基于电化学双共价键法构建可再生高灵敏的电化学发光适体传感器检测可卡因

基于点击化学和重氮盐法的双共价键固定化方法,制备了一种高灵敏、可重复使用的电化学发光(ECL)适体传感器. 该方法以可卡因为分析物,以可卡因适体为分子识别物质,以钌联吡啶衍生物为ECL信号物质. 采用电化学方法在玻碳电极表面重氮化叠氮苯胺,通过点击反应连接炔基功能化的钌联吡啶衍生物标记可卡因适体,获得适体传感器. 该传感器在共反应剂存在下,产生弱的电化学发光信号,可卡因存在下,电化学发光信号增加. 基于此,建立了“信号增强”型检测可卡因的电化学发光分析新方法. 电化学发光信号与可卡因浓度在0.1 nmol·L^-1 ~ 100 nmol·L^-1范围内呈良好的线性关系,检出限为60 pmol·L^-1. 该传感器具有良好的稳定性,可重复多次使用. 该双共价键法在构建ECL传感器方面具有很好的应用前景.     

基于共轭聚合物的核酸生物传感器的应用

共轭聚合物的π电子体系及共轭离域结构,使其具有良好的发光性能。聚合物链可充当“分子导线”,能够成倍放大光学信号,从而有效提高检测灵敏度。而核酸适体(aptamer)在特异性、与靶物质亲合力、信号传导方面比其他识别元件具有更大的优势,因此共轭聚合物的核酸生物传感器在生物检测方面得到了迅速发展。本文主要总结了近年来共轭聚合物的核酸生物传感器在生物检测方面的应用,并进一步对该类型传感器的发展趋势作出了展望。     

基于核酸适体的电化学生物传感研究

核酸适体是一类经由指数富集的配体系统进化（SELEX）技术在体外筛选获得的单链寡核苷酸片段,由于具有可人工批量合成、价格低廉、易于功能化修饰、特异性强、亲和力高、免疫原性低、批间差异小、热稳定性好等优良特性,在分析化学、疾病治疗以及生物医学研究等诸多领域备受关注。结合代表性案例,该文综述了核酸适体在电化学生物传感领域的应用。首先简要概述了核酸适体及电化学适体传感器的特点,分类阐述了电化学适体传感器在小分子化合物、蛋白质、外泌体、循环肿瘤细胞（CTCs）以及病原微生物检测中的应用,并重点介绍了相关检测方法的原理、分析特性以及所应用的信号放大策略,最后对电化学适体传感器的发展进行了展望。     

非标记型p53抑癌基因电化学DNA生物传感器的研究

基于发夹型核酸探针的高特异性识别能力以及电活性物质与DNA磷酸骨架间的静电作用,以发夹型核酸作为分子识别探针,电活性物质六氨合钌(RuHex)作为杂交指示剂,构建了一种非标记型检测p53抑癌基因的电化学DNA生物传感器.实验结果表明,在10 μmol/L RuHex溶液中,该传感器对目标DNA具有灵敏的电化学响应,电化...     

基于裂开型核酸适配体的液晶生物传感检测三磷酸腺苷

利用“适配体-目标分子-适配体”的“三明治”夹心方式构建液晶生物传感检测三磷酸腺苷(ATP). 将ATP核酸适配体片段作为捕获探针固定在经TEA/DMOAP混合组装膜修饰的玻片基底表面, 当ATP存在时, 裂开的两部分核酸适配体与ATP结合形成双链结构, 有效诱导液晶分子取向发生变化从而引起光学信号的亮度及颜色发生变化, 实现对ATP的检测, 该方法在ATP浓度为10 nmol/L时仍可观测到明显的光学信号变化. 这种“适配体-目标分子-适配体”的“三明治”夹心式液晶生物传感方法具有无需标记, 操作简单等特点, 在快速检测小分子等物质领域中有广泛的应用前景.     

