EC:3.6.1.3 - FACTA Search

Gene/Protein Disease Symptom Drug Enzyme Compound
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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)

To determine whether basal phosphoinositide turnover plays a role in metabolic regulation in resting rabbit aortic intima-media incubated under steady state conditions, we used deprivation of extracellular myo-inositol as a potential means of inhibiting basal phosphatidylinositol (PI) synthesis at restricted sites and of depleting small phosphoinositide pools with a rapid basal turnover. Medium myo-inositol in a normal plasma level was required to prevent inhibition of a specific component of basal de novo PI synthesis that is necessary to demonstrate a discrete rapidly turning-over [1,3-14C]glycerol-labeled PI pool. Medium myo-inositol was also required to label the discrete PI pool with [1-14C]arachidonic acid (AA). The rapid basal turnover of this PI pool, when labeled with glycerol or AA, was not attributable to its utilization for polyphosphoinositide formation, and it seems to reflect basal PI hydrolysis. Depleting endogenous free AA with medium defatted albumin selectively inhibits the component of basal de novo PI synthesis that replenishes the rapidly turning-over PI pool. A component of normal resting energy utilization in aortic intima-media also specifically requires medium myo-inositol in a normal plasma level and a free AA pool; its magnitude is unaltered by indomethacin, nordihydroguaiaretic acid, or Ca2+-free medium. This energy utilization results primarily from Na+/K+ ATPase activity (ouabain-inhibitable O2 consumption), and in Ca2+-free medium deprivation of medium myo-inositol or of free AA inhibits resting Na+/K+ ATPase activity to a similar degree (60%, 52%). In aortic intima-media basal PI turnover controls a major fraction of resting Na+/K+ ATPase activity.
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PMID:Basal phosphatidylinositol turnover controls aortic Na+/K+ ATPase activity. 300 62

Artificial liver support is used to remove toxic substances accumulating in the circulation of patients with fulminant hepatic failure. Charcoal haemoperfusion with infusion of prostacyclin (PGI2) to prevent platelet damage has become a routine treatment and has led to improved survival. In 76 patients treated 29 (38%) survived to leave hospital and of these 31 patients were treated when in Grade III coma and 20 (65%) survived. Charcoal haemoperfusion also reduced the incidence of cerebral oedema which is a major cause of death in fulminant hepatic failure. Most episodes (congruent to 80%) of cerebral oedema can be managed using the osmotic agent mannitol. In a complete liver support system both protein-bound and compounds of a middle relative molecular mass as well as water soluble compounds should be removed. An albumin-coated resin has been developed to remove these compounds and in preliminary clinical studies it has been shown to have good blood compatibility and satisfactory adsorption properties. The importance of combined systems has been confirmed in studies on the removal of inhibitors of brain Na+K+-ATPase, where both resin and charcoal columns removed significant amounts of the inhibitory activity.
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PMID:Use of artificial liver support. 300 80

Isolation of non-esterified [14C]cholesterol bound to albumin from rat serum, 8 days after i.p. injection of [14C]cholesterol, was achieved by affinity chromatography, using Cibacron blue F3GA bound to Sepharose 4B and by Sephadex G-150 column chromatography. Both methods permit isolation of large quantities of cholesterol-loaded albumin, free of globulins and lipoproteins. The isolated albumin-cholesterol fraction was estimated to be 4.6 mg/100 ml serum, which represents approx. the 24% of the non-esterified cholesterol present in the rat serum. Albumin-cholesterol, cholesterol glucoside, cholesterol hemisuccinate and hydroxylated derivatives of cholesterol produced a biphasic curve of changes in synaptosomal plasma membranes (SPM)-bound (Na+ + K+)-stimulated ATPase activity. Low concentrations of the ligand progressively increased the enzyme activity, while increasing the ligand concentration above that which maximally stimulated the enzyme activity, produced a progressive inhibition. Lipoproteins did not have any effect on the enzyme activity. The fluorescence anisotropy of 1,6-diphenyl-1,3,5-hexatriene-labeled SPM, increased in albumin-cholesterol derivatives-treated SPM, which is consistent with a general decrease in membrane bilayer fluidity. The results provide evidence that the 'albumin-cholesterol' fraction of the serum may directly affect the cell membrane-bound enzyme activity.
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PMID:Evidence for the existence of non-esterified cholesterol carried by albumin in rat serum. 301 57

