无定形硒纳米粒子的交联酶模板法合成及其在生物传感器中的应用

本文以戊二醛交联的辣根过氧化物酶(HRP)为模板合成了均匀分散的无定形硒纳米粒子(粒径10~20 nm)，以所得合成产物为载体构建了HRP生物传感器。研究结果表明，无定形硒纳米粒子具有良好的生物相容性和吸附性，所得传感器灵敏度高，对测定底物的生物亲和性好。     

Synthesis of Nitroanilines Catalyzed by Horseradish Peroxidase in the Presence of NaNO2 and H2O2

The synthesis of nitroanilines catalyzed by horseradish peroxidase（HRP） in the presence of sodium nitrite and hydrogen peroxide was investigated, o-Nitroaniline and p-nitroaniline were found in the nitrated products. 2-Aminotoluene and 4-aminotoluene could also be nitrated to give corresponding nitrated products. This protocol has great potentials to open new avenues useful for the synthesis of nitroaniline and its derivatives.     

Nitration Reaction Catalyzed by Horseradish Peroxidase in the Presence of H2O2 and NaNO2

The enzymatic nitration of phenol and m-cresol catalyzed by horseradish peroxidase was studied in the presence of H2O2 and NaNO2. The results showed that the nitration products of phenol were 2-nitro and 4-nitrophenols. There was also a small amount of by-products of hydroquinone and catechol. The influences of various reaction parameters, including pH, organic solvent type, and concentrations of NaNO2 and H2O2, on the nitration products were investigated. The yields of 4-nitrophenol and 2-nitrophenol were 14% and 12%, respectively. The nitration products of m-cresol were 4-nitro-m-cresol and 6-nitro-m-cresol, and the yields of 4-nitro-m-cresol and 6-nitro-m-cresol were 19% and 30%, respectively.     

增强辣根过氧化物酶催化鲁米诺化学发光反应的新型增强剂四苯硼钠

报道了新型增强剂四苯硼钠对过氧化物酶催化鲁米诺－过氧化氢发光反应的增强作用，建立了流动注射化学发光测定或辣过氧化物酶（ＨＲＰ）的新体系。用该体系测定ＨＲＰ线性范围为１．０×１０－１２×１．２×１０－１３ｍｏｌ／Ｌ；检测限为０．６×１０－１３ｍｏｌ／Ｌ。对０．６×１０－１３ｍｍｏｌ／Ｌ的 ＨＲＰ进行１１次平行测定，相对标准偏差为 １． ５％。     

Electrochemical Detection of Horseradish Peroxidase at Zeptomole Level

Horseradish peroxidase (HRP) is the archetypal heme peroxidase. The determination of HRP is considerably important in clinical chemistry and analytical biochemistry, because HRP is the commonly used enzyme label for immunological detection systems1. We developed a novel method based on its catalytic reaction. A capillary catalytic reaction system was designed (Figure 1). In the assay, both HRP and H2O2 are injected into the polyacrylamide-coated injection capillary (10) by electromig…     

Horseradish Peroxidase Catalyzed Polymerization of Tyrosine Derivatives for Nanoscale Surface Patterning

Abstract

Tyrosine and its derivatives can be polymerized by enzymatic catalysis with horseradish peroxidase (HRP). In the present study, tyrosine ethyl ester hydrochloride was nanopatterned on mercaptohexadecanoic acid (MHA) modified gold surfaces using dip‐pen nanolithography (DPN). Enzymatic polymerization was carried out on the well‐organized nanofeatures and confirmed by atomic force microscopy (AFM) phase images and electrostatic force microscopy (EFM) phase‐lag images. The results extend DPN to amino acid derivatives as biocompatible conducting circuitry with nanoscale features.     