核酸适体在生物医学中的应用*

核酸适体是经配体指数富集系统进化技术（SELEX）筛选获得的一类能够特异性地结合离子、分子,甚至整个细胞的单链DNA或者RNA分子。本文介绍了核酸适体及相关筛选技术SELEX;综述了近年来以提高筛选效率和效果为目标的核酸适体筛选技术新进展;列举了核酸适体在无机离子、小分子、生物大分子和肿瘤细胞检测、肿瘤标记物的发现等方面的应用;讨论了基于核酸适体的靶向治疗策略;最后对核酸适体在生物医学上的应用前景进行了展望。     

基于核酸适体电化学生物传感器用于腺苷的免标记检测

以纳米MnO2作为适体固定的构建平台,制备了一种基于核酸适体的新型腺苷电化学生物传感器.固定于电极表面的适体探针与目标腺苷杂交后使电极界面的结构发生改变,通过[Fe(CN)6]3-/4-氧化还原探针监测传感器表面电子传递电阻的变化,以此作为检测信号进行腺苷的免标记检测.表面电子传递电阻的变化值与腺苷浓度的对数在1.0×...     

非标记夹心式电化学可卡因适体传感器的研究

设计一种基于双链核酸适体的非标记夹心式电化学适体传感器, 建立简单、高灵敏度的可卡因分析方法. 首先将末端巯基修饰的捕获适体探针组装在金电极表面, 构建可卡因适体传感器. 该传感器与目标分子可卡因和部分互补的检测适体探针作用后, 在电极表面形成适体/可卡因/适体复合物. 以六氨合钌为信号分子, 基于单链适体和适体/可卡因/适体复合物对六氨合钌吸附量的不同, 通过计时电量法检测电极表面吸附六氨合钌的还原电量, 进行可卡因的分析检测. 在优化的条件下, 还原电量与可卡因浓度在1～50 mmol/L范围内呈良好的线性关系, 检出限为0.1 mmol/L. 用于血清中可卡因的检测, 回收率为96.4%～104%. 该方法简单, 灵敏度高, 可作为一种通用型的适体传感器模型.     

电化学发光和电化学生物传感器的研究

本研究小组近年来在电化学发光DNA和适体传感器研究和无标记以及阵列电化学DNA和适体传感器方面进行了一些工作,重点介绍如何提高生物传感器灵敏度进行传感界面设计的一些思路.利用纳米粒子提高灵敏度和再现性的途径主要有三种,一是用纳米材料修饰电极上,提高待测物或探针在电极表面的固定量;二是用纳米材料作为信号分子的载体或信号粒子, 以提高检测信号的强度~([1]);三是纳米材料直接作为信号物质~([2]).     

DNA电化学生物传感器在重金属快速检测中的研究进展

DNA电化学生物传感器是一类以DNA为敏感元件或检测对象,将核酸分子特异性识别过程中产生的信号通过换能器转化为电信号,从而实现对目标物定性或定量检测的传感器,具有响应速度快、操作简单、选择性好、灵敏度高、检测成本低等优点,实现了多领域中重金属、真菌毒素、核酸等的快速实时检测。介绍了DNA电化学生物传感器的组装单元、电化学指示剂类型,以DNA二级构型角度综述了DNA电化学生物传感器的四大类特殊结构,并汇总其在临床、中医药、生态环境保护及食品安全等领域中重金属的检测应用研究,对新型DNA电化学生物传感器的设计与其在更多领域的拓展应用提供借鉴价值。     

Aptamer-based molecular recognition for biosensor development

Nucleic acid aptamers are an emerging class of synthetic ligands and have recently attracted significant attention in numerous fields. One is in biosensor development. In principle, nucleic acid aptamers can be discovered to recognize any molecule of interest with high affinity and specificity. In addition, unlike most ligands evolved in nature, synthetic nucleic acid aptamers are usually tolerant of harsh chemical, physical, and biological conditions. These distinguished characteristics make aptamers attractive molecular recognition ligands for biosensing applications. This review first concisely introduces methods for aptamer discovery including upstream selection and downstream truncation, then discusses aptamer-based biosensor development from the viewpoint of signal production.

RE-SELEX: restriction enzyme-based evolution of structure-switching aptamer biosensors

Aptamers are widely employed as recognition elements in small molecule biosensors due to their ability to recognize small molecule targets with high affinity and selectivity. Structure-switching aptamers are particularly promising for biosensing applications because target-induced conformational change can be directly linked to a functional output. However, traditional evolution methods do not select for the significant conformational change needed to create structure-switching biosensors. Modified selection methods have been described to select for structure-switching architectures, but these remain limited by the need for immobilization. Herein we describe the first homogenous, structure-switching aptamer selection that directly reports on biosensor capacity for the target. We exploit the activity of restriction enzymes to isolate aptamer candidates that undergo target-induced displacement of a short complementary strand. As an initial demonstration of the utility of this approach, we performed selection against kanamycin A. Four enriched candidate sequences were successfully characterized as structure-switching biosensors for detection of kanamycin A. Optimization of biosensor conditions afforded facile detection of kanamycin A (90 μM to 10 mM) with high selectivity over three other aminoglycosides. This research demonstrates a general method to directly select for structure-switching biosensors and can be applied to a broad range of small-molecule targets.

