尺寸可控的金纳米粒子在功能化的MWNTs表面的自组装

提出了一个有效的、以晶种媒介的光化学法可控生长不同尺寸的胶体金纳米粒子在多壁碳纳米管(MWNTs)表面的自组装.方法基于羧基化的MWNTs以双官能团巯基乙酸分子化学修饰而连接上巯基,随后,不同尺寸的胶体金纳米粒子以共价结合的方式分别被直接锚定在其表面,从而获得良好的Au/MWNTs杂化材料.通过UV-Vis光谱、TEM和XRS等技术对胶体金纳米粒子、Au/MWNTs复合物及其自组装过程的表征,详细研究了金纳米粒子尺寸对功能化MWNTs表面自组装的影响,结果表明,直径为2.5～5.2nm范围很好分散的金纳米粒子能够很好自组装在平均直径约20nm的功能化MWNTs表面上.同时探讨了双官能团分子的化学修饰和金纳米粒子对MWNTs表面自组装的驱动力。     

微波辐射高效共价固定青霉素酰化酶

为提高青霉素酰化酶的共价固定化效率, 在微波辐射条件下将酶蛋白共价固定于介孔泡沫硅(MCFs)的孔道中. 通过正硅酸四乙酯水解缩合制备介孔泡沫硅, 再于微波辅助下将青霉素酰化酶共价固定在其孔道中. 以固定化酶相对活力和活力回收为指标, 考察了加酶量、固定化温度、微波辐射时间等条件对酶固定化效率的影响. 实验结果表明: 当加酶量为60 mg/g, 固定化温度为20 ℃, 微波辐射140 s, 固定化酶相对活力达到178.1%, 表观活力为1191.3 U/g(以湿重计). 与常规方法相比, 微波辅助固定化酶时, 固定化酶相对活力提高34.5%, 固定化时间亦大幅缩短至数分钟, 这为青霉素酰化酶的高效共价固定化提供了一条新的途径.     

化学修饰木瓜蛋白酶的固定化及性质研究

在底物保护和无底物保护下,用丁二酸酐对木瓜蛋白酶进行化学修饰,以三硝基苯磺酸法测定修饰酶的平均氨基修饰度,以棉布为载体,戊二醛为交联剂,对修饰前后的木瓜蛋白酶分别进行固定化.考察了温度、pH和表面活性剂SDS对化学修饰的固定化木瓜蛋白酶活力的影响,并与固定化天然木瓜蛋白酶进行了比较.研究表明,化学修饰固定化木瓜蛋白酶的最适反应温度为80℃;最适pH为9.0;在SDS浓度为20mg/mL时酶活也仍能保持在40%左右;米氏常数为187g/L.与天然的固定化酶相比,化学修饰的固定化木瓜蛋白酶的热稳定性、耐碱性和耐洗涤性得到了显著提高.     

纳米结构TiO2/SiO2的逐层自组装

采用逐层自组装方法在二氧化硅球表面交替组装了十二烷基硫酸钠单分子膜和二氧化钛纳米粒子膜 ,该复合多层膜经高温煅烧后得到了核壳型纳米结构二氧化钛 /二氧化硅复合颗粒 .利用XRD ,SEM ,X射线能谱等对复合颗粒进行了表征 .结果表明 :二氧化钛在复合颗粒表面排列紧密、均匀 ,粒径在 5 0nm左右 ,为锐钛矿型结构 .复合颗粒中二氧化钛的含量随组装层数的增加而均匀增加     

帽状银纳米粒子的制备及表面增强拉曼活性研究

采用真空热蒸发法在自组装的单层阵列二氧化硅纳米粒子表面沉积银膜制备了帽状银纳米粒子。通过透射电镜(TEM)、扫描电镜(SEM)和紫外-可见-近红外分光光度计 (UV-Vis-NIR)对其表面形貌及光学性质进行了表征。以吡啶-(2-偶氮-4)间苯二酚作为探针分子，研究了该复合纳米粒子的表面增强拉曼散射 (SERS) 活性，增强因子高达2.88×10⁶。结果表明在二氧化硅纳米粒子表面制备的帽状银纳米粒子是很好的表面增强拉曼散射活性基底。     

