基于金纳米微粒的化学发光金属免疫分析

建立了基于金纳米微粒溶解的化学发光反应体系,并探讨了金纳米微粒溶解及化学发光测定的最佳条件。首次将金纳米微粒引入生物素和IgG的化学发光金属免疫分析,比较了不同粒径金纳米微粒、不同检测系统对IgG测定的影响。在(一抗-IgG-二抗修饰金纳米微粒)检测系统中,基于10 nm和30 nm金纳米微粒测定IgG的线性范围分别为1~75 ng和0.5~25 ng,检出限分别为0.5 ng和0.1 ng。在(一抗-IgG-生物素化抗体-链霉亲和素修饰金纳米微粒)检测系统中,5 nm和10 nm金纳米微粒测定IgG的线性范围分别为10~250 ng和1~250 ng;检出限分别为5 ng和1 ng。     

纳米金免疫凝集比率光度法检测IgG

利用柠檬酸钠还原法制备了13nm胶体金,透射电子显微镜表征其具有良好的单分散性,通过它与牛血清蛋白(BSA)作用的紫外-可见光谱表明其对蛋白具有良好的生物亲和性。以羊抗人免疫球蛋白G(IgG)修饰的金纳米粒子作探针,基于金纳米粒子免疫聚集导致其消光系数和分散度的变化建立了人IgG的比率光度分析方法。结果表明所制备的纳米金标记探针在人IgG浓度100ng/mL～100μg/mL范围内有良好的线性响应,加标法测定结果表明该法具有良好的回收率和精密度。以细胞色素C(CytoC)和辣根过氧化物酶(HRP)两种蛋白质作对照实验,发现所制备的金纳米探针对IgG具有高度的特异性。     

抗体和寡核苷酸双标记纳米金生物探针的制备及生物学特性

纳米金通过静电吸附抗体, 与寡核苷酸共价结合制备双标记纳米金生物探针, 比较了双标记纳米金生物探针和单标记抗体IgG或ss-DNA的稳定性和反应性. 结果表明, 在水溶液中纳米金由于ss-DNA的结合使IgG抗体的吸附能力明显改善, IgG的吸附也影响二硫苏糖醇(DDT)对ss-DNA的解离作用. 双标记纳米粒上覆盖(50±15)条ss-DNA和(10±2)条IgG, 较单标记ss-DNA纳米金上的(70±15)条要少. 斑点免疫和杂交实验证明, 纳米金表面标记的IgG和ss-DNA具有良好生物学活性. 双标记纳米金生物探针在超微量蛋白质的检测中具有应用价值.     

基础实验:金纳米粒子的制备及其光学性质

围绕金纳米粒子前沿内容,设计了一个简易的本科生基础实验,利用柠檬酸钠还原氯金酸法制备分散性好的金纳米粒子溶液,讨论了其尺寸与颜色的关系,探究了不同电解质和非电解质对金纳米粒子团聚及其颜色的影响,初步了解金纳米粒子的光学特性和探针效应基本原理。     

基于胶体金标记的阳极溶出伏安免疫分析用于免疫球蛋白G的测定

提出了一种基于胶体金标记的阳极溶出伏安免疫分析方法。免疫反应在聚苯乙烯微孔板中以夹心分析模式进行,通过物理吸附将兔抗人免疫球蛋白G(IgG)抗体固定于微孔板上,与相应抗原IgG发生免疫反应后,再通过夹心模式捕获相应的纳米金标记的羊抗人IgG抗体,然后再与金标羊抗人IgG抗体和金标兔抗羊二抗形成的免疫复合物反应,在微孔板上进一步引入大量的纳米金,将金溶解后,在碳糊电极上用阳极溶出伏安法(ASV)对金离子进行检测,溶出峰电流的大小间接与待分析物IgG的浓度成正比。对免疫分析的一些实验条件进行了优化。阳极溶出峰电流与IgG的对数浓度在1.1~1 143 ng/mL范围内呈良好的线性关系,检出限为1 ng/mL。将该方法应用于人血清中IgG浓度的测定,取得了满意结果。     

