Lead Sulfide Nanoparticle as Oligonucleotides Labels for Electrochemical Stripping Detection of DNA Hybridization

We report a method for the detection of DNA hybridization in connection to lead sulfide (PbS) nanoparticle tags and electrochemical stripping measurement of the lead. A kind of lead sulfide nanoparticle with free carboxyl groups on its surface was synthesized in aqueous solution. The nanoparticle was used as a marker to label a sequence‐known oligonucleotide, which was then employed as a DNA probe for identifying a target ssDNA immobilized on a PPy modified electrode based on a specific hybridization reaction. The hybridization events were monitored by the oxidation dissolution of the lead sulfide anchored on the hybrids and the indirect determination of the lead ions by anodic stripping voltammetry (ASV). The detection limit is 0.3 pmol L^?1 of target oligonucleotides. The PbS nanoparticle combining its easy conjugation to the DNA molecule with the highly sensitive stripping voltammetry detection of lead shows its promising application in the electrochemical DNA hybridization analysis assay.     

Preparation of Nanogapped Gold Nanoparticle Array for DNA Detection

A novel DNA detection technique using a gold nanoparticle array film electrode has been reported here. The gold nanoparticles molecularly linked with binder molecule (1,10‐decanedithiol) were separated 1.3 nm from each other, and the DNA conductivity change from single to double strand was measured by monitoring a voltage drop across the particles, between which a probe of a 12‐mer oligonucleotide was immobilized. In adding a complementary oligonucleotide on the nanoparticle film chip, an immediate decrease in the film resistance (ca. 1.4 Ω) due to a hybridization event occurred in a reproducible manner with this simple setup. In the paper, we have an interest in the primary sensing properties; effect of the film resistance on the sensor response, dependence of the resistance change on the DNA concentration, and the performance of the system for DNA detection including single nucleotide polymorphisms were described.     

柔红霉素修饰的纳米金电极的制备及其对DNA检测

利用双硫醇分子作为连接剂, 将纳米金颗粒固定于金电极上, 用伏安法、紫外-可见光谱和电化学交流阻抗对其组装过程以及活性进行了表征. 制备的纳米金修饰电极用于DNA测定及其对DNA损伤的检测. DNA的检测限为 1.2×10^－9 mol/L. 该法灵敏、简便.     

Gold Nanoparticle‐Catalyzed Silver Electrodeposition on an Indium Tin Oxide Electrode and Its Application in DNA Hybridization Transduction

In this work, we report a simple, rapid and sensitive approach for the electrochemical gold nanoparticle‐based DNA detection with an electrocatalytic silver deposition process. The catalytic and preferential silver electrodeposition on gold nanoparticle surfaces using an indium tin oxide (ITO) electrode at certain potentials, without any chemical pretreatments of the electrode, is demonstrated. More importantly, the application of this methodology for hybridization transduction is explored. The ITO electrode surface is first coated with an electroconductive polymer, poly(2‐aminobenzoic acid), to enable the chemical attachment of avidin molecules for the subsequent probe immobilization. The hybridization of the target with the probe in turn permits the binding of the gold nanoparticle labels to the transducer surface via biotin‐streptavidin interaction. The amount of bound gold labels, which is proportional to the amount of the target, is determined by the electrocatalytic silver deposition process. A significant improvement of the signal‐to‐background ratio is achieved with this scheme compared to the conventional chemical hydroquinone‐based silver deposition process.     

Construction of CdS Nanoparticle Chain on DNA Template

Salmon sperm DNA was used as template to assembly and nucleate CdS nanoparticles.Transmission electron microscopy(TEM)images showed that the CdS nanoparticles fromed unique nanostructure which present regular and parallel chains along DNA molecular chaing.The width of every chain was about 3 nm.Raman and Xray photoelectron energy spectroscopy(XPS) confirmed that the nucleation sites of CdS nanoparticles were phosphate acid groups of DNA.     

DNA步行器调控的纳米粒子超晶格

作为一种精巧的DNA纳米机器, DNA步行器因其优异的可设计性及可编程性在众多研究领域中展示出强大的应用价值. 本工作通过将基于催化发夹组装的双足DNA步行器与DNA功能化的金纳米粒子(即球形核酸)组装相结合, 开发了一种具有时间依赖性的DNA步行器驱动球形核酸恒温有序组装的策略. 以单组分球形核酸组装体系为例, DNA步行器通过发夹催化组装反应驱动在球形核酸表面上随机行走并逐渐产生带有活性粘性末端的DNA杂交结构, 促使球形核酸表面粘性末端间的“键合”速率与其组装速率在时间尺度上保持同步, 从而得到面心立方(FCC)晶型的超晶格结构. 基于类似原理, 作者还构建了一种DNA步行器驱动的双组分球形核酸组装体系并以此得到氯化铯(CsCl)晶型的超晶格结构.     