葡聚糖分子量和接枝度对阿霉素/白蛋白-葡聚糖纳米粒子体外抗肿瘤效果的影响

以Maillard反应制备的牛血清白蛋白-葡聚糖共价接枝物作为载体, 通过调节混合溶液的pH值和温度制备负载阿霉素的白蛋白-葡聚糖纳米粒子. 利用分子量为5×10³, 10×10³和62×10³的葡聚糖制备了多种共价接枝物, 研究了共价接枝物分子量对载药纳米粒子的粒径和稳定性及载药量的影响. 用短链葡聚糖(分子量5×10³和10×10³)制备的纳米粒子粒径为60 nm左右, 用长链葡聚糖(分子量62×10³)制备的纳米粒子粒径约为200 nm; 阿霉素的包埋效率为81%~98%, 包埋量为7.4%~16.9%. 细胞实验结果表明, 共价接枝物具有很好的生物相容性; 与自由阿霉素相比, 纳米粒子可以促进阿霉素进入人口腔上皮癌细胞; 受缓释性质的影响, 纳米粒子在低浓度时的细胞毒性要小于自由阿霉素. 与长链葡聚糖纳米粒子相比, 接枝度高的短链葡聚糖纳米粒子由于具有较小的粒径、 密集的葡聚糖分子刷表面、 一定的自由阿霉素浓度和较快的阿霉素释放速率, 因而更容易进入细胞并具有更好的体外抗肿瘤活性.     

铁表面银纳米粒子自组装膜及其缓蚀性能研究

应用化学还原法于水溶液中制备银纳米粒子.在十二烷基硫醇的保护下,将银纳米粒子从水相转移到甲苯相,并将处理好的铁电极浸泡在含有十二烷基硫醇保护的银纳米粒子/甲苯溶液中,制得十二烷基硫醇/银纳米粒子自组装混合膜.电化学方法如交流阻抗谱(EIS)、极化曲线等研究该自组装膜在0.5 mol.L-1H2SO4溶液中的缓蚀作用.XPS测试证实该自组装膜十二烷基硫醇和银纳米粒子之存在.     

银纳米粒子有序自组装体中偶联分子的表面增强拉曼光谱研究

采用自组装方法,分别以1,4-二巯基苯和对巯基苯胺为偶联分子,在光滑银基底表面上构筑了银纳米粒子的单层和双层有序结构.表面增强拉曼光谱研究表明,在有序银纳米粒子组装体中偶联分子的拉曼散射得到很大增强,其中1,4-对巯基苯的拉曼散射增强效应主要来自光滑银基底表面与单层银纳米粒子间的电磁耦合,而对巯基苯胺的拉曼散射增强效应则主要由两层银纳米粒子之间耦合作用所致.两种不同的耦合作用所产生的增强效应大致相近.     

Preparation of Silica Microspheres Containing Ag Nanoparticles

Two sol-gel fabrication processes were investigated to make silica spheres containing Ag nanoparticles: (1) a modified Stöber method for silica spheres below 1 m size, and (2) a SiO₂-film formation method on spheres of 3–;7 m size. The spheres were designed to incorporate silver nanoparticles of high ⁽³⁾ in a spherical optical cavity structure for the resonance effect. For the incorporation, interaction between [Ag(NH₃)₂]⁺ ion and Si-OH was important. In the Stöber method, the size of the silica spheres was determined by a charge balance of plus and minus ions on the silica surface. In the film formation method, the capture of Ag complex ion on the silica surface depended on whether the surface was covered with OH groups or not. After doping [Ag(NH₃)₂]⁺ into silica particles or SiO₂ films on the spheres, these ions w ere reduced by NaBH₄ to form silver nanoparticles. From plasma absorption at around 420 nm wavelength and TEM photographs of nanometer-sized silver particles, their formation inside the spherical cavity structures was confirmed.     

Circular dichroism analysis of penicillin G acylase covalently immobilized on silica nanoparticles

Circular dichroism (CD) was used to characterize the secondary structure of penicillin G acylase upon covalent immobilization on silica nanoparticles. Covalent immobilization was achieved by functionalizing the silica nanoparticles with glutardialdehyde and coupling to the free NH(2) groups of the enzyme (lysine and arginine side chains). The loading of the covalently bound enzyme was increased up to saturation, which was reached at 54.6 mg immobilized enzyme per g silica nanobeads. For structural characterization of the commercially available enzyme its exact molecular mass was determined by mass spectrometry in order to enable precise evaluation of the CD data. The fraction of secondary structure elements of the free and immobilized enzyme were estimated from the respective CD spectra using standard algorithms (CONTINLL, CDSSTR, SELCON3). The fractions obtained by the different algorithms for the free enzyme agreed well with one another and also with data from X-ray diffraction described in the literature. Interestingly, the secondary structure fractions found for the immobilized enzyme were very similar to the free enzyme and nearly constant over all experiments. These results indicate that even a loading of up to 55.8 mg/g (enzyme per silica nanoparticles) causes only slight structural changes. However, the specific activity determined by a kinetic assay decreased by around 60%, when increasing the loading from 14.9 to 55.8 mg/g. Because of the fact that we found no major changes in the secondary structure, diffusion limitation seems to be the main reason for the decline of the specific activity.     