A crude fraction was isolated from pig heart left ventricle (150 g) homogenates after extraction of lipids, chromatographic separation and desalting. The extract contained an ionic content of 0.21, 0.27, 0.33 and 1.7 mM respectively for Mg2+, Ca2+, K+, and Na+. The albumin extract, used as a reference control, contained an ionic content of 0.88 and 2.1 mM respectively for K+ and Na+ and negligible amounts of Mg2+ and Ca2+. The isolated fraction exhibited digitalis-like properties in the inhibition of sarcolemmal Na+, K+-ATPase in a dose dependent manner, the displacement of [3H]-ouabain binding from membrane receptor sites and produced +ve inotropic response in isolated perfused heart in a dose dependent manner. The albumin extract tested in the same manner showed no digitalis-like properties. The ventricular fraction was unable to displace (-) 3H-DHA binding from membrane sites and its inotropic action was not blocked by propranolol. The data suggests that the fraction isolated from pig heart left ventricle contains a substance which has some properties like digitalis.
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PMID:Endogenous digitalis-like substance in pig left ventricle. 302 38

To establish if epidermal Langerhans cells (LC) are related to spleen dendritic cells, we have considered the morphology, phenotype, and function of the 2 cell types in culture. Cultured LC could be partially enriched (up to 50%) on the basis of 2 simple physical properties: nonadherence to plastic, and low buoyant density in dense albumin columns. The morphology of cultured LC and spleen dendritic cells were similar. In particular both cell types had many cell processes and/or veils, and cultured LC lost their distinguishing Birbeck granules. Freshly isolated LC exhibited nonspecific esterase and ATPase, as well as the F4/80 (alpha-macrophage) and 2.4G2 (alpha-Fc receptor) antigens. However all these traits were lost in culture, while Ia and Mac-1 antigens persisted. As a result, the cytochemical and antigenic phenotype of LC became similar to spleen dendritic cells. The one exception was that LC lacked the 33D1 dendritic cell antigen. The function of LC at first differed from spleen dendritic cells in that fresh LC were weak stimulators of T cell proliferation in the mixed leukocyte reaction and in sodium periodate-induced mitogenesis. However, stimulatory activity per cell increased at least 30 fold in culture so that by 2-3 days, LC were 3-10 times more potent than dendritic cells. Maturation of LC function was radioresistant and was accompanied by a small increase in cell surface Ia antigens. Although LC have been likened both to lymphoid dendritic cells and to macrophages, our data suggest a different conclusion. LC seem to be dendritic cell precursors and are immunologically immature. Possibly, lymphoid dendritic cells are in general derived from substantial pools of precursors in nonlymphoid tissues, such as epidermal LC.
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PMID:A comparison of murine epidermal Langerhans cells with spleen dendritic cells. 315 9

Hepatocytes of transgenic mouse fetuses harboring SV40 virus transforming gene sequences in the SV delta e-MGH fusion gene construct 202 driven by the mouse metallothionein (MT-I) enhancer [R. D. Palmiter, H. Y. Chen, A. Messing, and R. L. Brinster (1985) Nature (London) 316, 457-460] were cultured at Day 19 of gestation and established as a differentiated line expressing albumin and alpha-fetoprotein (AFP) mRNAs. Hepatocyte line FMH-202 contains integrated SV40 sequences, expresses SV40 T-antigen genes, and exhibits unlimited growth potential because it has been cultured 18 months without apparent decrease in cell viability or in growth rate that could suggest the occurrence of a crisis period. Immortalized cells multiply in chemically defined medium deficient in arginine with transferrin plus insulin, whereas EGF, insulin, and transferrin are obligatory requirements for fetal or newborn mouse hepatocyte multiplication in primary cultures. Cells did not grow in agar and were not tumorigenic in nude mice. Their immortalized, nonmalignant phenotype was further documented by low saturation densities of confluent monolayers showing no overgrowth, and by growth arrest in the absence of insulin with subsequent induction of DNA synthesis and resumption of cell growth in response to insulin. Thus, it appears that immortalized SV40 T-antigen-expressing hepatocytes are present in the liver of the transgenic mice. However, at later points in liver development the transforming activity of T-antigen becomes apparent and leads to hepatocellular carcinoma formation in vivo.
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PMID:Immortalized differentiated hepatocyte lines derived from transgenic mice harboring SV40 T-antigen genes. 328 99

