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排序方式: 共有31条查询结果,搜索用时 31 毫秒
1.
A flow-injection system is described for the determination of d-mannitol. Mannitol dehydrogenase is immobilized on poly(vinyl alcohol) beads and packed in a column (5 cm × 4 mm i.d.). The NADH formed is detected fluorimetrically. The response is linear between 5 × 10?7 and 1 × 10?4 M mannitol and the detection limit is 1 × 10?7 M. The throughput is 30 samples per hour. The reactor is stable for at least 8 weeks.  相似文献   
2.
Abstract. Photodimerization of thymine in aqueous solution in the presence of tyrosine was studied with monochromatic UV irradiation. The total dimer formation was sensitized in the presence of tyrosine. The action spectrum of sensitized total dimer formation has a peak near 280 nm corresponding to the absorption maximum of tyrosine. Triplet quenchers reduced the sensitization substantially. It seems probable that tyrosine-sensitized photodimerization of thymine occurred via triplet-triplet energy transfer from tyrosine to thymine.  相似文献   
3.
Extraction of carbazole in heptane was performed at 25±1°C with an aqueous dimethyl sulfoxide (DMSO) medium containing -cyclodextrin (CD) at consecutive concentrations in the range of 0–10 mM. The fluorescence intensity of carbazole remaining in the heptane phase was measured by synchronous scanning fluorimetry. The apparent formation constant (K f) for a 1:1 carbazole: CD inclusion complex in water-DMSO medium was determined by using a linear plot of the distribution ratio calculated from the fluorescence intensities vs. the -CD concentration. The values thus obtained ranged from 477 M–1 in a 10% v/v DMSO medium to 12.1 M–1 in a 60% v/v medium. Good linear relationships were observed between logK f and the DMSO concentration ([DMSO]), and also between logK f and the logarithm of the distribution coefficient (K d) for carbazole. The formation constant in 100% water was estimated to be approximately 1.0×103 M–1 on the basis of the logK f vs. [DMSO] and the logK f vs. logK d correlations.  相似文献   
4.
Simple separation of carbazole and anthracene from monosubstituted anthraquinones is achieved through the application of the zone-melting technique used biphenyl as a medium. Determination limits for both compounds measured by synchronous fluorimetry are 2 μg g?1 in 2-methyl-, 2-ethyl-, 1-hydroxy- and 1-chloroanthraquinones, and 10 μg g?1 in another four derivatives.  相似文献   
5.
We prove additivity violation of minimum output entropy of quantum channels by straightforward application of \({\epsilon}\) -net argument and Lévy’s lemma. The additivity conjecture was disproved initially by Hastings. Later, a proof via asymptotic geometric analysis was presented by Aubrun, Szarek and Werner, which uses Dudley’s bound on Gaussian process (or Dvoretzky’s theorem with Schechtman’s improvement). In this paper, we develop another proof along Dvoretzky’s theorem in Milman’s view, showing additivity violation in broader regimes than the existing proofs. Importantly,Dvoretzky’s theorem works well with norms to give strong statements, but these techniques can be extended to functions which have norm-like structures-positive homogeneity and triangle inequality. Then, a connection between Hastings’ method and ours is also discussed. In addition, we make some comments on relations between regularized minimum output entropy and classical capacity of quantum channels.  相似文献   
6.
We developed a growth method for forming a GaAs quantum well contained in an AlGaAs/GaAs heterostructure nanowire using selective-area metal organic vapor phase epitaxy. To find the optimum growth condition of AlGaAs nanowires, we changed the growth temperature between 800 and 850 °C and found that best uniformity of the shape and the size was obtained near 800 °C but lateral growth of AlGaAs became larger, which resulted in a wide GaAs quantum well grown on the top (1 1 1)B facet of the AlGaAs nanowire. To form the GaAs quantum well with a reduced lateral size atop the AlGaAs nanowire, a GaAs core nanowire about 100 nm in diameter was grown before the AlGaAs growth, which reduced the lateral size of AlGaAs to roughly half compared with that without the GaAs core. Photoluminescence measurement at 4.2 K indicated spectral peaks of the GaAs quantum wells about 60 meV higher than the acceptor-related recombination emission peak of GaAs near 1.5 eV. The photoluminescence peak energy showed a blue shift of about 15 meV, from 1.546 to 1.560 eV, as the growth time of the GaAs quantum well was decreased from 8 to 3 s. Transmission electron microscopy and energy dispersive X-ray analysis of an AlGaAs/GaAs heterostructure nanowire indicated a GaAs quantum well with a thickness of 5−20 nm buried along the 〈1 1 1〉 direction between the AlGaAs shells, showing a successful fabrication of the GaAs quantum well.  相似文献   
7.
Molecular shuttles based on the motor protein kinesin and microtubule filaments have the potential to extend the lab-on-a-chip paradigm to nanofluidics by enabling the active, directed and selective transport of molecules and nanoparticles. Based on experimentally determined parameters, in particular the trajectory persistence length of a microtubule gliding on surface-adhered kinesin motors, we developed a Monte-Carlo simulation, which models the transport properties of guiding structures, such as channels, rectifiers and concentrators, and reproduces the properties of several experimentally realized systems. Our tool facilitates the rational design of individual guiding structures as well as whole networks, and can be adapted to the simulation of other nanoscale transport systems.  相似文献   
8.
9.
A flow-injection system for the determination of l-alanine is described. Alanine dehydrogenase is immobilized on poly(vinyl alcohol) beads and used in a packed-bed enzyme reactor. The system responds linearly to injected samples (50 μl) in the concentration range 0.5–500 μM. The maximum throughput was 40 samples per hour. The immobilized enzyme reactor was stable for at least 6 weeks. Its usefulness for assay of l-alanine in serum and beverages is described.  相似文献   
10.
A fluorimetri method is described for the determination of glycerol, 1,2-propanediol and triglycerides in serum by high-performance liquid chromatography with an on-line post-column reactor containing immobilized glycerol dehydrogenase. Before separation, triglycerides are cleaved with lipase and esterase. The polyhydric alcohols are separated from each other on a Finepak SIL C18 (10 μm) column with water as eluent. The NADHI produced from the enzymatic reaction is monitored by fluorimetry. Calibration curves are linear between 0.01 mM and 1.0 mM for glycerol or 2.0 mM for 1,2-propanediol. The method gave satisfactory results for control sera.  相似文献   
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