CAS:7782-44-7 - FACTA Search

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The photooxidation of diphenylamine is acetonitrile and methanol using Hypocrellin A as sensitizer will be reported in this paper. The products in the two solvents were isolated and identified. The reaction mechanisms were investigated. In acetonitrile, diphenylamine was oxidized by singlet oxygen to form N-phenyl-p-benzoquinonimine. In methanol, N-phenyl-p-benzoquinonimine was produced predominantly through a mechanism irrelevant to singlet oxygen. A small amount of diphenylamine reacted with methanol and singlet oxygen to give a novel product: N-phenyl-2-methoxy-p-benzoquinonimine.
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PMID:Photochemistry of hypocrellin A (IV)--Hypocrellin A-sensitized photooxidation of diphenylamine. 317

Oxygen-17 isotope was introduced into the alpha-carboxyl group of glycine, 1-phenylalanine, 1-leucine and 1-tyrosine by acid catalyzed exchange of 17O from H2O(17) or by acid hydrolysis of respective amino acid methyl esters in H2O(17). Quantitative enrichment of glycine was achieved by acid hydrolysis of amino acetonitrile in H2O(17). For alpha-amino protection in amino acids t-butoxycarbonyl (Boc) group was employed for 17O labeled enkephalin synthesis. Five analogues of Leu-enkephalins (I-V) labeled with 17O at different amino acid residues were synthesized by solid phase method. 17O n.m.r. spectra were measured at 24.4 and 67.8 MHz for Leu-enkephalins 17O labeled at Gly2 and Phe4 positions. A downfield shift was observed for 17O labeled Gly2 Leu-enkephalin upon heating. This shift is indicative of the rupture of intramolecular hydrogen bonds. The preliminary results confirm the hypothesis that an intramolecular hydrogen bond exists between the carbonyl group of Gly2 and NH group of Leu5.
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PMID:Synthesis of 17O isotope labeled Leu-enkephalin and 17O n.m.r. 322 Jun 55

Palm oil carotenoids are analyzed by nonaqueous reversed-phase high-performance liquid chromatography (NARP-HPLC) with UV/vis diode-array detection. Isocratic elution with 60% acetonitrile/35% methanol/5% methylene chloride at 2 mL/min on a 25-cm C18 column results in an analysis time of 30 min. Identification is made through absorption spectra and chromatographic elution behaviors, for example, polyenic pi conjugation, dipole moment of end-groups, and oxygen function on the chromophores. At least 12 carotenoids are identified with alpha- and beta-carotene as the dominant carotenoids (1:2 ratio). Several mono- and di-epoxides of alpha- and beta-isomers and hydrocarbon carotenes are found, including the UV-absorbing phytoene identified by spectral substraction. cis-Isomerization is found and discussed in the light of spectral evidence. The effect of saponification time on the amount of extracted carotenes is investigated. Quantitation results in a combined alpha- and beta-carotene concentration of at least 506 ppm. The detection limit for beta-carotene is 31 ng.
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PMID:Analysis of palm oil carotenoids by HPLC with diode-array detection. 322 10

A liquid chromatographic (LC) method with electrochemical detection in the reductive mode was developed for the quantitative determination of dimetridazole (DMZ) and its major metabolite (HMMNI) at residue levels in pork tissue. For blood plasma, a sample is precipitated with 2 volumes of acetonitrile and centrifuged, and a diluted aliquot of the supernatant liquid is chromatographed. For muscle, a 10 g sample is extracted 3 times with dichloromethane. After evaporation of the combined extracts, the residue is redissolved in a mixture of hexane and mobile phase (0.3% TEA in 0.6M ammonium acetate pH 5.0 and acetonitrile, 85 + 15) and centrifuged, and an aliquot of the lower phase is chromatographed. Chromatography is accomplished using valve switching with 2 liquid circuits, employing the same mobile phase for both. The sample is deaerated by sparging with helium under slight positive pressure to prevent rediffusion of the oxygen. The sample is first loaded into a deoxygenator and the flow is stopped for complete deoxygenation. The flow is then resumed to transfer the sample into the first, low back-pressure column (ODS, 10 microns, 4.6 x 200 mm). Switching the valve at this point removes the deoxygenator from the circuit and connects the first column to a second one (ODS, 5 microns, 4.6 x 150 mm) in tandem. After the effluent is passed through a second deoxygenator to reduce the residual oxygen in the mobile phase, it is monitored by an electrochemical detector with a screened wall jet cell and a gold mercury electrode, set at -1.2 V.(ABSTRACT TRUNCATED AT 250 WORDS)
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PMID:Dimetridazole residues in pork tissue. I. Assay by liquid chromatography with electrochemical detector. 324 Sep 70

