抑制型离子色谱法测定白酒中的F-、Cl-、NO2-、H2 PO4-、NO3-

用抑制型离子色谱法测定白酒中的F^-、Cl^-、NO2^-、H2PO4^-、NO3^-。流动相为4mmol／LNa2CO3—3 mmol／LNaHCO3混合溶液,流速为1．5mL／min,进样量为0、5mL,在最佳色谱条件下,5种无机阴离子10min内实现基线分离。F^-、Cl^-、NO2^-、H2PO4^_、NO3^-的检出限分别为0、008、0．012、0、030、0．068、0．077mg／L。测定结果的相对标准偏差分别为1．86％、1．30％、2．06％、1．82％、1．50％,回收率分别为108．0％、94．0％、101．0％、98．7％、94．4％。     

血红蛋白与葡萄糖氧化酶偶联荧光法测定葡萄糖

利用血红蛋白(Hb)作为辣根过氧化物酶(HRP)的模拟酶,催化H2O2与对甲基酚的荧光反应.并将该反应与葡萄糖氧化酶(GOD)催化氧化葡萄糖的反应偶联,建立了测定葡萄糖的荧光分析法.方法的线性范围为0.0～5.0×10-5mol/L葡萄糖.检测限为6.5×10-8mol/L.用于测定人血清中葡萄糖的含量,获得了满意的结果.     

芯片式流通池顺序注射可更新表面反射光谱法用于酶反应检测

将芯片式流通池顺序注射可更新表面反射光谱法用于酶反应检测。HRP催化H2O2氧化BPR底物的反应用于对H2O2的检测。此反应体系与葡萄糖氧化酶联用，用于对血清中葡萄糖的检测。     

基于固定化纳米金增强化学发光双酶传感器测定葡萄糖

研制了一种新型流动注射化学发光（CL）双酶传感器,用于葡萄糖的检测．该传感器将掺杂金纳米粒子（GNPs）的壳聚糖膜包覆在硅烷化试剂预处理的玻璃微珠上,用于吸附固定葡萄糖氧化酶（GOD）和辣根过氧化物酶（HRP）．葡萄糖在GOD的催化下发生氧化反应生成H2O2,生成的H2O2在HRP的催化作用下与鲁米诺发生反应,并产生化学发光信号．实验表明,壳聚糖中掺杂的GNPs不仅能够有效的吸附酶分子并保持其生物活性,还对Luminol-H2O2-HRP化学发光体系具有增敏作用．通过化学发光光谱和紫外光谱表征,详细研究了固定化GNPs增强Luminol—H2O2-HRP体系的化学发光机理．在优化的实验条件下,该传感器对葡萄糖检测的线性范围为0．01～6．0mmol／L,检测限为5．0μmol／L（3σ）．将所建立的方法用于临床血清样品中葡萄糖含量的测定,获得了满意的结果．     

肌红蛋白在海藻酸钠水凝胶中的电化学和电催化特性

海藻酸钠(Sodium Alginate,SA)是由L-葡萄糖醛酸与D-甘露糖醛酸组成的高分子线性糖醛酸,常作为固定化酶包埋材料。本文研究了海藻酸钠水凝胶膜中的肌红蛋白在磷酸盐缓冲溶液中的直接电化学和酶催化性质,探讨了测定H2O2和NO2^-的可能性。     

离子色谱法测定粮食鲜样中的硝酸盐含量

粮食鲜样经超声提取后，用离子色谱法测定浸提液中的硝酸盐。采用DX-100型离子色谱仪．以2．7mmol／L Na2CO3—0．3mmol／LNaHCO3的混合溶液作为淋洗液，流速为1．2mL／min，测定玉米、大豆、小麦中的NO3^-含量。NO3^-浓度在0．5—40．0mg／L范围内与色谱峰高呈良好的线性关系，相关系数r=0．9995，检出限为0．05mg／L，测定结果的相对标准偏差小于5％．加标回收率为96．0％-100．7％。     