基于铕螯合物纳米粒子标记的时间分辨荧光免疫法检测嗜水气单胞菌

以铕螯合物荧光纳米粒子标记嗜水气单胞菌菌株B15兔抗IgG,得到纳米粒子-IgG复合物,建立了新的嗜水气单胞菌双抗夹心时间分辨荧光免疫检测(TRFIA)法.采用正交试验优化了兔抗IgG的包被时间和包被浓度,以及纳米粒子-IgG的免疫反应时间和稀释度.偶合了铕螯合物的纳米粒子发光强度大,光稳定性高,因此灵敏度被改善.方法...     

罗丹明B硅纳米粒子探针及其在蛋白芯片检测中的应用

本工作将罗丹明B分子通过共价结合的方式成功地包裹在二氧化硅纳米粒子中,制备的纳米粒子荧光强度和罗丹明B分子相比提高了1000倍.对此硅纳米荧光粒子进一步进行了链亲和素修饰,成功制备了可特异性结合生物素修饰蛋白的纳米荧光检测探针.以反相蛋白质芯片检测为模式,研究了此探针对微量蛋白的检测性能.实验中将不同微量浓度的人IgG固定于醛基修饰玻璃片表面,并加入生物素标记的抗人IgG,结果显示在800fg～100pg含量的微量蛋白检测中此纳米荧光探针具有良好的线性关系,最小蛋白检测量可达100fg.与商品化亲和素偶联cy3荧光探针对比分析发现,本方法制备的荧光探针对蛋白的检测灵敏度可提高8倍,且具有成本低,生物修饰简单等优点.     

一种新的测定痕量IgG的纳米金标免疫共振散射光谱探针

在pH8.5条件下，用粒径为9nm的金纳米微粒标记羊抗人IgG获得IgG金标免疫探针。在pH5.8磷酸氢二钠-柠檬酸缓冲溶液中及聚乙二醇存在下，金标记羊抗人IgG与人IgG产生特异性结合,羊抗人IgG包裹的金纳米微粒释放出来，聚集形成较大的微粒，导致体系在580 nm处的共振散射峰增强。IgG浓度在1.3~1.5×10³ ng·mL^-1范围内与580 nm处的共振散射光强度增加值呈线性，方法的检出限为0.78ng.mL^-1。该法用于定量分析人血清IgG,，简便快速，结果令人满意。     

金自组膜免疫芯片的研制

用光刻掩膜真空沉积技术在石英晶片上沉积上一层 8列× 6行的金膜阵列 ,用金表面N 乙酰半胱氨酸分子自组装及EDC偶联技术将人IgG、兔IgG和鼠IgG固定在石英膜阵列上来制备免疫芯片。用FITC荧光标记兔抗羊IgG、夹心法可同时测定羊抗人IgG、羊抗兔IgG和羊抗鼠IgG。用样点荧光强度与空白比Rf 作定量指标。在抗体浓度 0 .5～ 1 0 0mg L内 ,Rf与抗体浓度的对数成线性关系。最低可检出 0 .5mg L的羊抗兔IgG。测定仅需样品 1 5 0 μL ,2～ 3h,适合于快速微量分析     

基于金纳米棒的DNA超灵敏检测研究

采用氯金酸和硼氢化钠为原料合成金纳米粒子,在含有CTAB的生长溶液中加入一定量的种子溶液成长形成金纳米棒。在金纳米棒表面分别组装两种不同的巯基寡核苷酸探针,并通过靶探针进行"三明治"杂交。采用透射电子显微镜、紫外-可见-近红外光谱对杂交体系进行了表征。结果表明,所制备的金纳米棒分布均匀、分散性好,对寡核苷酸的检测限可达1pmol/L,能明显区分正错配。该方法简单易行,可应用于DNA、蛋白质等生物分子的识别。     

Dendrimer-based biosensor for chemiluminescent detection of DNA hybridization

We report on a highly sensitive chemiluminescent (CL) biosensor for the sequenc-specific detection of DNA using a novel bio barcode DNA probe modified with gold nanoparticles that were covered with a dendrimer. The modified probe is composed of gold nanoparticles, a dendrimer, the CL reagent, and the DNA. The capture probe DNA was immobilized on magnetic beads covered with gold. It first hybridizes with the target DNA and then with one terminal end of the signal DNA on the barcoded DNA probe. CL was generated by adding H₂O₂ and Co(II) ions as the catalyst. The immobilization of dendrimer onto the gold nanoparticles can significantly enhance sensitivity and gives a detection limit of 6 fmol L^-1 of target DNA.