稀土铽离子对辣根过氧化物酶活力指数的影响(英)

0IntroductionHorseradishperoxidase(HRP)isaplanthemeenzymecatalyzingoxidationofawidevarietyofaro鄄maticmoleculesbyhydrogenperoxideanditisthemostwidelystudiedmemberoftheperoxidasefamily[1~3].ThecrystalstructureofHRPhasbeensolved[2].ThestructuralfeaturesofHR…     

辣根过氧化物酶分光光度法测定黄嘌呤氧化酶的活性

研究了以辣根过氧化物酶-苯酚-4-氨基安替比林反应显色新体系,检测黄嘌呤氧化酶(XOD)活力的新方法。确定该酶活性测定的最佳条件为:辣根过氧化物酶(HRP)7000 U/L,4-氨基安替比林(AAP)1 mmol/L,苯酚(PA)6 mmol/L,黄嘌呤(XAN)1 mmol/L溶于50 mmol/L Tris-CL缓冲液(pH 8.4);反应温度为37℃,保温时间为20 m in;检测波长为508 nm。本方法测定XOD酶活的线性范围为5.0~100.0 U/L,线性关系良好(r=0.9992),检出限为1.3 U/L。该方法操作简单易行,测定结果准确可靠。可有效应用于普通实验室和临床常规生化检测。     

循环连续流动分析法测定辣根过氧化物酶的活性

基于H2O2-辣根过氧化物酶(HRP)-邻苯二胺(OPDA)催化反应体系,建立了测定游离及固定化HRP酶活性的循环连续流动分析法(CCFA).CCFA实现了反应液、反应过程的循环连续检测.用CCFA法对酶催化反应条件进行研究,得到的最佳反应条件是:pH 5.0,反应温度27 ℃, 66.0 μmol/L H2O2 , 2 mg/L OPDA,缓冲液为0.1 mol/L柠檬酸-柠檬酸钠缓冲液; 测定游离HRP的线性范围为0～10 U/L,检出限为0.21 U/L,RSD＜1.03%.使用CCFA法测定了固定化HRP的活性,并对HRP酶促动力学进行了研究,得到的游离HRP的米氏常数为0.078 mmol/L,最大反应速度为0.26 mmol/(L min),催化常数为5.2 × 104 min-1.CCFA法操作简便、准确度高、节省试剂、易于实现自动化.     

纳米二氧化钛对辣根过氧化酶催化作用

将辣根过氧化物酶(HRP)固定在二氧化钛(TiO2)纳米颗粒或纳米管修饰玻碳电极(GC)上,形成纳米TiO2微粒/HRP修饰GC电极和TiO2纳米管/HRP修饰GC电极.比较了HRP在纳米TiO2微粒、TiO2纳米管电极上的直接电子转移反应.实验表明,HRP在TiO2纳米管电极表面更能有效地促进它的电活性中心发生电子交换反应.此外,还测定了HRP标记抗体的电化学性能,为抗原抗体免疫反应信号的选择提供了参考依据.     

基于伴刀豆球蛋白固定过氧化物酶无介体新型生物传感器的研制

以纳米金吸附辣根过氧化物酶,用活化的伴刀豆球蛋白(Con A)将其固定在裸金电极表面,研制成一种新型的无介体辣根过氧化物酶生物传感器。探讨了纳米金的尺寸、组装膜层数、工作电位和pH等实验条件对传感器性能的影响。在pH7.0,外加电压-150mV(vs.SCE)条件下,传感器对H2O2在5.0×10-6~1.2×10-2mol/L范围内呈线性关系;检出限为2.9×10-6mol/L。将传感器用于实际样品的测定,结果良好。     

