纳米颗粒增强的葡萄糖生物传感器

研制的纳米增强葡萄糖传感器是用纳米憎水Ａｕ颗粒。亲水Ａｕ颗粒、憎水ＳｉＯ_２颗粒以及Ａｕ和－ＳｉＯ_2颗粒混合与聚乙烯醇缩丁醛（ＰＶＢ）构成复合固酶膜基质,用溶胶－凝胶法固定葡萄糖氧化酶（ＧＯＤ）,组成葡萄糖生物传感器．实验表明,纳米颗粒可以大幅度提高固定化酶的催化活性,响应电流从相应浓度的几十纳安增强到几千纳安,电极响应迅速, １ｍｉｎ达到稳态,探讨了纳米颗粒效应在固定化酶中所起的作用,开辟了制备直接电子传递第三代生物传感器的新途径和纳米颗粒应用的新领域。     

纳米铜颗粒-酶-复合功能敏感膜生物传感器

用水合联肼作还原剂研制成亲水纳米铜颗粒,用琥珀酸二异酯磺酸钠／丙三醇／正庚烷反胶束体系合成出憎水纳米铜颗粒,并通过透射电镜和紫外光谱考察了制得的纳米颗粒样品,用憎水纳米铜颗粒及亲水纳米铜颗粒与聚 烯醇缩丁醛构成复合固酶膜基质,用溶胶－凝胶法固定葡萄糖氧化酶,构建葡萄糖生物传感器,实验结果表明,纳米铜颗粒可大幅度提高固定化酶的催化活性,响应电流从相应浓度的几十纳安增强到几千纳安,从理论和实验上证明了     

亲水金和憎水二氧化硅纳米颗粒对葡萄糖生物传感器响应灵敏度的增强作用

用亲水金、憎水二氧化硅纳米颗粒固定葡萄糖氧化酶 (GOD) ,采用聚乙烯醇缩丁醛 (PVB)为辅助固酶膜基质来制备葡萄糖生物传感器 ,并考察了亲水金、憎水二氧化硅纳米颗粒对酶电极电流响应的影响 .实验表明 ,引入纳米粒子可显著增强电极响应灵敏度 .并对两种不同性质纳米颗粒所起作用的可能机理进行讨论 ,从理论和实验上证明了纳米颗粒对固定酶的作用 .为制备有实用价值的葡萄糖生物传感器提供了可供参考的实验和理论依据 .     

亲水金和憎水二氧化硅纳米颗粒对葡萄糖生物传感器响应灵 …

用亲水金、憎水二氧化硅纳米颗粒固定葡萄糖氧化酶（ＧＯＤ）,采有聚乙烯醇缩丁醛（ＰＶＢ）为辅助固酶膜基质来制备葡萄糖生物传感器,并考察了亲水金、憎水二氧化硅纳米颗粒对酶电极电流响应的影响。实验表明,引入纳米粒子可显著增强电极响应灵敏度,并对两种不同性质纳米所起作用的可能机理进行讨论,从理论和实验上辛 明了纳米颗粒对固定酶的作用。为制备有实用价值的葡萄糖生物传感器提供了可供参考的实验和理论依据。     

纳米颗粒复合材料增强的葡萄糖生物传感器

二氧化硅和金或铂组成的复合纳米颗粒可以大幅度地提高葡萄糖生物传感器的电流响应,其效果明显优于这三种纳米颗粒单独使用时对葡萄糖生物传感器的增强作用。除了具有吸附浓缩效应,吸附定向和量子尺寸颗粒 应外,复合纳米颗粒比单独一种纳米颗粒更易于形成连续势场,降低电子在电极和固定化酶间的迁移阻力,提高电子迁移率,有效地加速了酶的再生过程,因此复合纳米颗粒显著增强了传感器电流响应。     

