosmotic hypothesis of energy transduction are discussed point by point. It is agreed that "The systems are plugged through a topologically closed insulating membrane," which probably is not "a nonaqueous osmotic barrier," and which probably does not have an unusually "low permeability to solutes and to H+ and OH- in particular" when compared with other membranes. There is disagreement with the statement that "Respiratory and photoredox systems are chemiosmotic membrane-located protonmotive chains" in that it is suggested by others that chemiosmosis is chemically nonexistent and that thermodynamically it would lack control. The subsequent statement, "having a characteristic----H+/2 epsilon- stoichiometry," is rendered uncertain by the experimental findings of values greater than 2H+/2 epsilon-/site and probably as large as 4H+/2 epsilon-/site. The proposal that "The synthetase is a chemiosmotic membrane-located reversible motive ATPase" requires the assumption that the ATP synthetase is the same enzyme as the ATPase, but functioning in the reverse direction. It is considered possible that there are two enzymes in the multi-subunit ATPase complex: one the hydrolase, and the other the synthetase. The further proposal, "having characteristic----H+/P stoichiometry" requires that the ratio be 2 according to Mitchell. However, values of 3, as well as larger values, have been reported by others, which introduces a large element of uncertainty. There is no disagreement with the statement that "There are proton-linked (or hydroxyl ion-linked) solute porter systems for osmotic stabilization and metabolite transport." In fact, this may be the principal reason for having proton efflux or "proton-pumping.''(ABSTRACT TRUNCATED AT 400 WORDS)
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PMID:An assessment of the chemiosmotic hypothesis of mitochondrial energy transduction. 286 62

Acetaminophen is activated metabolically to yield reactive species that bind covalently to liver cell macromolecules. The extent of covalent binding correlates with the occurrence and severity of hepatic necrosis. We reported previously [J. O. Tsokos-Kuhn, E. L. Todd, J. B. McMillin-Wood and J. R. Mitchell, Molec. Pharmac. 28, 56 (1985)] that active Ca2+ accumulation of isolated liver plasma membranes is decreased 60-75% after a hepatotoxic dose of acetaminophen in vivo. We now report that the protein of isolated liver plasma membranes was substantially labeled with drug metabolites after administration of [3H]acetaminophen. There was no increase in passive membrane permeability that might cause diminished Ca2+ accumulation. Intravesicular volume and relative purity of the vesicle preparations after acetaminophen were not different from controls. However, (Ca2+,Mg2+)-ATPase, a possible biochemical expression of the Ca2+ pump, was decreased 31% (P less than 0.025) after acetaminophen treatment. ATPase activity in both control and treated groups was enhanced by isolating membranes in the presence of 5 mM reduced glutathione (GSH), but the effects of drug treatment were not reversed. A similar effect of GSH on Ca2+ accumulation was observed previously [J. O. Tsokos-Kuhn, E. L. Todd, J. B. McMillin-Wood and J. R. Mitchell, Molec. Pharmac. 28, 56 (1985)]. These data are consistent with a hypothesis wherein alkylation of membrane proteins by reactive acetaminophen metabolites is a factor in the onset of hepatic necrosis after acetaminophen. They are not consistent with an oxidative stress hypothesis where thiol S-thiolation of membrane components is postulated to produce altered membrane permeability or thiol-reversible alterations in membrane protein structure and enzymatic function.
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PMID:Alkylation of the liver plasma membrane and inhibition of the Ca2+ ATPase by acetaminophen. 296 3

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