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. The specific activity of rat and pig liver nuclear-envelope nucleoside triphosphatase (EC 3.6.1.3) decreases when the system is depleted of RNA. The activity can be restored by adding high concentrations of yeast RNA to the assay medium. 2. Exogenous RNA also increases the activity of the enzyme in control envelopes (not RNA-depleted). The effect appears to be largely specific for poly(A) and poly(G); it is not stimulated by rRNA or tRNA preparations, ribonuclease-hydrolysed RNA, AMP, or double- or single-stranded DNA. 3. Inhibitors of the enzyme, in concentrations at which half-maximal inhibition of the enzyme is achieved, do not affect the percentage stimulation of the enzyme by yeast RNA. 4. The simulation is abolished by the inclusion of 150 mM-KCl or -NaCl in the assay medium, but not by increasing the assay pH to 8.5. 5. The results are discussed in the light of the possible role of the nucleoside triphosphatase in vivo in nucleo-cytoplasmic ribonucleoprotein translocation. 6. It is proposed that poly(G)-stimulated Mg2+-activated adenosine triphosphatase activity should be adopted as an enzymic marker for the nuclear envelope.
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PMID:Ribonucleic acid stimulation of mammalian liver nuclear-envelope nucleoside triphosphatase. A possible enzymic marker for the nuclear envelope. 14 Dec 76

Multiplication-stimulating activity (MSA), a protein which stimulates DNA synthesis and growth of chicken embryo fibroblasts, was purified from serum-free medium conditioned by the growth of a rat liver cell line. Purified MSA was shown to rapidly stimulate ouabain-sensitive Na+, K+-ATPase activity as measured by both enzyme assay and rate of 86Rubidium uptake. Labeled ouabain binding was also shown to increase after stimulation of quiescent cells by serum or purified MSA. Conditions which interfere with the ability of the cells to accumulate potassium, such as the presence of the specific inhibitor, ouabain; incubation in potassium-free medium; or the presence of the potassium ionophore, valinomycin, were all demonstrated to inhibit the stimulation of DNA synthesis by serum or purified MSA. These results suggest that an early event in the stimulation of DNA synthesis by purified MSA is an activation of membrane Na+, K+-ATPase with a resulting accumulation of potassium ions inside the cell.
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PMID:Increased ouabain-sensitive 86Rubidium uptake after mitogenic stimulation of quiescent chicken embryo fibroblasts with purified multiplication-stimulating activity. 14 53

When human lymphocytes were incubated with rabbit red blood cells (RRBC) in vitro at 4 degrees C overnight, they adhered to form rosettes. 44 +/- 4.5% of thymocytes and o.7 +/- o.3% of peripheral blood lymphocytes (PBL) formed these rosettes. The rosette-forming cells (RFC) increased to 10--40% when the PBL were stimulated by mitogens. The increases were detected 4 h after culture and reached a maximum at 24 h, thus preceding significant increases in DNA syntheses. In another set of experiments, PBL were stimulated by a range of concentrations of each of 5 mitogens. The concentrations whick led to high DNA synthesis rates also generated high percentages of the rosettes. Lastly, PBL were activated by mitogens and the effect of inhibitors of DNA synthesis, protein synthesis and ATPase activity investigated. Only the latter could inhibit the generation of the RFC. In conclusion, 1y RRBC rosettes in mitogen stimulated human PBL were markers of activated lymphocytes, 2) the percentages of RFC could constitute a reliable index of mitogenic responses, and 3) this index was independent of the usual criteria of protein and DNA synthesis.
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PMID:Human lymphocytes subpopulations: rabbit red blood cell rosettes. 14 86

A deoxyribonuclease was purified approx. 800-fold from crude extracts of the bacterium Alcaligenes faecalis. The enzyme requires ATP and Mn2+; ATP could be replaced by any other ribo- or deoxyribo-nucleoside triphosphate, and Mn2+ could be replaced by Mg2+ in 0.1 M-Tris/HCl, pH 8.0 at 37 degrees C. The enzyme could degrade linear duplex or denaturated DNA, but was inactive with closed-circular duplex DNA from bacteriophase PM-2. In the course of nucleolytic activity, ATP was hydrolysed. We have measured deoxyribonuclease and adenoxine triphosphatase activity in the presence of various salts, and found that the amount of ATP hydrolysis associated with a given amount of deoxyribonuclease activity was decreased in the presence of tetraethylammonium ions. Since these ions decrease the stability of the DNA helix, we conclude that one function of the ATP hydrolysis is to unwind the DNA.
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PMID:An adenosine triphosphate-dependent deoxyribonuclease from Alcaligenes faecalis. 14 25

1. Primary heart cell cultures from neonatal hamsters yielded a heterogeneous cell population, containing muscle cells undergoing progressive differentiation, as well as non-muscle cells. 2. Addition of 5-bromo-2'-deoxyuridine, at an early stage, to such cultures enhanced the formation of beating sheets of differentiated muscle cells. Accumulation of myosin heavy chains and creatine kinase also occurred in the presence of the analogue. 3. To obtain these effects, the analogue had to be added during the initial rapid growth phase of the cells. Division of the treated cells then ceased when the cell numbers had approximately doubled. 4. Similar results were obtained with other inhibitors of DNA synthesis. Thus improved muscle cell cultures can be obtained by preventing non-muscle cells from overgrowing the cultures. 5. One effect caused only by 5-bromo-2'-deoxyuridine was a large increase in the Ca2+-stimulated ATPase (adenosine triphosphatase) activity which sedimented at low ionic strength. This increase was not due to a greater content of myofibrillar myosin, or to myosin isoenzyme changes, because purified myosin prepared from treated and untreated cultures did not exhibit the increased Ca2+-stimulated ATPase activity.
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PMID:Effects of 5-bromo-2'-deoxyuridine on beating heart cell cultures from neonatal hamsters. 14 80