葡萄糖氧化酶催化荧光测定的非酶体系研究

多数氧化酶及其底物都是重要的临床检验指标[1]，目前普遍采用酶荧光法或酶显色法，通过氧化酶催化氧化底物生成H刃。，过氧化物酶（HRP）催化H刃2氧化生成荧光／生色底物，实现间接测定［’j．酶法测定的缺点是体系不稳定、反应条件苛刻、费用较高．最近Mitani等［’j报道了非酶法化学发光测定葡萄糖氧化酶，灵敏度高，但需要特殊试剂，且测定时间较长．我们用Fenton反应［‘j将H。O。转化为羟基自由基（“OH），进而氧化对苯二甲酸生成荧光物质，建立了荧光测定葡萄糖氧化酶的非酶法，详细研究了荧光指示剂的选择、Fenton试剂的改进…     

固定化葡萄糖氧化酶活性的X射线微区分析

利用X射线微区分析方法,对固定化活性葡萄糖氧化酶进行了定位分析;葡萄糖作为底物,FeSO4和KI作为捕捉剂,底物经固定化葡萄糖氧化酶催化产生H2O2,后者和捕捉剂反应生成沉淀,可以确定固定化葡萄糖氧化酶的催化活性部位。结果表明：颗粒越小,酶活越高,活性葡萄糖氧化酶在凝胶内分布均匀,且绝大多数葡萄糖氧化酶固定在凝胶的内部。作者还研究了固定化活性葡萄糖氧化酶定位的最佳条件。     

离子色谱法测定马龙茶叶中的F^—、NO2^—、NO3^—

应用离子色谱法测定乌龙茶叶中的F^-、NO2^-和NO3^-。测得3种样品中F^-、NO2^-和NO3^-的含量分别为1.19-1.75、0.000-0.020和0.024-0.058mg/g，回标回收率分别为94.9%、96.7%和93.4%。     

离子色谱法测定AgNO3中的微量Cl-、NO2-和SO42-

用离子色谱法测定AgNO3溶液中的Cl^-、NO2^-和SO4^2-，以5.0mmol/L Na2CO3-5.0mmol/L NaHCO3混合溶液作淋洗液，采用离子交换法将AgNO3转换成KNO3，以除去Ag ^ 。讨论了NO3^-对Cl^-、NO2^-和SO4^2-测定的影响。AgNO3溶液中Cl^-、NO2^-和SO4^2-的回收率分别为93.3%、108%和94%。     

Glucose Biosensor Based on Carbon/PVC-COOH/Ferrocene Composite with Covalently Immobilized Enzyme

A carbon/PVC-COOH/ferrocene composite electrode used for the determination of glucose has been prepared. The ferrocene acted as mediator was incorporated into the PVC-COOH polymer and the leakage could be prevented. The presence of carboxyl groups on the electrode surface allowed immobilizing enzyme via EDC and NHS. The ratio of PVC-COOH to graphite powder （w/w） has been studied. Amperometric determination of glucose has been performed at potential of 0.30 V vs SCE. The response time was 〈 15 s. The linear response range was of 0.1-20 mmol/L with a detection limit of 48μmol/L.     

Nafion-二茂铁-双酶修饰的葡萄糖传感器

用二茂铁作为过氧化物酶与玻碳电极的电子传递体,通过牛血清白蛋白-戊二醛交联剂把葡萄糖氧化酶和过氧化物酶固定在Nafion-二茂铁修饰玻碳电极上,制备成葡萄糖传感器。由于工作电位低,电活性物质如抗坏血酸、尿酸等对测定无干扰。该传感器的线性范围为5.0×10～(-4)～2.5×10～(-2)mol/L,响应时间小于30s.     