金属纳米颗粒的制备及其在酶生物传感器中的应用研究

近年来,金属纳米颗粒的制备研究引起了人们的广泛兴趣.与相应的块体材料相比,金属纳米颗粒具有独特的化学和物理性质,可应用于电学、催化、磁性材料、光催化、生物染色剂、药物输送等许多领域.其中,传感器是纳米颗粒最有前途的应用领域之一.传感器的微型化是传感器发展的主要研究方向,将纳米颗粒用于传感器的研究将促进这一目标的实现.本论文利用纳米颗粒材料的独特效应来提高葡萄糖传感器的响应电流.将自制的银-金、铂以及二氧化硅和铂复合纳米颗粒用于固定化酶,使酶电极的电流响应值得到了大幅度的提高,从而为纳米增强的新型葡萄糖生物传感器的研究、制备和应用提供了可供参考的实验和理论依据,并为传感器的小型化开辟了一条新途径.论文的主要结果如下:     

天青Ⅰ为电子媒介体金纳米颗粒修饰葡萄糖生物传感器

用纳米金溶胶与聚乙烯醇缩丁醛(PVB)构成复合固酶基质,采用溶胶凝胶法固定葡萄糖氧化酶(GOx)于铂金电极表面,并在葡萄糖溶液中加入天青Ⅰ作为电子媒介体,制成了新型葡萄糖生物传感器。实验证明,葡萄糖氧化酶吸附在纳米金颗粒表面上稳定且保持其生物活性;而电子媒介体的存在,显著提高了传感器的响应灵敏度。该传感器对葡萄糖响应的线性范围为2.5×10-5～7.5×10-3mol/L;检出限为8.5×10-6mol/L(S/N=3)。该生物传感器用于人体血清中的葡萄糖测定,结果令人满意。     

光照纳米银颗粒对葡萄糖生物传感器响应电流的抑制

采用纳米银-壳聚糖复合膜固定葡萄糖氧化酶,构建葡萄糖生物传感器.利用计时电流法对不同光照时间纳米银颗粒组装的酶电极响应电流进行了表征.实验结果表明,光照纳米银颗粒可以抑制葡萄糖生物传感器的响应电流;随着光照时间的延长,纳米银颗粒的抑制作用逐渐增强,当光照时间达到120min时,葡萄糖生物传感器的响应电流最小(-3.953μA/cm2).葡萄糖生物传感器响应电流的抑制可能是由纳米银颗粒表面的Ag+离子浓度及表面性能的变化引起的.     

高分子对酶,抗体DNA的修饰,固定化及其生物医学应用

为发展适于生物医用的生物功能高分子材料，本实验室近年来研究了可溶性高分子对Ｌ－天冬酰胺酶的修饰，纳米磁性高分子微粒对酶或抗体的固定化，亚微米高分子微球固定化碱性磷酸酶及其在ＤＮＡ检测中的应用，高分子微球固定化酶的合成与性能，酶在导电高分子膜上的固定化及生物传感器制备等，本文对此进行简要总结。     

CuTAPc-Fe3O4纳米复合粒子及其漆酶固定化研究

漆酶的固定化研究对基于漆酶催化的光纤生物传感器具有十分重要的意义，制备了四氨基酞菁铜(CuTAPc)-Fe3O4纳米复合粒子，并用红外(IR)、场发射扫描电镜(FEG—SEM)、X射线衍射(XRD)、能谱、粒径仪等对其进行了表征．结果表明形成了以CuTAPc包覆在Fe3O4纳米粒子表面的纳米复合粒子，粒子呈现不规则球形，且分布均匀，粒子平均粒径在50nm左右，用此纳米复合粒子通过戊二醛交联法固定了漆酶，固定后的酶比游离酶具有更好的贮存稳定性及操作稳定性，这为研制高性能的光纤生物传感器打下了较好的基础。     

Glucose biosensor enhanced by nanoparticles

Glucose biosensors have been formed with glucose oxidase (GOD) immobilized in composite immobilization membrane matrix, which is composed of hydrophobic gold, or hydro-philic gold, or hydrophobic silica nanoparticles, or the combination of gold and silica nanoparticles, and polyvinyl butyral (PVB) by a sol-gel method. The experiments show that nanoparticles can significantly enhance the catalytic activity of the immobilization enzyme. The current response can be increased from tens of nanoamperometer (nA) to thousands of nanoamperometer to the same glucose concentration, and the electrodes respond very quickly, to about 1 min. The function of nanoparticles effect on immobilization enzyme has been discussed.     