辣根过氧化物酶直接电化学传感器检测过氧化物的研究

该文以高比表面积的泡沫镍电极(Ni foam)为基础,通过电沉积碳纳米管(CNTs)制备了CNTs/Ni foam。然后在十六烷基三甲基溴化铵(CTAB)的辅助下,通过一步法电沉积纳米金(AuNPs)将辣根过氧化物酶(HRP)固定到电极表面,制备了HRP-AuNPs/CNTs/Ni foam直接电化学酶传感器。并采用SEM、能谱(EDS)和电化学方法对该电极进行了表征,优化了测试电位和pH值,将该传感器对过氧化氢及2种有机过氧化物进行了检测。结果表明,该传感器性能良好,对过氧化氢、过氧化氢异丙苯、2-过氧化丁酮具有良好的催化检测性能,其检出限分别为1.2×10~(-7)、4.5×10~(-7)、2.5×10~(-7) mol/L。     

一步电沉积法构建辣根过氧化物酶传感器

在恒电位沉积钴铝水滑石(CoAl-LDH)时将辣根过氧化物酶(HRP)和碳纳米管(CNTs)固定于基底电极表面,构建CoAl-LDH-HRP-CNTs修饰电极并用于过氧化氢的检测。 利用SEM对电化学沉积的CoAl-LDH-HRP-CNTs的形貌进行了表征。 采用电化学阻抗对所制备的电极进行了表征。 用循环伏安法对电极的电化学行为进行了研究。 探讨了pH值和测定电位对修饰电极的催化还原性能的影响。 该传感器对过氧化氢的检测在2.5×10^-6~3.35×10^-4 mol/L范围内呈良好的线性关系,灵敏度为0.0049 A·L/mol。     

Determination of Mercury at the Picogram per Milliliter Level Using Immobilized Horseradish Peroxidase

Abstract

New test method and test device for the mercury (II) determination at the pg/mL level were developed based on the mercury inhibitory action on horseradish peroxidase immobilized on solid supports – in the cells of the polystyrene plate and on the chromatographic paper. The reactions of o-dianisidine, 3,3′,5,5′-tetramethylbenzidine and o-phenylenediamine oxidation by hydrogen peroxide were used as the indicator reactions. The mercury inhibitory effect increased in the presence of thiourea. Under the elucidated optimal conditions the calibration curves for the mercury determination showed a linear relationship between the peroxidase inhibition degree and the mercury concentration in the range of 0,1–1000 pg/mL. The mercury detection limits were 0,1–10 pg/mL in dependence on the concrete indicator reaction. The analysis completed in 15 min. The proposed test device was applied to the mercury determination in underground waters of Moscow region. The mercury content obtained was coincident with that obtained by atomic-fluorescent method with cold vapour.     

Multicommutated Flow Analysis System for Determination of Horseradish Peroxidase and Its Inhibitors

A fully mechanized multicommutated flow analysis (MCFA) system dedicated to determining horseradish peroxidase (HRP) activity was developed. Detection was conducted using a flow-through optoelectronic detector-constructed of paired LEDs operating according to the paired emitter-detector diode (PEDD) principle. The PEDD-MCFA system is dedicated to monitoring the enzyme-catalyzed oxidation of p-phenylenediamine (pPD) by a hydrogen peroxide. Under optimized conditions, the presented bioanalytical system was characterized by a linear response range (33.47–200 U/L) with a detection limit at 10.54 U/L HRP activity and 1.66 mV·L/U sensitivity, relatively high throughput (12 signals recordings per hour), and acceptable precision (RSD below 6%). Additionally, the utility of the developed PEDD-MCFA system for the determination of HRP inhibitors allowing the detection of selected thiols at micromolar levels, is demonstrated. The practical utility of the flow system was illustrated by the analysis of some dietary supplements containing L-cysteine, N-acetylcysteine, and L-glutathione.     