电化学葡萄糖传感器

作为电化学生物传感器中最重要的研究内容之一,葡萄糖生物传感器在数十年的发展中取得了巨大进展。本文综述了近年来利用纳米技术设计的新型电化学葡萄糖传感器的主要研究进展,并从纳米材料维度分类进行了讨论。其中,零维纳米材料主要讨论了包括金纳米颗粒、银纳米颗粒以及铜、铂等金属纳米颗粒材料; 一维纳米材料主要讨论了通过模板法制备的金属或金属氧化物纳米线以及单臂或者多壁纳米管材料; 二维纳米材料主要总结了以碳为基础的石墨烯材料和一些片状的金属材料。纳米材料对电化学葡萄糖传感器的影响主要集中在生物相容性、增强检测灵敏度、酶的固定等方面。此外,本文也对电化学葡萄糖传感器的今后发展做了展望。     

Determination of Glucose in Diluted Blood with a Thermal Flow Injection Analysis Biosensor

Abstract

The glucose concentration in diluted whole blood has been measured, using a miniaturized thermal biosensor based on the enzyme thermistor principle. The biosensor is a small flow injection system. A sample volume of 20μl is injected into a flow of 50μl/min. The heat produced when the sample passes the enzyme column is measured with a thermistor connected to a Wheatstone bridge. The enzyme column contains glucose oxidase and catalase co-immobilized on a solid support material. Samples of whole blood usually cause problems in flow-systems. The blood cells tend to block the enzyme column and the back pressure increases. We have tested a superporous agarose material as enzyme support material using tenfold diluted samples of whole human blood. The blood was collected from the finger-tip and diluted with buffer containing an anticoagulant and sodium fluoride. The number of samples possible to inject and the accuracy compared to the Boehringer Mannheim Reflolux have been determined. At least 100 ten-fold diluted blood samples could be injected on a micro-column of superporous agarose. The obtained glucose concentration correlated well with the one obtained with the reference instrument.     

Biological Glucose Metabolism Regulated Peptide Self‐Assembly as a Simple Visual Biosensor for Glucose Detection

A glucose oxidase (GOx)‐mediated glucose metabolism was in vitro mimicked and employed to regulate the self‐assembly of peptide‐based building blocks. In this new stimuli‐responsive self‐assembly system, two peptide‐based building blocks, respectively, having aspartic acid (gelator 1 ) and lysine (gelator 2 ) residues were designed and prepared. When adding glucose and GOx to the aqueous solution of gelator 1 or the self‐assembled fibrillar hydrogel of gelator 2 to construct glucose metabolism system, the metabolic product (gluconic acid) can trigger the protonation of the peptide molecules and induce the phase transitions of gelators 1 (sol‐gel) and 2 (gel‐sol). Because this glucose metabolism regulated peptide self‐assembly is built on the oxidation of glucose, it can be used as a simple visual biosensor for glucose detection.     

N-[3-(4-乙氧基苄基)-4-氯苯基]-1-脱氧野尻霉素的合成及其降血糖作用

以具有降血糖活性的达格列净、卡格列净和脱氧野尻霉素为参照,设计合成了新化合物N-[3-(4-乙氧基苄基)-4-氯苯基]-1-脱氧野尻霉素(A)。以2-氯-5-硝基苯甲酸为原料,先将羧酸转化为酰氯、再经Friedel-Crafts酰基化、羰基还原及硝基还原,合成了中间体2-氯-5-氨基-4'-乙氧基二苯基甲烷;另一方面,以单丙酮葡萄糖为原料,经选择性氧化和水解反应得到5-氧化-D-葡萄糖。该化合物和2-氯-5-氨基-4'-乙氧基二苯基甲烷发生双还原胺化反应得到化合物A的粗品。将粗品A与乙酸酐反应,经柱色谱分离得到高纯度的四乙酰基-N-[3-(4-乙氧基苄基)-4-氯苯基]-1-脱氧野尻霉素(B),再将其水解制得纯的化合物A。将化合物A口服给药SD大鼠后,发现该化合物可以降低SD大鼠血糖,增加尿量和葡萄糖从尿液中的排出。     