Gold nanoparticle-based immunoassay by using non-stripping chemiluminescence detection

A novel microplate-compatible chemiluminescence (CL) immunoassay has been developed for the determination of human immunoglobulin G (IgG) based on the luminol-AgNO(3)-gold nanoparticles CL system. Polystyrene microtiter plates were used for both immunoreactions and CL measurements. The primary antibody, goat-anti-human IgG, was first immobilized on polystyrene microwells. Then the antigen (human IgG) and the gold-labeled second antibody were connected to the microwells successively to form a sandwich-type immunocomplex. The gold label could trigger the reaction between luminol and AgNO(3), accompanied by light emission. Under the optimized conditions, the CL intensity of the system was linear with the logarithm of the concentration of human IgG in the range from 25 to 5000 ng mL(-1), with a detection limit of 12.8 ng mL(-1) ( approximately 80 pM) at a signal to noise ratio of three (S/N = 3). Compared with other reported CL immunoassay method based on gold labels, the proposed CL protocol avoids a strict stripping procedure or difficult to control synthesis processes, making the method more simple, time-saving and easily automated. The present CL method is promising for the determination of clinically important bioactive analytes.     

Chemiluminescence accompanied by the reaction of gold nanoparticles with potassium permanganate

It was found that potassium permanganate (KMnO(4)) could react with gold nanoparticles in a strong acid medium to generate particle size-dependent chemiluminescence (CL). For gold nanoparticles with the size of 2.6 or 6.0 nm, the reaction was fast and could produce the excited state Mn(II) with light emission around 640 nm. For gold nanoparticles larger than 6.0 nm, no light emission was observed due to a much slower reaction rate. The CL intensity was found to increase linearly with the concentration of 2.6 nm gold nanoparticles. The effects of the acid medium, concentration of KMnO(4) and presence of N(2) and O(2) were investigated. UV-Vis absorption spectra and X-ray photoelectron spectra (XPS) measured before and after the CL reaction were analyzed. A CL mechanism has been proposed suggesting that the potassium permanganate was reduced by gold nanoparticles in the strong acid medium to the excited state Mn(II), yielding light emission. The results bestow new light on the size-dependent chemical reactivities of the gold nanoparticles and on nanoparticle-induced chemiluminescence. The CL reaction was considered to be of potential use for bioanalysis applications.     

Heat-Induced Formation of Monodisperse Gold Nanoparticles in Different Conditions

We investigate the preparation of nearly monodisperse gold nanoparticles by heat treatment in different conditions. The effects of various solvents, heating temperature, and heating time length on the monodispersity of gold nanoparticles were studied systematically and a general route to generate gold nanoparticles with uniform size was determined. The first step was to prepare gold nanoparticles with less than 3 nm and the following operation was to heat the gold nanoparticles in the present of thiolated solvents where monodispersed gold nanoparticles could be obtained easily. Our approach has enriched synthesis of monodisperse gold nanoparticles, and may provide some valuable experimental data about how the heating process affects the size evolution of gold nanoparticles.     

