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401.
以2种配体去甲基斑蝥酸钠(Na2DCA=7-氧杂二环[2.2.1]庚烷-2,3-二甲酸钠)和咪唑(IM),分别与镍(Ⅱ)和镉(Ⅱ)的醋酸盐通过溶液法合成了2种配合物[Ni(IM)(DCA)(H2O)2]·2H2O(1),[Cd2(IM)4(DCA)2]·2H2O(2)。应用元素分析、热重分析、红外光谱及X-射线单晶衍射法对配合物的组成和结构进行了表征。配合物1与2的中心离子分别与咪唑的亚胺氮原子、去甲基斑蝥酸根的羧基氧原子和醚键氧原子配位,配位数均为6,分别为单核(1)和双核(2)配合物。通过紫外光谱法、荧光光谱法和粘度法研究了配合物与DNA的相互作用。结果表明,配合物能通过部分插入模式与DNA发生较强的结合作用(Kb:5.51×103(1)、1.01×103(2)L·mol-1)。同时,利用荧光光谱法研究了配合物与牛血清白蛋白(BSA)的相互作用。配合物能与BSA发生强烈的相互作用(KA:1.91×105(1)和6.17×105(2)L·mol-1),结合位点数均为1。测试了配合物对人肝癌细胞(SMMC7721)和人乳腺癌(MCF-7)的体外抗增殖活性。结果显示,配合物对不同癌细胞具有选择性抑制作用。镍配合物(1)对SMMC7721的抗癌活性较去甲基斑蝥酸钠有明显提高。  相似文献   
402.
采用荧光光谱、同步荧光光谱、紫外-可见吸收光谱及分子模拟技术研究了模拟生理条件下丽春红2R(P2R)与牛血清白蛋白(BSA)的相互作用。实验结果表明,P2R-BSA体系的荧光猝灭机制为内源荧光猝灭,猝灭原因为静态猝灭和非辐射能量转移;计算了不同温度下体系的结合常数Ka及结合位点数n;根据热力学参数推断出作用力类型;求出室温下荧光给体-受体间的结合距离;同步荧光法证实丽春红2R对BSA构象未产生影响;分子模拟研究结果表明二者间的主要作用力为氢键和疏水作用力。  相似文献   
403.
Three capillary zone electrophoresis (CZE) methods of the frontal analysis (FA), vacancypeak (VP) and simplified Hummel-Dreyer (SHD) were applied to investigate interaction betweenbovine serum albumin (BSA) and lomefloxacin, the experimental condition was established after alarge number of tests. Based on the site-binding model, the binding parameters were measuredaccording to the site model by Scatchard.  相似文献   
404.
应用静态荧光光谱研究了嵌段共聚物PluronicP103对牛血清白蛋白(BSA)荧光光谱的猝灭。研究表明,PluronicP103对BSA的荧光有猝灭作用,动态猝灭是引起BSA荧光猝灭的主要原因。发现嵌段共聚物PluronicP103在水溶液中的蔟集状态影响其与BSA的相互作用,以胶团形式存在的PluronicP103对BSA的猝灭作用更强。  相似文献   
405.
荧光法研究磷酰化黄酮与牛血清白蛋白的相互作用   总被引:1,自引:1,他引:0  
用荧光猝灭法研究了5,7-二羟基磷酰化黄酮对牛血清白蛋白的相互作用。根据荧光猝灭双倒数图计算了磷酰化黄酮与牛血清白蛋白的结合常数。根据Foester能量传递原理计算出磷酰化黄酮在牛血清白蛋白的结合位置。  相似文献   
406.
应用荧光光谱法研究了盐酸表阿霉素与血清白蛋白之间的相互作用,求得它们之间的结合常数KA=2.342×10~4(t=25℃),KA=1.993×10~4(t=35℃),KA=1.638×10~4(t=45℃),以及金属离子对结合常数的影响,确定了药物与血清白蛋白之间的相互作用力,并根据Forster非辐射能量转移理论求出给体-受体间的结合距离r=4.25 nm和能量转移效率E=0.018。又进一步在生理条件下成功的测定了药物在血清与尿样中的含量。  相似文献   
407.