碳纳米管电极上辣根过氧化物酶的直接电化学

制备了碳纳米管修饰玻碳电极(CNT/GC).将辣根过氧化物酶(HRP)固定在CNT/GC电极表面,形成HRP-CNT/GC电极.研究了HRP的直接电子转移.实验结果表明,HRP在CNT/GC电极表面能进行有效和稳定的直接电子转移反应,其循环伏安曲线上表现出一对良好的、几乎对称的氧化还原峰;式量电位E^0'几乎不随扫速(至少在20～100 mV/s的扫速范围内)而变化,其平均值为(-0.319±0.002) V (vs. SCE, pH 6.9); HRP在CNT/GC电极表面直接电子转移的速率常数为(2.07±0.56) s^-1;式量电位E^0'与溶液pH 的关系表明HRP的直接电化学是(1e+1H⁺)的电极过程.进一步的实验结果显示,固定在CNT/GC电极表面的HRP能保持其对H₂O₂还原的生物电催化活性,而且能快速地响应H₂O₂浓度的变化.本文制备碳纳米管修饰电极和固定酶的方法具有简单和易于操作等优点,可用于获得其它生物氧化还原蛋白质和酶的直接电子转移.     

钙离子对HRPC结构和电催化活性影响的研究

通过比较辣根过氧化物酶同工酶C(HRPC)中Ca²⁺移除前后的HRPC的光谱和电化学特性,阐明了Ca²⁺的存在对HRPC的重要作用。移除Ca²⁺后HRPC的紫外-可见吸收光谱发生了变化,Soret带的最大特征吸收峰以及α带和β带特征吸收峰均发生不同程度的蓝移和峰强减弱,表明其血红素微环境及结构发生了变化。移除Ca²⁺后的HRPC也可在与聚L型赖氨酸共修饰的石墨电极上表现出对H₂O₂的催化响应,但是天然HRPC比去除Ca²⁺后的HRPC对H₂O₂表现出更低的检测限,更宽的检测范围,更高的灵敏度以及更好的稳定性。实验结果表明,Ca²⁺对HRPC血红素微环境的保持、催化活性和稳定性均有重要的作用。     

辣根过氧化物酶在亲水性离子液体中的活性与稳定性研究

基于辣根过氧化物酶对过氧化氢氧化愈创木酚这个显色反应的催化作用,研究了辣根过氧化物酶在七种亲水性离子液体[C2mim][BF4]、[C4mim][BF4]、[C6mim][BF4]、[C4mim]HSO4、[C4mim]Cl、[C4mim]NO3、[C4mim][CF3CO2]中的活性与稳定性变化.结果表明辣根过氧化物酶在不同离子液体中均有不同程度的失活,辣根过氧化物酶活性随离子液体极性增强而降低.辣根过氧化物酶在含[C4mim]Cl离子液体的介质中,随着温度升高,[C4mim]Cl对辣根过氧化物酶的失活过程起加速作用,离子液体浓度越高,酶的热稳定性越差.紫外-可见光谱研究表明,在含[Cnmim][BF4]、[C4mim]HSO4、[C4mim]Cl、[C4mim]NO3的介质中,辣根过氧化物酶血红素中心最大吸收峰没有发生变化,但吸收值增强,证明离子液体使酶的血红素基团暴露于介质中而增强了吸收;而在含[C4mim][CF3CO2]的介质中,辣根过氧化物酶血红素基团最大吸收峰区发生蓝移,证明有部分血红素基团被离子液体破坏而脱落.     

明胶固定辣根过氧化物酶制备H_2O_2传感器

用明胶将辣根过氧化物酶(HRP)固定于多壁碳纳米管(MWNT)和茜素红(AR)修饰的玻碳(GC)电极上,制成HRP生物传感器(HRP/AR/MWNT/GC),然后在3%戊二醛(GA)中进行交联改性,以克服明胶膜易溶胀的缺点,并提高膜的稳定性.同时详细探讨了该传感器对H2O2的响应性能,并优化了实验条件.结果表明,该传感器对H2O2的线性响应范围为5.0×10-6～1.0×10-3mol/L,线性相关系数为0.9932,检出限为1.0×10-7mol/L,且放于4℃环境30d后,峰电流值约为原来的72.1%.该传感器响应快速,灵敏度高,且具有良好的重现性、稳定性及较长的使用寿命,具有潜在的应用价值.