Determination of DNA Hybridization on Gold Nanoparticle Conjugated Polystyrene Particle Thin Film Using Attenuated Total Reflectance Fourier Transform Infrared Spectroscopy

Attenuated total reflectance Fourier transform infrared spectroscopy was used to detect DNA hybridization on a polystyrene conjugated gold nanoparticle thin film. The gold nanoparticles were synthesized on the surface of poly(ethylenimine) coated polystyrene particles by citrate reduction. Single-stranded DNA was then immobilized on the nanoparticle surface via thiol bonding. Ultraviolet-visible spectrometry was used to monitor the conjugation of the nanoparticles on polystyrene particles and the immobilization of a single-stranded DNA probe. The morphology of the polystyrene-gold nanoparticle thin film was characterized using scanning electron microscopy and showed successful conjugation and immobilization. The infrared spectra obtained from the hybridization showed features of DNA structure and peak shifts at 1657 cm^?1 compared to the non-complementary DNA due to changes in hydrogen bonding between N-H and C?O of complimentary bases pairs. The peaks at 1067, 975, 920, and 859 cm^?1, which were shifted to lower wavenumbers in the polystyrene-gold nanoparticle probe and target DNA, indicated hydrogen bonding formation between N-H and N of complimentary base pairs. ATR-FTIR spectroscopy provided simple, fast, and portable label-free detection of target DNA sequence on the polystyrene-gold nanoparticle thin film.     

羧基二茂铁-脱氧核糖核酸探针的制备和脱氧核糖核酸分析的应用

在偶联活化剂碳二亚胺的存在下,通过羧基二茂铁(FCA)上的羧基与DNA分子上的氨基共价键合,将FCA标记在氨基修饰的寡聚核苷酸片段上,制备成FCA-ssDNA探针。探针与固定在电极上的ssDNA在一定的条件下进行杂交反应,测定杂交后FCA对Lum inol-H2O2体系的电致化学发光催化信号,从而对目标ssDNA进行序列识别及含量测定。实验结果表明,该探针能够很好的识别三碱基错配序列,对完全互补序列的响应可以达到5×10-11mol/L。     

DNA/CdS纳米粒子复合体系的光谱和光电化学性质

在水溶液中以DNA作为模板和稳定剂, 构筑了DNA与CdS纳米粒子复合体系(DNA/CdS NPC), 研究DNA的含量, 单双链等对复合体系光电响应的影响, 并综合TEM, UV-Vis, IR和荧光光谱等对其形貌和光谱性质进行表征. 结果表明, CdS纳米粒子(CdS NPs)与DNA链之间主要通过静电作用结合; DNA模板对CdS NPs的禁带宽度没有影响; 以DNA模板合成的CdS NPs具有较高的表面态密度, 其对CdS NPs的荧光有增强作用, 而对光电流响应有抑制作用, 并且DNA在复合体系中的含量影响荧光增强和光电流减弱的程度. 该复合体系在荧光标记检测和DNA的定量分析方面可能具有应用前景.     

碳点对鲁米诺电化学发光体系抑制作用的研究及其在DNA分析中的应用

发现碳点对鲁米诺电化学发光体系有明显的抑制作用, 并且由于碳点对单双链DNA的吸附性差异, 与单双链结合的碳点对鲁米诺电化学发光体系的抑制程度不同, 基于此实现了对DNA的快速、简便、灵敏的检测. 考察了碳点粒径、浓度对鲁米诺电化学发光体系的抑制行为的影响. 优化了溶液pH值, 鲁米诺浓度等电化学发光条件. 在优化的最佳实验条件下, 该方法检测DNA的线性范围为1.0×10^-10～7.5×10^-9 mol/L, 检出限为5.2×10^-11 mol/L.     