纳米增强型毛细管酶柱用于葡萄糖液滴生物传感器的研究

葡萄糖的检测在临床医学以及食品工业等领域中十分重要.以往的检测方法主要包括化学发光法[1]、吸光光度法[2]、电化学法[3]和荧光法[4]等.固定化酶柱的制作是发展葡萄糖传感器的关键技术之一.传统的固定化方法主要是将具有生物活性的酶通过物理吸附、共价键合和交联的方法固定于载体基质上或包埋于有机聚合物的基质中.近期研究[5,6]表明,采用溶胶凝胶(Sol-gel)法将蛋白质和酶等生物活性物质包埋于无机陶瓷或玻璃材料内,保持生物组分的活性,且SiO2作为基质材料具有较好的坚固性、抗磨性、化学惰性以及高的光稳定性和透过性,但目前该法多用于电化学型生物传感器[7,8].本文利用纳米颗粒的比表面积大和吸附能力强等特点,将酶吸附在SiO2纳米颗粒表面,用易成膜的聚乙烯醇缩丁醛(PVB)作辅助基质在毛细管上固定酶,并采用分立式酶柱,克服了以往混合型酶柱普遍存在的酶促效率不高和使用寿命较短的局限性.所制得的酶柱具有表面反应活性高、表面活性中心多和催化效率高等特点.结合自行设计的液滴光化学传感装置[9,10],建立了一种高效、快速、微量的葡萄糖实时检测方法.     

Glucose oxidase–magnetite nanoparticle bioconjugate for glucose sensing

Immobilization of bioactive molecules on the surface of magnetic nanoparticles is of great interest, because the magnetic properties of these bioconjugates promise to greatly improve the delivery and recovery of biomolecules in biomedical applications. Here we present the preparation and functionalization of magnetite (Fe₃O₄) nanoparticles 20 nm in diameter and the successful covalent conjugation of the enzyme glucose oxidase to the amino-modified nanoparticle surface. Functionalization of the magnetic nanoparticle surface with amino groups greatly increased the amount and activity of the immobilized enzyme compared with immobilization procedures involving physical adsorption. The enzymatic activity of the glucose oxidase-coated magnetic nanoparticles was investigated by monitoring oxygen consumption during the enzymatic oxidation of glucose using a ruthenium phenanthroline fluorescent complex for oxygen sensing. The glucose oxidase-coated magnetite nanoparticles could function as nanometric glucose sensors in glucose solutions of concentrations up to 20 mmol L^–1. Immobilization of glucose oxidase on the nanoparticles also increased the stability of the enzyme. When stored at 4°C the nanoparticle suspensions maintained their bioactivity for up to 3 months.     

基于DNA链置换反应的新型固定化酶反应器制备及应用

建立了一种新型的酶固定化方法,采用DNA链置换反应成功地在单链DNA标记的磁性纳米粒子上实现了酶的链置换无损更替。该技术可实现目标酶的再利用,节约了生产成本。制备的固定化胰蛋白酶微反应器具有较好的重复利用性和高酶切效率,重复使用10次后仍可保持原酶活性的86%;利用链置换反应制备的MNPs@DNATrypsin酶切马心肌红蛋白5 min后,即可获得95%±0%(n=3)的氨基酸序列覆盖率,远超过相同条件下自由酶酶切12 h的结果。实验表明,发展的固定化酶技术具有高磁响应性,便于从反应体系中回收固定化酶和重复使用,同时此技术可显著提高酶活性,因此可用于固定各种重要的酶,同时可将其广泛应用于各种酶促反应中。     