单分散球状纳米金颗粒的合成*

综述了近年来单分散球状金纳米颗粒的合成研究进展。分析了球状单分散金纳米颗粒的应用前景,介绍了单分散球状金纳米颗粒的主要合成方法如种子生长、回流熟化、尺寸选择沉淀分级以及电泳法等,评述了各种方法的优缺点。最后提出了单分散球状金纳米颗粒合成的一些问题,并展望了单分散球状金纳米颗粒的研究和发展方向。     

Chemiluminescence from the decomposition of peroxymonocarbonate catalyzed by gold nanoparticles

In this work, an online preparation of peroxymonocarbonate was formed innovatively, which offered the reliable intermediate for further investigation. Gold colloids with nanoparticles of different sizes were found to enhance the chemiluminescence (CL) of the peroxymonocarbonate-eosin Y system, and the most intensive CL signals were obtained with 50 +/- 1 nm diameter gold nanoparticles. UV-visible adsorption spectra, fluorescence spectra, transmission electron microscopy images, electron paramagnetic resonance spin-trapping spectra, and mass spectra were obtained in order to study the CL enhancement mechanism. Peroxymonocarbonate, a reactive oxygen species, can be decomposed to singlet oxygen which transfers its energy to eosin Y. The CL can be induced by excited eosin Y. Gold nanoparticles facilitated the radical generation and singlet oxygen molecular formation on the surface of the gold nanoparticles. Thus, the CL emission enhanced greatly by adding gold nanoparticles into the system.     

Influence of particle size on the binding activity of proteins adsorbed onto gold nanoparticles

We used optical extinction spectroscopy to study the structure of proteins adsorbed onto gold nanoparticles of sizes 5-60 nm and their resulting biological binding activity. For these studies, proteins differing in size and shape, with well-characterized and specific interactions-rabbit immunoglobulin G (IgG), goat anti-rabbit IgG (anti-IgG), Staphylococcal protein A, streptavidin, and biotin-were used as model systems. Protein interaction with gold nanoparticles was probed by optical extinction measurements of localized surface plasmon resonance (LSPR) of the gold nanoparticles. Binding of the ligands in solution to protein molecules already immobilized on the surface of gold causes a small but detectable shift in the LSPR peak of the gold nanoparticles. This shift can be used to probe the binding activity of the adsorbed protein. Within the context of Mie theory calculations, the thickness of the adsorbed protein layer as well as its apparent refractive index is shown to depend on the size of the gold nanoparticle. The results suggest that proteins can adopt different orientations that depend on the size of the gold nanospheres. These different orientations, in turn, can result in different levels of biological activity. For example, we find that IgG adsorbed on spheres with diameter ≥20 nm does not bind to protein A. This study illustrates the principle that the size of nanoparticles can strongly influence the binding activity of adsorbed proteins. In addition to the importance of this in cases of direct exposure of proteins to nanoparticles, the results have implications for proteins adsorbed to materials with nanometer scale surface roughness.     

Effect of gold nanoparticle as a novel nanocatalyst on luminol-hydrazine chemiluminescence system and its analytical application

In this work the catalytic role of unsupported gold nanoparticles on the luminol–hydrazine reaction is investigated. Gold nanoparticles catalyze the reaction of hydrazine and dissolved oxygen to generate hydrogen peroxide and also catalyze the oxidation of luminol by the produced hydrogen peroxide. The result is an intense chemiluminescence (CL) due to the excited 3-aminophthalate anion. In the absence of gold nanoparticles no detectable CL was observed by the reaction of luminol and hydrazine unless an external oxidant is present in the system. The size effect of gold nanoparticles on the CL intensity was investigated. The most intensive CL signals were obtained with 15-nm gold nanoparticles. UV–vis spectra and transmission electron microscopy studies were used to investigate the CL mechanism. The luminol and hydroxide ion concentration, gold nanoparticles size and flow rate were optimized. The proposed method was successfully applied to the determination of hydrazine in boiler feed water samples. Between 0.1 and 30 μM of hydrazine could be determined with a detection limit of 30 nM.     

SERS标记纳米粒子用于免疫识别

激光拉曼光谱技术近年来已成为研究生物分子结构常用的光谱手段.尤其在研究水溶液中蛋白质的结构和构象方面发挥了重要作用.然而,常规拉曼光谱的信号强度很低,限制了其在各个领域中的应用.表面增强拉曼光谱(SERS)和表面增强共振拉曼光谱(SERRS)技术可使信号增强6～10个数量级,尤其是SERS技术已发展到检测单分子的水平,更为其在生物方面的应用开拓了新的局.