磁性纳米粒子负载木瓜蛋白酶的制备、表征及用于果汁澄清(英文)

The preparation,characterization,and application of silica-coated magnetic nanoparticles for papain immobilization is reported.Papain was covalently attached onto the(3-chloropropyl) trimethoxysilane-modified silica-coated magnetic nanoparticles. The enzyme-immobilized nanoparticles were characterized by Fourier transform infrared spectroscopy,X-ray powder diffraction,scanning electron microscopy,and vibrating sample magnetometry techniques.Response surface methodology combined with statistical analyses using Minitab were employed to evaluate optimum operating conditions to immobilize papain on the magnetic nanoparticles.The optimum conditions were: temperature = 27.3℃,pH of the enzyme solution = 7.1,concentration of papain = 3.3 mg/mL,and immobilization time = 10 h.Compared with the free papain,the immobilized papain displayed enhanced enzyme activity,better tolerance to variations in the medium pH and temperature,improved storage stability,and good reusability.Both the free and immobilized enzymes were effective for the clarification of pomegranate juice.     

Synthesis with Glutaraldehyde and Characterization of Uniformly Coated Alkaline Phosphatase-Nanoparticle Bioconjugates

Alkaline phosphatase from raw milk was immobilized on cysteine-functionalized silver nanoparticles with high efficiency. The nanoparticles were characterized by ultraviolet–visible spectroscopy, X-ray diffraction, and transmission electron microscopy. The surface functionalization was confirmed by infrared spectroscopy. The spherical nanoparticles were from 40 to 60?nm in size and used for the covalent immobilization of alkaline phosphatase on the surface with glutaraldehyde treatment. As compared to soluble enzyme, an enhanced enzymatic activity of 79.87% was obtained with a percentage immobilization of 75.41%. The immobilization process did not significantly affect the structure and size of the nanoparticles, while providing a uniform coating of the enzyme on the nanoparticle as characterized by electron microscopy. The bioconjugates were reusable for up to eight times with 85% retention of the initial enzymatic activity. The synthesis of these enzyme–nanoparticle bioconjugates with high activity and stability suggests their use in biological applications.     

Textile with silver silica spheres: its antimicrobial activity against <Emphasis Type="Italic">Escherichia coli and Staphylococcus aureus</Emphasis>

The aim of this study was to investigate antimicrobial activity of textiles doped with silver in different forms. Three types of textiles were prepared and examined: textiles doped with commercially available Ag nanoparticles, textiles doped with commercial colloidal silver and textiles doped with silver silica SiO₂/Ag spheres. The specimens of silica submicron spheres were synthesized by the sol–gel method as a matrix for biological active silver. The results of microbiological tests revealed that among three kinds of Ag doped textiles only these doped with SiO₂/Ag spheres are bacteriostatically active. During the experiments minimal inhibiting bacteria growth concentration of active SiO₂/Ag spheres added to textiles was determined.     

Catalytic properties of silver nanoparticles supported on silica spheres

In this work, we investigate the catalytic properties of silver nanoparticles supported on silica spheres. The technique to support silver particles on silica spheres effectively avoids flocculation of nanosized colloidal metal particles during a catalytic process in the solution, which allows one to carry out the successful catalytic reduction of dyes. The effects of electrolytes and surfactants on the catalytic properties of silver particles on silica have been investigated. It is found that the presence of surfactants depresses the catalytic activity of the silver particles to some extent by inhibiting the adsorption of reactants onto the surface of the particles. Electrolytes either increase the migration rate of reactants in the solution resulting in an increase in the catalytic reaction rate or inhibit the adsorption of reactants onto the surface of the silver particles leading to a loss in the activity of the metal particles.     