A high-performance liquid chromatographic system is presented for determination of organonitro pesticides, metabolites and industrial chemicals having a variety of chemical structures. The compounds are chromatographed on a C8 column with an acetonitrile-aqueous ammonium monochloroacetate gradient. The chromatographic responses of the compounds are monitored indirectly by oxidative detection of the coulometrically reduced organonitro functionality by means of a porousgraphite detector. Three nitrophenols (2,4-dinitrophenol, 4,6-dinitro-o-cresol and dinoseb), a dinitrophenyl aliphatic ester (binapacryl) and a nitroaniline (dicloran) were detected at low nanogram levels (3-10 ng for 50% recorder full-scale deflection). This technique overcomes the problems of high background currents and oxygen interference, observed in the direct reductive detection of organonitro compounds.
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PMID:Oxidative detection of coulometrically reduced organonitro pesticides in reversed-phase high-performance liquid chromatography. 324 94

Oral acetone exposure delays and potentiates acetonitrile toxicity in rats. Results of previous pharmacokinetic studies suggested that acetone exerted a biphasic effect on the metabolism of acetonitrile to cyanide; the presence of acetone in vivo appeared to inhibit the metabolism of acetonitrile to cyanide, whereas the disappearance of acetone from serum was followed by stimulation of acetonitrile metabolism. The current experiments were designed to characterize further the metabolism of acetonitrile to cyanide and the effects of acetone and other compounds upon this metabolism. Liver microsomes were isolated and pooled 24 hr after oral pretreatment of female Sprague-Dawley rats (180-250 g) with acetone (1960 mg/kg) or water. Microsomal metabolism of acetonitrile to cyanide was found to be oxygen and NADPH dependent, and heat-inactivated tissue was unable to catalyze the reaction. NADH antagonized the NADPH-dependent metabolism of acetonitrile. The metabolism of acetonitrile to cyanide was linear with protein concentrations of 0-8 mg per incubation. Following a characteristic lag period of 10 min, the reaction was linear from 15 to 30 min. This metabolism was inhibited by carbon monoxide, metyrapone and SKF 525-A. Acetone pretreatment (-24 hr) in vivo increased the apparent Vmax for acetonitrile metabolism without affecting the apparent Km. When added in vitro, acetone competitively inhibited the metabolism of acetonitrile, with a KI of 0.41 mM. Dimethyl sulfoxide (KI = 0.51 mM) and ethanol (KI = 0.11 mM) were also competitive inhibitors of acetonitrile metabolism, and aniline HCl (KI = 4.77 microM) appeared to be a mixed inhibitor. These data are consistent with the hypothesis that the metabolism of acetonitrile to cyanide is mediated by a specific acetone-inducible isozyme of cytochrome P-450.
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PMID:Microsomal metabolism of acetonitrile to cyanide. Effects of acetone and other compounds. 335 89

Benzo[a]pyrene (BaP), a well-known carcinogen, is frequently measured as an "indicator" of the potential dermal tumorigenicity of a sample. The present sequential high-performance liquid chromatography--high-performance liquid chromatography method overcomes problems in trace-level sample enrichment and recovery corrections encountered earlier. An amount of 5 g of naphtha or fuel oil is diluted to 10 ml with dichloromethane and spiked with a small quantity (ca. 0.25 micrograms) of 14C-labeled BaP tracer. A BaP-enriched fraction is obtained from a 1-ml aliquot of this sample by semipreparative chromatography on a Partisil PAC 10 column with dichloromethane-hexane (10:90) as the eluent, and concentrated to exactly 0.3, 0.5, or 1.0 ml in acetonitrile. Quantitation is performed using a reversed-phase Vydac 201 TP 5415 column with acetonitrile-water (75:25) as eluent and a Waters Model 420 E/420 AC fluorescence detector, employing an excitation/emission filter pair of 360/425 nm. The recovery of the radiolabeled tracer is evaluated by combustion of 50 microliter of the final isolate in pure oxygen, collection of the liberated 14CO2 in an alkaline desorber, and liquid scintillation counting. The recovery of BaP normally exceeded 90%, but values as low as ca. 50% were occasionally observed. Potential matrix interferences in the recovery determination were eliminated by sample combustion. The nominal precision of the overall method is approximately +/- 30% relative standard deviation at a BaP concentration of 30 ppb. The nominal analysis time for a single sample is approximately 4 h.
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PMID:Liquid chromatographic determination of benzo[a]pyrene at part-per-billion concentrations in highly refined coal- and petroleum-derived fuels. 355 98

