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31.
甲基营养细菌No1甲胺脱氢酶是以色氨酸-色氨酰醌为辅基的一种特殊氧化还原酶.粗酶液经纯化后,其比活力和收得率分别为5.1nmol·g-1和28%.该酶的分子量为67000,等电点为8.3和8.5,组成它的大、小两个亚基的分子量分别为37000和15000.甲胺脱氢酶有较好的耐热性,它能催化包括一级甲胺和二胺在内的底物反应,与甲胺反应的Km值为26.6μmol·L-1,最适pH为8.0.其酶催化反应可被Cu2+抑制.该酶的吸收光谱是,在328nm和426nm呈现两个特征峰 相似文献
32.
A simple, indirect fluorescence detection method has been developed for detecting specific mono-amino sugars (D-glucosamine, D-galactosamine, D-mannosamine) following chromatographic separation. The eluting amino sugars release L-tryptophan (L-Trp) from a copper-tryptophan complex which is introduced postcolumn. Analyte detection is based on measuring the increase in L-Trp fluorescence, which is quenched when complexed with copper. Two tryptophan analogues, 5-hydroxy-L-tryptophan (5-HTP) and DL-5-methoxytryptophan (5-MTP), were also evaluated as postcolumn reagents. 5-MTP was found to be a suitable alternative to L-Trp for the detection of these mono-amino sugars. Detection limits for D-glucosamine, D-galactosamine, and D-mannosamine are in the range of 0.15-0.30 nmol injected. 相似文献
33.
We report an ab initio simulation study of the ultrafast broad bandwidth ultraviolet stimulated resonance Raman spectra (SRRS) of l ‐tyrosine, l ‐tryptophan, and trans‐l ‐tryptophan‐l ‐tyrosine (WY) dipeptide. Two‐pulse one‐dimensional SRRS and three‐pulse two‐dimensional SRRS that reveal inter‐residue and intra‐residue vibrational correlations are simulated using electronically resonant or pre‐resonant pulse configurations that select the Raman signal and discriminate against excited state pathways. Multimode effects are incorporated via the cumulant expansion. The two‐dimensional SRRS technique is more sensitive to residue couplings than spontaneous Raman. Copyright © 2013 John Wiley & Sons, Ltd. 相似文献
34.
AbstractThe interaction of pioglitazone hydrochloride bound to tryptophan residues and tyrosine residues in bovine transferrin was investigated using synchronous fluorescence spectroscopy at various temperatures (298, 310, and 318?K). From binding constants and thermodynamic parameters, it was shown that 1:1 stable compound was formed by the electrostatic force interaction of pioglitazone hydrochloride bound to tryptophan residues and tyrosine residues in bovine transferrin. The extent of binding between pioglitazone hydrochloride and tryptophan residues in bovine transferrin was more than that between pioglitazone hydrochloride and tyrosine residues in bovine transferrin. At 310?K, the fluorescence quenching ratio number of tyrosine residues and tryptophan residues in bovine transferrin were 47.52% and 54.19%, respectively, which indicated that the fluorescence contribution of tryptophan residues was greater. At 310?K, pioglitazone hydrochloride-tyrosine residues(in bovine transferrin) binding rate were 55.60–73.82%, and the combined model was W?=??0.0315R2???0.1520R?+?0.7385. The value of Hill’s coefficients was greater than 1, which suggested that there was a positive cooperativity between pioglitazone hydrochloride and subsequent ligands. The results of molecular docking were consistent with that of experimental calculation. 相似文献
35.
The protein, hen egg white lysozyme, on photoexcitation undergoes electron transfer with menadione (2-methyl-1,4-naphthoquinone), a widely known anticancer drug. With the addition of menadione the fluorescence of lysozyme is quenched with the simultaneous formation of an excited state charge-transfer complex in the longer wavelength and a ground state complex. The former is further evident from laser flash photolysis studies, which indicate a tryptophan to menadione electron transfer. From fluorescence quenching studies the binding constant is found to be ∼1.7×104 M−1 with the corresponding changes in enthalpy (ΔH°) and entropy (ΔS°) as 12.24 kJ mol−1 and 124.12 J mol−1 K−1, respectively, indicative of an entropy-driven process. The circular dichroism studies also show some structural changes with increase in α-helical content in the protein on interaction with menadione. Finally, docking studies give some insight into the role of Trp 108 of lysozyme in the interaction. 相似文献
36.
37.
基于尿嘧啶作为一种碱基,具备一定的分子识别能力,制备了一种新颖的尿嘧啶共价修饰电极,用X射线光电子能谱和电化学方法进行了表征,并研究了酪氨酸、色氨酸、儿茶酚胺(如多巴胺,肾上腺素,去甲肾上腺素)及相关的化合物尿酸、抗坏血酸在该电极上的电化学行为,获得相应的氧化电位、电流灵敏度、线性范围和检测限等信息。其中,色氨酸检测线性范围:1.8 - 120 mM,检测限(s/n=3):0.8 mM;酪氨酸检测线性范围:1.8 - 89mM,检测限(s/n=3):0.8 mM。实验表明,尿嘧啶修饰电极能催化氧化上述电活性物质,但催化能力不同,据此,我们讨论了尿嘧啶与上述物质的相互作用,详细探讨了催化机理,扩展了对基于分子识别的传感器的研究。 相似文献
38.
Hilda Marta Szabo Raghida Lepistö Tuula Tuhkanen 《International journal of environmental analytical chemistry》2016,96(3):257-270
This work investigates the use of HPLC-SEC to characterise dissolved organic matter (DOM) of complex wastewater effluents. A silica-based column, sodium acetate eluent and multiple detections were employed: UV-254 absorbance for humictype, and tryptophan-like (Ex/Em = 270/355) and tyrosine-like (Ex/Em = 270/310) fluorescence for protein type compounds. Effects of eluent pH, eluent ionic strength and injection volume on separation efficiency were tested. Humic-type and protein-type fractions were clearly differentiated and eluted within and out of calibration range. Eluent ionic strength had the greatest influence on global resolution; the lowest eluent concentration of 0.01 M produced the best separation for all wastewater effluents tested at any detection. UV-254 absorbance was higher at neutral and basic eluent pH while tryptophan-like fluorescence depended on the sample composition rather than on the eluent pH or ionic strength. Tyrosine-like fluorescence decreased significantly with the increase of eluent ionic strength. Accurate molecular weight measurements could not be done, the separation being influenced by secondary interactions, but could be approximated using separate calibrations with sodium salts of polystyrene-sulfonates and protein standards. The results show that this method is suitable for determining DOM in wastewater at low eluent concentrations (up to 0.03 M), at neutral or slightly basic pH. 相似文献
39.
Synthetic oligopeptides with a tryptophan residue at the C-terminus have been used for the synthesis of gold and silver nanoparticles at pH 11. The tryptophan residue in the peptides is responsible for the reduction of metal ions to the respective metals, possibly through electron transfer. A mechanistic pathway has been proposed to explain the reductive properties of the tryptophan moiety of the peptide based on some spectroscopic techniques, such as UV-visible and fluorescence spectroscopy. This study reveals that some of the peptide molecules are converted to its corresponding ditryptophan, kynurenine form and some cross-linked products, all of which are highly fluorescent species. The resultant peptide-functionalized metal nanoparticles have also been characterized by UV-visible spectroscopy, transmission electron microscopy, and Fourier transform IR spectroscopy and thermogravimatric analysis. 相似文献
40.