Silica–silver core–shell particles for antibacterial textile application

The silica–silver core–shell particles were synthesized by simple one pot chemical method and were employed on the cotton fabric as an antibacterial agent. Extremely small (1–2 nm) silver nanoparticles were attached on silica core particles of average 270 nm size. The optimum density of the nano silver particles was found which was sufficient to show good antibacterial activity as well as the suppression in their surface plasmon resonance responsible for the colour of the core–shell particle for antibacterial textile application. The change in the density and size of the particles in the shell were monitored and confirmed by direct evidence of their transmission electron micrographs and by studying surface plasmon resonance characteristics. The colony counting method of antibacterial activity testing showed excellent results and even the least silver containing core–shell particles showed 100% activity against bacterial concentration of 10⁴ colony counting units (cfu). The bonding between core–shell particles and cotton fabric was examined by X-ray photoelectron spectroscopy. The antibacterial activity test confirmed the firm attachment of core–shell particles to the cotton fabric as a result 10 times washed sample was as good antibacterial as that of unwashed sample. The bacterial growth was inhibited on and beneath the coated fabric, at the same time no zone of inhibition which occurs due to the migration of silver ions into the medium was observed indicating immobilization of silver nanoparticles on silica and core–shell particles on fabric by strong bonding.     

Efficient Immobilization of Porcine Pancreatic α-Amylase on Amino-Functionalized Magnetite Nanoparticles: Characterization and Stability Evaluation of the Immobilized Enzyme

The potential of the modified magnetic nanoparticles for covalent immobilization of porcine pancreatic α-amylase has been investigated. The synthesis and immobilization processes were simple and fast. The co-precipitation method was used for synthesis of magnetic iron oxide (Fe₃O₄) nanoparticles (NPs) which were subsequently coated with silica through sol–gel reaction. The amino-functionalized NPs were prepared by treating silica-coated NPs with 3-aminopropyltriethoxysilane followed by covalent immobilization of α-amylase by glutaraldehyde. The optimum enzyme concentration and incubation time for immobilization reaction were 150 mg and 4 h, respectively. Upon this immobilization, the α-amylase retained more than 50 % of its initial specific activity. The optimum pH for maximal catalytic activity of the immobilized enzyme was 6.5 at 45 °C. The kinetic studies on the immobilized enzyme and its free counterpart revealed an acceptable change of K_m and V_max. The Km values were found as 4 and 2.5 mM for free and immobilized enzymes, respectively. The V_max values for the free and immobilized enzymes were calculated as 1.75 and 1.03 μmol mg^?1 min^?1, in order, when starch was used as the substrate. A quick separation of immobilized amylase from reaction mixture was achieved when a magnetically active support was applied. In comparison to the free enzyme, the immobilized enzyme was thermally stable and was reusable for 9 cycles while retaining 68 % of its initial activity.     

l‐Cysteine‐modified silver‐functionalized silica‐based material as an efficient solid‐phase extraction adsorbent for the determination of bisphenol A

A new silver‐functionalized silica‐based material with a core–shell structure based on silver nanoparticle‐coated silica spheres was synthesized, and silver nanoparticles were modified using strongly bound l‐ cysteine. l‐ Cysteine‐silver@silica was characterized by scanning electron microscopy and FTIR spectroscopy. Then, a solid‐phase extraction method based on l‐ cysteine‐silver@silica was developed and successfully used for bisphenol A determination prior to HPLC analysis. The results showed that the l‐ cysteine‐silver@silica as an adsorbent exhibited good enrichment capability for bisphenol A, and the maximum adsorption saturation was 20.93 mg/g. Moreover, a short adsorption equilibrium time was obtained due to the presence of silver nanoparticles on the surface of the silica. The extraction efficiencies were then optimized by varying the eluents and pH. Under the optimized conditions, good linearity for bisphenol A was obtained in the range from 0.4 to 4.0 μM (R² > 0.99) with a low limit of detection (1.15 ng/mL). The spiked recoveries from tap water and milk samples were satisfactory (85–102%) with relative standard deviations below 5.2% (n = 3), which indicated that the method was suitable for the analysis of bisphenol A in complex samples.     

Photochemical deposition of SERS active silver nanoparticles on silica gel and their application as catalysts for the reduction of aromatic nitro compounds

We report an impregnation technique for immobilization of silver(I) gelatin complex on silica gel. Subsequent UV exposure of the dry impregnated silica gel deposited silver nanoparticles on the solid matrix. Conventional techniques (UV-visible spectroscopy, TEM, EDAX, and thermal analysis) have been used to identify and characterize silver particles on silica surfaces. The photoproduced silver particles have shown unique SERS activity that authenticates the presence of silver nanoclusters in the silica matrix. Hence, the surface of the silica matrix remains SERS-active for months. This surface activity of the silica matrix inspired us to successfully study the catalytic reduction of nitro-compounds in aqueous, organic, and three different micellar media. Different thermodynamic parameters for the reduction processes have also been evaluated. Catalytic activity of the particles in micelles is explained in the light of hydrophobic and electrostatic interactions between the substrate and the micelles.