Label-Free Electrochemiluminescent Determination of DNA Using Luminol and Hemin Functionalized Nanoparticles

Luminol and hemin dual-functionalized silica nanoparticles were synthesized using a typical reverse water-in-oil microemulsion protocol. The obtained nanoparticles were further characterized by transmission electron microscopy, scanning electron microscopy, atomic absorption spectrometry, chemiluminescence, and electrochemiluminescence. The results indicated that the luminol and hemin dual-functionalized silica nanoparticles exhibited significantly higher chemiluminescence and electrochemiluminescence intensities than those of luminol functionalized silica nanoparticles due to the catalytic effect of hemin on the chemiluminescence and electrochemiluminescence of luminol. Furthermore, a simple and sensitive label-free electrochemiluminescence DNA biosensor was developed based on the chitosan modified luminol and hemin dual-functionalized silica nanoparticles and a single-stranded DNA probe. The chitosan modified luminol and hemin dual-functionalized silica nanoparticles were immobilized on the surface of an indium-doped tin oxide electrode and the single-stranded DNA probe was immobilized on the surface of the nanoparticles through electrostatic interactions between single-stranded DNA and chitosan, which allowed hybridization with the target DNA sequences. The hybridization events were evaluated by electrochemiluminescence, and only the complementary sequence formed double-stranded DNA with the DNA probe to give strong electrochemiluminescence signals. Finally, the electrochemiluminescence intensity was found to be linearly related to the concentration of the complementary sequence at concentrations from 1.0?×?10^?12 to 1.0?×?10^?6?mol·L^?1 with a detection limit of 5.0?×?10^?13?mol·L^?1.     

银纳米颗粒的制备及表征

用鞣酸还原法制得了PVP保护的Ag纳米颗粒,并通过TEM、XRD、TG、DTA及FT IR对其结构进行了表征.结果表明在所选择的实验条件下制备了粒径小、单分散且化学稳定的Ag PVP纳米颗粒,其粒径约10nm,有良好的水分散性.PVP的加入和银氨络离子的形成对制备出小尺寸纳米银起了重要作用.     

DNA Hybridization at Magnetic Nanoparticles with Electrochemical Stripping Detection

A simple and practical method for electrochemical DNA hybridization assay has been developed to take advantage of magnetic nanoparticles for ssDNA immobilization and zinc sulfide nanoparticle as oligonucleotide label. Magnetic nanoparticles were prepared by coprecipitation of Fe²⁺ and Fe³⁺ with NH₄OH, and then amino silane was coated onto the surface of magnetite nanoparticles. The magnetic nanoparticles have the advantages of easy preparation, easy surface modification and low cost. The target ssDNA with the phosphate group at the 5′ end was then covalently immobilized to the amino group of magnetite nanoparticles by forming a phosphoramidate bond in the presence of 1‐ethyl‐3‐(3‐dimeth‐ylaminopropyl)carbodiimide (EDAC). The zinc sulfide (ZnS) nanoparticle‐labeled oligonucleotides probe was used to identify the target ssDNA immobilized on the magnetic nanoparticles based on a specific hybridization reaction. The hybridization events were assessed by the dissolution of the zinc sulfide nanoparticles anchored on the hybrids and the indirect determination of the dissolved zinc ions by anodic stripping voltammetry (ASV) at a mercury film glassy carbon electrode (GCE). The proposed method couples the high sensitivity of anodic stripping analysis for zinc ions with effective magnetic separation for eliminating nonspecific adsorption effects and offers great promise for DNA hybridization analysis.     

单分子层保护纳米 Au 粒子表面配位催化剂的制备及其应用

 贵金属纳米粒子由于其小尺寸效应而表现出特殊的催化性能. 综述了纳米 Au 粒子表面配位催化剂的制备方法及其在催化中的应用. 由于 Au 可与硫化物形成配位键, 所以硫化物可在 Au 表面形成有序单分子膜. 单分子膜保护的 Au 纳米粒子具有非常好的溶解性、分散性、稳定性, 以及由不同的表面功能团而导致的不同的催化性能. 该催化体系兼具均相催化剂和多相催化剂的特点, 这对开发新型催化剂具有重要的理论和实际意义.     

MCM-41型介孔二氧化硅纳米颗粒的制备及其在DNA生物传感器中的应用

MCM-41型介孔二氧化硅纳米颗粒具有独特的结构特征和理化性质,能够与DNA、信号探针以及多种活性纳米颗粒结合,在DNA生物传感器中得到了广泛应用.其中,球形和薄膜形的MCM-41型介孔二氧化硅具有高负载量、孔口控释和高比表面积等优点,能有效装载各种信号探针、控制粒子的扩散以及固定大量活性纳米颗粒,可大大提高DNA生物...     