一种基于壳聚糖固定葡萄糖氧化酶的葡萄糖生物传感器的研究

本文选用生物相容性好的壳聚糖作为基体材料，使其与戊二醛交联成网状结构包埋葡萄糖氧化酶制成电化学传感器。这种壳聚糖膜不仅可以减小葡萄糖氧化酶的流失，而且能为酶提供了适宜的微环境。用红外光谱、紫外光谱及透射电镜对膜的形态和性质进行了表征。实验结果表明该传感器具有很快的响应速度，很好的稳定性和重现性，能选择性地催化葡萄糖并测定其浓度。该传感器的制备方法简单，成本低，于冰箱中放置两周信号保持在90％以上，对葡萄糖测量的线性范围为1×10^-5 - 3.4×10^-3mol•L^-1，当信噪比为3:1时检测限为5×10^-6mol•L^-1。     

Effect of Hydrolyzable Tannins on Glucose-Transporter Expression and Their Bioavailability in Pig Small-Intestinal 3D Cell Model

Intestinal transepithelial transport of glucose is mediated by glucose transporters, and affects postprandial blood-glucose levels. This study investigates the effect of wood extracts rich in hydrolyzable tannins (HTs) that originated from sweet chestnut (Castanea sativa Mill.) and oak (Quercus petraea) on the expression of glucose transporter genes and the uptake of glucose and HT constituents in a 3D porcine-small-intestine epithelial-cell model. The viability of epithelial cells CLAB and PSI exposed to different HTs was determined using alamarBlue^®. qPCR was used to analyze the gene expression of SGLT1, GLUT2, GLUT4, and POLR2A. Glucose uptake was confirmed by assay, and LC–MS/ MS was used for the analysis of HT bioavailability. HTs at 37 µg/mL were found to adversely affect cell viability and downregulate POLR2A expression. HT from wood extract Tanex at concentrations of 4 µg/mL upregulated the expression of GLUT2, as well as glucose uptake at 1 µg/mL. The time-dependent passage of gallic acid through enterocytes was influenced by all wood extracts compared to gallic acid itself as a control. These results suggest that HTs could modulate glucose uptake and gallic acid passage in the 3D cell model.     

Glucose Biosensor Based on the Fabrication of Glucose Oxidase in the Bio-Inspired Polydopamine-Gold Nanoparticle Composite Film

A highly efficient enzyme immobilization method has been developed for electrochemical biosensors using polydopamine films with gold nanoparticles (AuNPs) embedded. This simple enzyme fabrication method can be performed in very mild conditions and stored in a long time with high bioactivity. The fabricated amperometric glucose biosensor exhibited a high and reproducible sensitivity, wide linear dynamic range and low limit of detection (LOD) (0.1 μmol·L^?1). A low value of 1.5 mmol·L^?1 for the apparent Michaelis‐Menten constant K^app_M was obtained. The high sensitivity, wide linear range, good reproducibility and stability make this biosensor a promising candidate for portable amperometric glucose biosensor.     

Glucose-Responsive Monoolein Cubic Phase Containing Glucose Oxidase

Glucose-responsive monoolein (MO) cubic phase was prepared by immobilizing proteinoid composed of Asp and Leu (PAL) and hydrophobically modified glucose oxidase (HmGOD) onto the MO bilayers. The hydrodynamic mean diameter of PAL aggregate in aqueous solution decreased with increasing the pH value. The number of pamitic acid residue per one molecule of HmGOD was determined to be 6.3 by a calorimetric method. HmGOD could acidify glucose solution in a few hours, possibly because it converted glucose to gluconic acid. PAL- and HmGOD-immobilized MO cubic phase was prepared by hydrating MO melt with the mixture aqueous solution of PAL and HmGOD. The cubic phase exhibited its phase transition around 62.5°C, determined by polarizing microscopy. The release of carboxylic fluorescein (CF) from the cubic phase was suppressed when the pH value of release medium decreased, possibly because PAL can aggregate more at a lower pH value. The release was suppressed when glucose concentration increased, possibly because the release medium can be more acidified and PAL will be more aggregated at a higher glucose concentration. The cubic phase could be used as a drug carrier which releases its content in a sustained manner when the glucose concentration is abnormally high.