The beta-bungarotoxin-induced depolarization of the synaptosomal plasma membrane monitored by the efflux of 86Rb+ is potentiated by raising the albumin in the incubation, is Ca2+-dependent and is due neither to inhibition of the (Na+ + K+)-dependent ATPase nor to activation of the voltage-dependent Na+ channel. Occupancy of the beta-bungarotoxin-binding site by dendrotoxin inhibits partially the action of beta-bungarotoxin. The efflux of 86Rb+ is parallelled by a release of lactate dehydrogenase from the synaptosome, and the two processes are maximal with 2 nM-toxin. Digitonin induces a release of 86Rb+ and lactate dehydrogenase closely similar to that seen with beta-bungarotoxin. It is concluded that the toxicity of beta-bungarotoxin for mammalian nerve terminals can be largely accounted for by specific site-directed phospholipase A2-induced permeabilization of the plasma membrane.
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PMID:The mechanism of action of beta-bungarotoxin at the presynaptic plasma membrane. 395 50

The distribution of I-labelled luteinizing hormone (LH) was studied by autoradiography of the murine pregnant ovary 10 min after intravenous administration. The grains in autoradiograms were localized around the luteal cells. The pregnant ovary showed the highest uptake of I-labelled LH 30 min. after the injection. No similar accumulation of I-labelled follicle-stimulating hormone, I-labelled albumin of free I was obtained. The ribosomal fraction of the corpus luteum contained a slightly higher level of radioactivity than the other subcellular fractions after injection of I-labelled LH. Sucrose density gradient centrifugation of the luteal particle preparation resulted in an enrichment of radioactivity in particles containing Na+,K+-activated ATPase, a marker enzyme of the plasma membrane. These findings support the concept of plasma membrane binding as the initial event in LH action on the target tissue.
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PMID:Attachment to the luteal plasma membranes: an early event in the action of luteinizing hormone. 414 22

1. Everted sacs of new-born pig intestines incubated in bicarbonate saline at 37 degrees C, transferred bovine plasma albumin across the mucosa into fluid bathing the serosa, the amount transferred increasing as the concentration of albumin in the mucosal fluid was raised from 0.5 to 16 g/100 ml.2. The rate of albumin transfer across the foetal pig intestine showed an apparent maximum, about 400 mug/g intestine/hr, 2 weeks before birth. The transfer at birth, about 200 mug/g intestine/hr, fell sharply during the next 2 days but later returned to that previously found at birth.3. When sacs were prepared from the intestines of 1 to 7-day-old pigs part of the recovered albumin was degraded. No digestion was found when the intestines of new-born or foetal pigs were used.4. The transfer of water and sodium, but not glucose, measured across the foetal and new-born pig intestine, was consistently higher when albumin was present in the mucosal fluid: the transmural potential difference was lowered by the presence of albumin. These differences disappeared during the first 2 days of life.5. Both the total and ouabain-sensitive adenosine triphosphatase (ATPase) activities of the pig intestinal epithelium fell within 24 hr of birth. There was some increase in total ATPase activity in older pigs but the ouabain-sensitive activity remained low.6. The relation between albumin and sodium transport, seen at a time when albumin is not being metabolized, suggests that the transfers are closely coupled. The movement of sodium into a mucosal cell down its own concentration gradient may provide energy for the translocation of albumin.
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PMID:Interdependence of albumin and sodium transport in the foetal and new-born pig intestine. 423 38

Human platelets separated from blood by six different methods have been compared for aggregability, adhesion to glass, adenine nucleotide content and release, and adenosine triphosphatase and cholinesterase activities. Methods of separation of platelets from blood included three differential centrifugation technics, gel filtration and two albumin density gradient methods. Platelets prepared by the different methods aggregated comparably except those separated by albumin density gradient technics which tended to be hyporeactive. Differences in adhesion to glass, adenine nucleotide content and release, and monitored enzyme activities of the various platelet preparations were noted in several cases but were not marked in general. Ultrastructural studies, reported elsewhere, revealed that platelets separated by the method of Mustard or by gel filtration were less altered morphologically than those separated by the other methods. Platelets separated from blood by gel filtration also appeared somewhat superior functionally to platelets separated by other methods.
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PMID:Comparison of certain functions of human platelets separated from blood by various means. 427 71

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