The determination of ascorbic acid by liquid chromatography (LC) was improved by performing the analysis in the presence of solvents that had been purged with argon to reduce the concentration of oxygen. This methodological modification eliminated the oxidation of ascorbic acid during the chromatographic procedure and reduced the minimum detection level to 1 microgram. Solutions of ascorbic acid have been successfully stabilized for 67 days by addition of dithiothreitol to a deaerated solution of water-acetonitrile (25 + 75 v/v), sealed under argon in amber vials and stored at -20 degrees C. In a second independent study, a procedure for the extraction of ascorbic acid from nonfat dry milk in a single step was developed. The ascorbic acid content of Nonfat Dry Milk (SRM 1549) was determined by LC, using the method of standard additions. The mean ascorbic acid content was 54 +/- 5 micrograms/g of sample. Analysis of variance of the analytical results indicates that there is a significant continual increase in the content of the ascorbic acid in each bottle from first to last sample.
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PMID:Stabilization of ascorbic acid and its measurement by liquid chromatography in nonfat dry milk. 368 Jan 14

The 1-nitroacridine nitracrine [NC,1-nitro-9-(dimethylaminopropyl-amino)acridine] is a potent hypoxia-selective cytotoxic agent in culture, but lacks activity against hypoxic tumor cells in vivo at therapeutically accessible doses. To clarify reasons for this failure in vivo the metabolism of NC was investigated in stirred suspension cultures of Chinese hamster ovary cells, in EMT-6 spheroids, and in mice. One major low molecular weight metabolite (identical to that generated by NaBH4/Pd/C reduction) was observed in hypoxic (less than 10 ppm O2) single cell suspensions, while [G-3H-acridinyl]NC formed trichloroacetic acid- and acetonitrile-insoluble macromolecular adducts (MA) at a rate seven-fold higher than in aerobic (20% O2) cultures. Formation of these adducts correlated with cytotoxicity under air or nitrogen, and hence may provide a dosimeter for NC-induced damage. Autoradiographic investigation of the distribution of MA in spheroids equilibrated with 5% O2 showed that the label was restricted to the outer cell layers rather than being localized in the hypoxic central region. Thus metabolic activation is probably too rapid, even in well-oxygenated cells, to allow adequate distribution to hypoxic microenvironments in tumors. In mice, levels of MA were higher in liver, kidney, spleen and lung than in Lewis lung tumors, indicating that oxygen concentration does not exert a dominant influence on relative rates of metabolic activation in vivo. The development of nitroacridines with useful hypoxic selectivity in vivo will require identification of analogs for which reductive metabolism is more completely inhibited at oxygen concentrations found in normal tissues.
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PMID:Reductive metabolism and hypoxia-selective toxicity of nitracrine. 374 44

We have characterized certain catalytic properties of cytosolic epoxide hydrolases purified from untreated and clofibrate-treated mouse liver. The enzyme activity was found to be sensitive to oxygen, but nitrogen-saturated buffers containing dithiothreitol maintained high activity for at least 12 h at 0 degrees C. Linearity of the hydration of trans-stilbene oxide with time and protein was established, the pH optimum was broad (6.5 to 7.4) and the temperature optimum was close to 50 degrees C for both forms. The activity was independent of ionic strength, with the exception of the control form in the absence of dithiothreitol, where a lower activity was observed at low ionic strength. The activity decreased when ethanol was replaced by acetone or acetonitrile as solvent for the substrate. Tetrahydrofuran was found to be highly inhibitory, while dimethylsulfoxide had less pronounced effects. The apparent Km values were 4.9 microM, 73 microM and 1980 microM for the control form with trans-stilbene oxide, cis-stilbene oxide and styrene oxide as substrates, respectively. The Km values for the enzyme from clofibrate-treated mice were in the same range, although the V values were higher for all three substrates with this form. The highest turnover was found for trans-beta-propylstyrene oxide as substrate, followed by trans-beta-ethylstyrene oxide. Little or no activity was observed with benzo[a]pyrene 4,5-oxide or cholesterol 5,6 alpha-oxide. The enzymes were found to be sensitive to 5,5'-dithiobis(2-nitrobenzoic acid) and a phenylmercuric salt. alpha-Naphthoflavone, beta-naphthoflavone and chalcone derivatives also inhibited the activity, while none of the compounds known to activate microsomal epoxide hydrolase activated the cytosolic forms.
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PMID:Properties of cytosolic epoxide hydrolase purified from the liver of untreated and clofibrate-treated mice. Characterization of optimal assay conditions, substrate specificity and effects of modulators on the catalytic activity. 401 80

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