Fabrication of poly(ethylene glycol)‐based hydrogels entrapping enzyme‐immobilized silica nanoparticles

In this study, we immobilized enzymes by combining covalent surface immobilization and hydrogel entrapment. A model enzyme, glucose oxidase (GOX), was first covalently immobilized on the surface of silica nanoparticles (SNPs) via 3‐aminopropyltriethoxysilane (APTES), and the resultant SNP‐immobilized enzyme was physically entrapped within photopolymerized hydrogels prepared from two different molecular weights (MWs) (575 and 8000 Da) of poly(ethylene glycol)(PEG). The hydrogel entrapment resulted in a decrease in reaction rate and an increase in apparent K_m of SNP‐immobilized GOX, but these negative effects could be minimized by using hydrogel with a higher MW PEG, which provides higher water content and larger mesh size. The catalytic rate of the PEG 8000 hydrogel was about ten times faster than that of the PEG 575 hydrogel because of enhanced mass transfer. Long‐term stability test demonstrated that SNP‐immobilized GOX entrapped within hydrogel maintained more than 60% of its initial activity after a week, whereas non‐entrapped SNP‐immobilized GOX and entrapped GOX without SNP immobilization maintained less than 20% of their initial activity. Incorporation of SNPs into hydrogel enhanced the mechanical strength of the hydrogel six‐fold relative to bare hydrogels. Finally, a hydrogel microarray entrapping SNP‐immobilized GOX was fabricated using photolithography and successfully used for quantitative glucose detection. Copyright © 2009 John Wiley & Sons, Ltd.     

Protease Immobilization on γ‐Fe2O3/Fe3O4 Magnetic Nanoparticles for the Synthesis of Oligopeptides in Organic Solvents

The use of nanobiocatalysts, with the combination of nanotechnology and biotechnology, is considered as an exciting and rapidly emerging area. The use of iron oxide magnetic nanoparticles, as enzyme immobilization carriers, has drawn great attention because of their unique properties, such as controllable particle size, large surface area, modifiable surface, and easy recovery. In this study, various γ‐Fe₂O₃/Fe₃O₄ magnetic nanoparticles with immobilized proteases were successfully prepared by three different immobilization strategies including A) direct binding, B) with thiophene as a linker, and C) with triazole as a linker. The oligopeptides syntheses catalyzed by these magnetic nanoparticles (MNPs) with immobilized proteases were systematically studied. Our results show that i) for magnetic nanoparticles immobilized α‐chymotrypsin, both immobilization strategies A and B furnished good reusability for the Z‐Tyr‐Gly‐Gly‐OEt synthesis, the MNPs enzymes can be readily used at least five times without significant loss of its catalytic performance: ii) In the case of Z‐Asp‐Phe‐OMe synthesis catalyzed by magnetic nanoparticles immobilized thermolysin, immobilization Strategy B provided the best recyclability: iii) For the immobilized papain, although Strategy A or B afforded an immobilized enzyme for the first cycle of Z‐Ala‐Leu‐NHNHPh synthesis in good yield, their subsequent catalytic activity decreased rapidly. In general, the γ‐Fe₂O₃ MNPs were better for use as an immobilization matrix, rather than the Fe₃O₄ MNPs, owing to their smaller particle size and higher surface area.     

Immobilization of glucose oxidase on nylon membranes and its application in a flow-through glucose reactor

The immobilization of glucose oxidase on hydrolyzed nylon-6,6 was studied. Various spacers were introduced on the support before the coupling of the enzyme. Best results were obtained when the membrane was covered with denatured bovine serum albumin (BSA) before spacer coupling and immobilization of glucose oxidase (GOD). The influence of various factors (pH, ionic strength, etc.) on the activity of the free and immobilized enzyme was investigated. It was found that the behavior of the fixed glucose oxidase and the free enzyme is very similar. The covalently immobilized enzyme had a lifetime of around 2 months (50% of initial activity).     

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.