Phase analysis, spectroscopic, and light scattering methods are applied to investigate the peculiarities of the interaction of oligochitosan (OCHI) with native and preheated bovine serum albumin (BSA) as well as the conformational and structural changes of BSA in BSA/OCHI complex. As shown, untreated BSA binds with OCHI mainly forming soluble electrostatic nanocomplexes, with the binding causing an increase in BSA helicity without a change in the local tertiary structure and thermal stability of BSA. In contrast, soft preheating at 56 °C enhances the complexation of BSA with OCHI and slightly destabilizes the secondary and local tertiary structures of BSA within the complex particles. Preheating at 64 °C (below the irreversible stage of BSA thermodenaturation) leads to further enhancement in the complexation and formation of insoluble complexes stabilized by both Coulomb forces and hydrophobic interactions. The finding can be promising for the preparation of biodegradable BSA/chitosan-based drug delivery systems.  相似文献   
408.
This study relates interfacial interactions of bovine serum albumin (BSA) molecules in dilute solutions with its dilatational rheology. Dynamic surface tension and the associated dilational elastic modulus and viscosity for BSA and mixtures of BSA with Hofmeister electrolytes—NaCl, NaClO4, Na2SO4, NaF and Na2HPO4 have been studied using a sinusoidal surface compression and expansion for frequencies ranging from 0.01 to 0.4 Hz. at solution/air interface. In all the BSA + electrolyte systems, both the elastic modulus and viscosity show unusually high values compared with pure BSA or pure electrolytes. In the presence of NaF and Na2SO4 the viscosity of protein increases almost by 50–80-fold and the corresponding elastic modulus also changes by 30–50-fold. Hydrated Hofmeister ions surely influence the measured rheological properties. In addition, the synergistic effect of the hydrated protein and the vicinal hydrated electrolytes possibly contribute to the high viscosity and elasticity due to change in dynamics of these assemblies. Thus the behavior of BSA is effected by salts in different ways, especially due to the dynamics and strength of the water molecules in the assembly.  相似文献   
409.
The adsorption of bovine serum albumin (BSA) on platinum surfaces with a root-mean-square roughness ranging from 1.49nm to 4.62nm was investigated using quartz crystal microbalance with dissipation (QCM-D). Two different BSA concentrations, 50microg/ml and 1mg/ml, were used, and the adsorption studies were complemented by monitoring the antibody interaction with the adsorbed BSA layer. The adsorption process was significantly influenced by the surface nano-roughness, and it was observed that the surface mass density of the adsorbed BSA layer is enhanced in a non-trivial way with the surface roughness. From a close examination of the energy dissipation vs. frequency shift plot obtained by the QCM-D technique, it was additionally observed that the BSA adsorption on the roughest surface is subject to several distinct adsorption phases revealing the presence of structural changes facilitated by the nano-rough surface morphology during the adsorption process. These changes were in particular noticeable for the adsorption at the low (50microg/ml) BSA concentration. The results confirm that the nano-rough surface morphology has a significant influence on both the BSA mass uptake and the functionality of the resulting protein layer.  相似文献   
410.
The activity of lipoprotein lipase (LPL), an enzyme responsible for lipoprotein metabolism, would vary in diseases and metabolic disorders. For determination of LPL activity, a highly sensitive high performance liquid chromatography (HPLC) method using a fluorescent reagent, 4-nitro-7-piperazino-2,1,3-benzoxadiazole (NBD-PZ) was applied to determinate the oleic acid (OA) generated from triolein by LPL activity without multiple solvents extraction step. We studied the optimal conditions of the reaction including the effect of emulsifiers, deproteinizing solvents, and the concentration of bovine serum albumin (BSA). Ten millimolar concentrations of triolein, 5% of BSA, 1% of Gum arabic (GA), and acetonitrile showed the optimum conditions for measuring the LPL activity. The accuracy values for the determination of LPL activity in 10 microL of rat post heparin plasma were 108.73 approximately 114.36%, and the intra- and inter-day precision values were within 1.28% and 2.91%, respectively. The limit of detection was about 4.53 nM (signal-to-noise ratio 3). The proposed method was applied to determination of LPL activity in post heparin plasma of normal and streptozotocininduced diabetic rats associated with 52.3% reduction. The established assay system could be used for determining LPL activity in different physiological and pathological conditions to clarify the relationship between LPL activity and diabetes mellitus.  相似文献   
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