油溶性金属Ni纳米微粒的制备与表征

纳米材料的制备、性能与应用已成为近年来的研究热点之一犤１犦。由于在催化、光学和电学材料中的广泛应用，超细单分散的金属微粒的制备与性质已引起人们的广泛兴趣。通常制备金属纳米微粒的方法有两种：一是把固体金属材料分裂为纳米尺寸的颗粒，如机械粉碎、电弧放电及金属原子蒸气沉积犤２犦，用这种方法制备的金属微粒粒径一般都比较大，且粒子尺寸分布宽，另一种是把金属原子制成纳米尺度的颗粒，如乳液聚合法犤３犦、热解犤４犦、γ－射线辐照犤５犦、脉冲电沉积犤６犦和化学还原犤７犦等，这种方法制备的微粒粒径通常分布窄且粒子小…     

基于纳米金探针和基因芯片的DNA检测新方法

运用荧光纳米金探针和基因芯片杂交建立一种新的DNA检测方法. 荧光纳米金探针表面标记有两种DNA探针: 一种为带有Cy5荧光分子的信号探针BP1, 起信号放大作用; 另一种为与靶DNA一部分互补的检测探针P532, 两种探针比例为5∶1. 当靶DNA存在时, 芯片上捕捉探针(与靶DNA的另一部分互补)通过碱基互补配对结合靶DNA, 将靶DNA固定于芯片上; 荧光纳米金探针通过检测探针与靶DNA及芯片结合, 在芯片上形成“三明治”复合结构, 最后通过检测信号探针上荧光分子的信号强度来确定靶DNA的量. 新方法检测灵敏度高, 可以检测浓度为1 pmol/L的靶DNA, 操作简单, 检测时间短. 通过改进纳米金探针的标记和优化杂交条件, 可进一步提高核酸检测的灵敏度, 这将在核酸检测方面具有重要的应用价值.     

Raman Enhancement of Nanoparticle Dimers Self-Assembled Using DNA Origami Nanotriangles

Surface-enhanced Raman scattering is a powerful approach to detect molecules at very low concentrations, even up to the single-molecule level. One important aspect of the materials used in such a technique is how much the signal is intensified, quantified by the enhancement factor (EF). Herein we obtained the EFs for gold nanoparticle dimers of 60 and 80 nm diameter, respectively, self-assembled using DNA origami nanotriangles. Cy5 and TAMRA were used as surface-enhanced Raman scattering (SERS) probes, which enable the observation of individual nanoparticles and dimers. EF distributions are determined at four distinct wavelengths based on the measurements of around 1000 individual dimer structures. The obtained results show that the EFs for the dimeric assemblies follow a log-normal distribution and are in the range of 10⁶ at 633 nm and that the contribution of the molecular resonance effect to the EF is around 2, also showing that the plasmonic resonance is the main source of the observed signal. To support our studies, FDTD simulations of the nanoparticle’s electromagnetic field enhancement has been carried out, as well as calculations of the resonance Raman spectra of the dyes using DFT. We observe a very close agreement between the experimental EF distribution and the simulated values.     

单分散氧气锌纳米粒子的制备及表征

用羟丙基甲基纤维素(HPMC)为空间分散剂,制备了前驱物[Zn2(OH)2CO3*HPMC],焙烧后得到的纳米ZnO同不加HPMC制备的ZnO相比较,产物粒度小、分散均匀、不易团聚.通过XRD, TEM及FT-IR对产物的组成、粒径及形貌进行了表征.利用UV-Vis测试了产物的光吸收性能,结果表明,所得的产物在200nm～400nm具有较强的吸收.     

Pt纳米粒子修饰的多孔硅电极的制备及其电催化性能

通过循环伏安法电沉积使直径约为7 nm的Pt纳米粒子均匀地分散于多孔硅表面, 拟用作微型质子交换膜燃料电池的催化电极. 与刷涂法相比较, 电沉积Pt纳米粒子的多孔硅电极(Pt/Si)呈现出高的Pt利用率和增强的电催化活性. 当Pt载量为0.38 mg•cm−2时, 其电化学活性比表面积高达148 cm2•mg−1, 是刷涂相近质量的纳米Pt/C催化剂的多孔硅电极Pt-C/Si的2倍多；该修饰电极对甲醇氧化也呈现了增强的催化性能和好的稳定性, 在0.5 V(vs SCE)极化1 h后电流密度为4.52 mA•cm−2, 而刷涂了相近Pt量的Pt-C/Si电极的电流密度只有0.36 mA•cm−2.