RE-SELEX is the first homogenous method for in vitro evolution of structure-switching DNA aptamers.     

An aptasensor for sensitive detection of human breast cancer cells by using porous GO/Au composites and porous PtFe alloy as effective sensing platform and signal amplification labels

A novel aptamer biosensor for cancer cell assay has been reported on the basis of ultrasensitive electrochemical detection. The assay uses the aptamer as a capture probe to recognize and bind the tumor marker on the surface of the cancer cells, forming an aptamer-based sandwich structure for MCF-7 cells detection. Functionalized nanoporous materials, porous graphene oxide/Au composites (GO/Au composites) and porous PtFe alloy have been introduced into the biosensor. Owing to the large surface area and versatile porous structure, the use of nanoporous materials can significantly improve the analysis performance of the biosensors by loading of large amounts of molecules and accelerating diffusion rate. Under the optimized experimental conditions, the proposed aptamer biosensor exhibited excellent analytical performance for MCF-7 cells determination, ranging from 100 to 5.0 × 10⁷ cells mL⁻¹ with the detection limit of 38 cells mL⁻¹. The biosensor showed good selectivity, acceptable stability and reproducibility, and developed a highly sensitive and selective method for cancer cells detection.     

Aptamer-based label-free method for hemin recognition and DNA assay by capillary electrophoresis with chemiluminescence detection

An aptamer-based label-free approach to hemin recognition and DNA assay using capillary electrophoresis with chemiluminescence detection is introduced here. Two guanine-rich DNA aptamers were used as the recognition element and target DNA, respectively. In the presence of potassium ions, the two aptamers folded into the G-quartet structures, binding hemin with high specificity and affinity. Based on the G-quartet–hemin interactions, the ligand molecule was specifically recognized with a K _d ≈ 73 nM, and the target DNA could be detected at 0.1 μM. In phosphate buffer of pH 11.0, hemin catalyzed the H₂O₂-mediated oxidation of luminol to generate strong chemiluminescence signal; thus the target molecule itself served as an indicator for the molecule–aptamer interaction, which made the labeling and/or modification of aptamers or target molecules unnecessary. This label-free method for molecular recognition and DNA detection is therefore simple, easy, and effective. Figure A label-free approach to aptamer-based hemin recognition and DNA detection is introduced, which gives great potential for using a small molecule itself as the indicator for molecular recognition and DNA detection thereby avoiding any labeling or modification step     

Label-free aptamer-based electrochemical impedance biosensor for 17β-estradiol

A novel aptamer-based label-free electrochemical impedance spectroscopy biosensor for 17β-estradiol has been fabricated. The aptamers were firstly immobilized on the gold electrode through Au-S interaction; the aptamer probe was then bound with the addition of 17β-estradiol to form the estradiol/aptamer complex on the electrode surface. This leads to a significantly larger interfacial electron transfer resistance than that without the addition of 17β-estradiol. The change in the resistance had a linear relationship with 17β-estradiol concentration in the range of 1.0 × 10(-8) to 1.0 × 10(-11) mol L(-1), with a detection limit of 2.0 × 10(-12) mol L(-1). The biosensor showed high selectivity to 17β-estradiol and good stability. The designed biosensor has been applied to detect 17β-estradiol in human urine with satisfactory results.     

Stabilizing structure-switching signaling RNA aptamers by entrapment in sol-gel derived materials for solid-phase assays

Structure-switching, fluorescence-signaling DNA and RNA aptamers have been reported as highly versatile molecular recognition elements for biosensor development. While structure-switching DNA aptamers have been utilized for solid-phase sensing, equivalent RNA aptamers have yet to be successfully utilized in solid-phase sensors due to their lack of chemical stability and susceptibility to nuclease attack. In this study, we examined entrapment into sol-gel derived organic-inorganic composite materials as a platform for immobilization of structure-switching fluorescence-signaling RNA aptamer reporters, using both the synthetic theophylline- and naturally occurring thiamine pyrophosphate-binding RNA aptamers as test cases. Structure-switching versions of both aptamers were entrapped into a series of sol-gel derived composites, ranging from highly polar silica to hydrophobic methylsilsesquioxane-based materials, and the target-binding and signaling capabilities of these immobilized aptamers were assessed relative to solution. Both immobilized aptamers demonstrated sensitivity and selectivity similar to that of free aptamers when entrapped in a composite material derived from 40% (v/v) methyltrimethoxysilane/tetramethoxysilane. Importantly, this material also conferred protection from nuclease degradation and imparted long-term chemical stability to the RNA reporter systems. Given the versatility of sol-gel entrapment for development of biosensors, microarrays, bioaffinity columns, and other devices, this entrapment method should provide a useful platform for numerous solid-phase RNA aptamer-based devices.     