1. Treatment of hamster heart cells in primary culture with 5-bromo-2'-deoxyuridine resulted in the greatly increased activity of a particulate Ca2+- or Mg2+-dependent ATPase (adenosine triphosphatase). 2. 5-Bromo-2'-deoxyuridine exerted these effects only when it was incorporated into cellular DNA, and then in a concentration-dependent manner. 3. Serially replated cells contained less of the activity (expressed as a function of total cell protein) than did the primary cultures, but the stimulation caused by 5-bromo-2'-deoxyuridine addition was much greater. 4. The affected enzyme was apparently localized in the plasma membrane of the cells with its active centre exposed to the outer environment [ecto-(ATPase) dependent on Ca2+ or Mg2+].5. The activity was unaffected by treatment with p-chloromercuriphenylsulphonate, ouabain andverapamil. 6. Ecto (5'-nucleotidase) activity was not increased by 5-bromo-2'-deoxyuridine treatment of cells, and ecto-(p-nitrophenyl phosphatase) activity was only slightly enhanced.
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PMID:5-bromo-2'-deoxyuridine-stimulated calcium ion- or magnesium ion-dependent ecto-(adenosine triphosphatase) activity of cultured hamster cardiac cells. 14 81

The first step in conversion of varphiX174 singlestranded DNA to the duplex replicative form in vitro is the synthesis of a nucleoprotein intermediate [Weiner, J. H., McMacken, R. & Kornberg, A. (1976) Proc. Natl. Acad. Sci. USA 73, 752-756]. We now demonstrate that dnaB protein (approximately one molecule per DNA circle) is an essential component of the intermediate and retains its ATPase activity. Synthesis of RNA primers, dependent on dnaG protein (primase), occurred only on DNA that had been converted to the intermediate form. In a coupled RNA priming-DNA replication reaction the first primer synthesized was extended by DNA polymerase III holoenzyme into full-length complementary strand DNA. In RNA priming uncoupled from replication, multiple RNA primers were initiated on a varphiX174 circle. The single dnaB protein molecule present on each DNA circle participated in initiation of each of the RNA primers, which appear to be aligned at regular intervals along the template strand. We propose that dnaB protein, once bound to the template, migrates in a processive fashion along the DNA strand, perhaps utilizing energy released by hydrolysis of ATP for propulsion; in this scheme the actively moving dnaB protein acts as a "mobile promoter" signal for dnaG protein (primase) to produce many RNA primers. Schemes are proposed for participation of dnaB protein both in the initiation of replication at the origin of the Escherichia coli chromosome and in the initiation of primers for nascent (Okazaki) fragments at a replication fork.
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PMID:Migration of Escherichia coli dnaB protein on the template DNA strand as a mechanism in initiating DNA replication. 14 14

Changes are reported in the DNA, RNA, protein and brush border enzymes in the small intestine mucosal lining cells and gut lumen, induced by maintaining rats on a diet containing chrysotile asbestos for 10 months. Intracellular levels of RNA, DNA and protein remained unchanged but significant alterations, consistent with a mineral-induced cytotoxicity, were found in the lumen level of DNA (increased) and RNA (decreased) in asbestos-treated rats. Most intracellular enzyme levels were consistently, but not significantly, elevated in animals maintained on diets containing asbestos whilst the activities within the lumen were significantly higher than those found in normal animals. The presence of cigarette smoke alone in the diet induced changes in intracellular RNA and lumen ATPase but the combined effect of cigarette smoke and asbestos was rarely different from the alterations induced by asbestos alone on the majority of parameters studied.
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PMID:A preliminary study of biochemical changes in the rat small intestine following long-term ingestion of chrysotile asbestos. 14 33

The residual effects of dihydroergotoxine mesylate (DHET: active substance of Hydergine), ethanol, and DHET + ethanol were investigated in aging male mice. Prolonged alcohol or DHET consumption was found to prolong hexobarbital sleeping time and increase oxygen consumption. Administration of alcohol combined with DHET inhibited the ability of each drug to prolong hexobarbital sleeping time and increase oxygen consumption. There were no significant differences between groups in forebrain synaptosomal (Na+-K+) adenosine- triphosphatase and acetylcholinesterase activity or cerebellar protein, DNA and RNA content. The relative proportion of phospholipid to protein in isolated myelin of the medulla was significantly reduced, whereas the sphingomyelin content of total phospholipid was highest in alcohol-treated mice. Conocomitant treatment of mice with alcohol combined with DHET prevented the physiological and neurochemical changes caused by alcohol and, in some cases, DHET, administered alone.
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PMID:Dihydroergotoxine and ethanol: physiological and neurochemical variables in male mice. 14 92

The combination effects of chlorpromazine (CPZ) and periphenazine (PPZ) with beta-lactam antibiotics (ampicillin, carbenicillin, cefazolin) and nalidixic acid group compounds (nalidixic acid, piromidic acid and pipemidic acid) have been estimated to be synergistic by the filter paper strip-agar diffusion method (Dye's method) with Escherichia coli and Pseudomonas aeruginosa as test organisms. The observed synergism might be associated with their inhibition of various enzymes including ATPase and DNAase as well as with their specific binding to DNA. Similar synergistic effects of CPZ and PPZ have been shown by the broth dilution method. Based on these findings, it seems to be a fascinating project to devise a new phenothiazine drug without influence in mental disease that will have a greater measure of synergistic effect when combined with the above-studied antibacterial agents.
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PMID:Synergistic effects of chlorpromazine and perphenazine on several chemotherapeutic agents. I. General profile of the effects measured by the filter paper strip-agar diffusion method with Escherichia coli and Pseudomonas aeruginosa. 14 36

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