Target induced dissociation (TID) strategy for the development of electrochemical aptamer-based biosensor

In this paper, we report a novel and more general signal-on strategy for the fabrication of electrochemical aptamer-based (E-AB) biosensor. The principle is that the interaction between the target and the aptamer strand may induce the formation and subsequent dissociation of target–aptamer complex from an electrode surface, and consequently, the remaining DNA strand on the electrode surface can hybridize again with a ssDNA containing an electrochemical probe. Differential pulse voltammetric studies have revealed that this target induced disassociation (TID) strategy is an effective signal-on method for the detection of ATP molecules with good selectivity. The TID strategy may also have several advantages, such as independence on the specific structure of either the aptamers or their complementary sequences and promotion of the generalization of E-AB sensors, the more convincible results due to the signal-on model, and the unnecessity to label the aptamers, which provides the optimized status for the reaction with the targets, etc.     

基于铁氰化镍的非标记型核酸适配体电化学传感器检测凝血酶

在玻碳电极（GCE）表面首先用增敏作用的多壁碳纳米管(MWCNTs)夹心于两层电沉积的铁氰化镍（NiHCF）氧化还原电化学探针之间,然后以金纳米粒子为固定核酸适配体的载体,构建了检测凝血酶的非标记型核酸适配体生物传感器。 利用扫描电子显微镜(SEM)对MWCNTs和NiHCF的形貌进行了表征。 利用电化学阻抗谱对传感器的组装过程进行了监测,用循环伏安法（CV）和差分脉冲伏安法（DPV）对传感器的电化学行为进行了研究。 以铁氰化镍为探针的传感器对凝血酶的检测在1.0 ng/L~1.0 mg/L范围内呈良好的线性关系,相关系数为0.998,检测限为0.2 ng/L(S/N=3)。     

核酸适配体生物传感器在三聚氰胺检测中的应用进展

三聚氰胺常被非法添加到食品中,以提高食品中蛋白质的含量。但是,三聚氰胺一旦进入体内,会对人们的健康造成伤害。因此,对三聚氰胺的检测十分必要。为了弥补传统仪器检测法和免疫检测法的不足,基于核酸适配体开发了一系列新的生物传感器,用于三聚氰胺的检测。按照与三聚氰胺的不同识别机制,把这些新的生物传感器分成了四类,分别为基于多聚胸腺嘧啶DNA链和三聚氰胺识别的生物传感器、基于无嘌呤位点的三链DNA结构和三聚氰胺识别的生物传感器、基于核酸适配体和三聚氰胺识别的生物传感器、基于三聚氰胺和汞离子/铜离子等配位识别的生物传感器。本文按照上述四类方法逐个展开,对核酸适配体生物传感器在三聚氰胺检测中的应用进行了综述,并对它们的优缺点进行阐述。     

Study on an electrochemical biosensor for thrombin recognition based on aptamers and nano particles

This paper presents a high specific, sensitive electrochemical biosensor for recognition of protein such as thrombin based on aptamers and nano particles. Two different aptamers were chosen to construct a sandwich manner for detecting thrombin. Aptamer I was immobilized on nano magnetic particle for capturing thrombin, and aptamer II labled with nano gold was used for detection. The electrical current generated from gold after the formation of the complex of magnetic particle, thrombin and nano gold, and then an electrochemical cell designed by ourselves was used for separating, gathering, and electrochemical detecting. Through magnetic separation, high specific and sensitive detection of the target protein, thrombin, was achieved. Linear response was observed over the range 5.6×10-12―1.12×10-9 mol/L, with a detection limit of 1.42×10-12 mol/L. The presence of other protein as BSA did not affect the detection, which indicates that high selective recognition of thrombin can be achieved in complex biological samples such as human plasma.