Application of enzyme-field effect transistor sensor arrays as detectors in a flow-injection analysis system for simultaneous monitoring of medium components. Part II. Monitoring of cultivation processes

Glucose, maltose, sucrose, lactose, ethanol and urea concentrations were monitored simultaneously during the cultivation of Escherichia coli and Saccharomyces cerevisiae by means of enzyme field effect transistors (EnFETs) applying glucose dehydrogenase (GDH), maltase (MAL)/GDH, invertase (INV)/GDH, β-galactosidase (β-GAL)/galactosedehydrogenase (GALDH), alcoholdehydrogenase (ADH)/aldehydedehydrogenase (ALDH), and urease. These enzymes were (co)immobilized on the pH sensitive gates of an eight-FET array. The FET array was integrated in a commercial FIA system.     

Quinoprotein glucose dehydrogenase modified carbon paste electrode for the detection of phenolic compounds

The development of an amperometric biosensor for the determination of phenolic compounds is described, using quinoprotein glucose dehydrogenase. The enzyme is integrated into carbon paste and its ability to donate electrons to oxidized phenolic compounds during glucose oxidation is exploited. The sensor response is based on electrochemical oxidation of the phenolic compound followed by its enzymatic regeneration when the bulk solution contains glucose and the electrode is potentiostated at +500 mV (vs. Ag/AgCl/0.1 mol/L KCl). As the result of the catalytic analyte regeneration the electrodes offer very sensitive measurements of redox species like p-aminophenol and hydroquinone and catecholamines such as epinephrine, norepinephrine, and dopamine. The sensor performance is characterized for the different substrates. Highest sensitivity is achieved for p-aminophenol which could be determined at sub-nanomolar level.     

薄层扫描法测定冬眠过程中刺猬活性组织酶的周期变化

薄层扫描法测定冬眠过程中刺猬活性组织酶的周期变化冯金城（天津师范大学天津３０００７４）孙金生（天津水产研究所天津３００２２１）１前言为了跟踪观察刺猬在冬眠过程中体内乳酸脱氢酶的周期性变化，利用薄层扫描仪测定了其相关的组织同工酶的差异。实践证明，此法简...     

Electroenzymatic reactions with sorbitol dehydrogenase on gold electrodes

Sorbitol dehydrogenase (SDH) originating from recombinant Escherichia coli cells is immobilized on gold electrodes. First of all, (4-carboxy-2,5,7-trinitrofluorenyliden)malon-nitrile (CTFM) is adsorbed on the surface as mediator. In a second step, the cofactor β-nicotinamide adenine dinucleotide (NAD⁺) is immobilized on the gold electrode. Due to the formation of a complex between the mediator and the cofactor, the electron transfer rate can be enhanced by adding calcium ions to the buffer. The immobilization of NAD⁺ and SDH on the surface has been achieved by cross-linking with the glutaraldehyde/bovine serum albumin system. The successful biofunctionalization is monitored by cyclic voltammetry.Paper presented at the “Jahrestagung der Fachgruppe Angewandte Electrochemie der Gesellschaft Deutscher Chemiker, Düsseldorf, 11.-14.09.2005”.     

土壤微生物ATP、脱氢酶和尿素酶活性的ED50值评价外源镧的生物毒性

０IntroductionRareearthsarenowappliedwidelyinChina，whichcanimprovecropsyieldsandthetheirqualit－ies犤１犦．Thebeneficialeffectsmaybeduetothestimu－latoryeffectsoftheseelementsonthenutrientuptakebyplantsorontheincreasingofchlorophyllsynthesisintheplants犤２犦．Whilealotofresearcheshavebeendoneontheimprovednutritionofcropsafterapplica－tionofrareearths，muchlessattentionhasbeenpaidtothedeteriorationofsoilqualityduetotheapplicationofrareearthsforyears犤３犦．Scientistshavediscoveredthataccumula…     

Purification of a marine bacterial glucose dehydrogenase fromCytophaga marinoflava and its application for measurement of 1,5-anhydro-d-glucitol

A novel glucose dehydrogenase (GDH) from a marine bacteriumCytophaga marinoflava IFO 14170 was isolated from its membrane fraction. This GDH catalyzes the oxidation of a hydroxy group of glucose, but does not react in its C-l position. This enzyme is composed of a single peptide with a mol wt of 67,000. The GDH can react under high salinity. The optimum pH is around 8.0, showing a typical property of marine bacterial enzymes. Using this novel enzyme, an enzymatic determination of 1,5-anhydro-D-glucitol (1,5AG) utilizing 2,6-dichrolophenolindophenol (DCIP) and phenazine methosulfate (PMS) as electron mediators was caried out. A good linear correlation was observed from 0.5 mM to 4 mM of 1,5AG.     

基于可见吸收信号的乳酸脱氢酶光纤传感器

报道一种测定乳酸脱氢酶活力的基于可见吸收信号的光纤生物传感器，在该传感体系中，通过辅酶Ｉ的氧化还原对（ＮＡＤ＾＋／ＮＡＤＨ）将乳酸脱氢酶和心肌黄酶催化的两个脱氢过阳以耦合，第一个脱氢过程对分析对象进行了化学识别，第二个脱氢过程引起可见吸收信号的变化，该传感器对０～４００Ｕ／Ｌ的乳酸脱氢酶有线性响应关系，检测下限为４８ＵＬ，该传感器已用于人体血清中乳酸脱氢酶活力的测定。     

山蝠,绒山蝠和爪哇伏翼乳酸脱氢酶同工酶的比较研究

采用聚丙烯酰胺凝胶盘状电泳法对山蝠,绒山蝠和爪哇伏翼的脑,肾,骨骼肌和胃４种组织的乳酸脱氢酶同工酶进行了研究。结果表明,从酶谱的区带数目,分布,迁移率,各区带相对含量和亚基的相对含量来看,均表明三者的相应组织的酶谱各具特征,而且差异极为显著,表现出很强的种属特异性。     

介体型乳酸脱氢酶生物传感器的研制及应用

本报道了能对丙酮酸产生良好响应的电流型乳酸脱氢酶生物传感器。该传感器以耐尔兰Ａ修饰浸石墨电极为基体电极，将酶直接固化在蚕丝蛋白膜上。在ＰＨ７．４的ＮａＨ２ＰＯ４－ＮａＯＨ介质中，当２．４×１０＾－４ｍｏｌ／Ｌ的辅酶Ｉ（ＮＡＤＨ）存在下，该传感器的响应电流与丙酮酸浓度在３．２×１０＾－５ｍｏｌ／Ｌ范围内有良好的线性关系。响应时间为６０ｓ．本讨论了影响传感器响应的各种因素，用此传感器测定了人血清中     

Preparation and partial characterization of a soluble site-to-site directed enzyme complex composed of alcohol dehydrogenase and lactate dehydrogenase

A soluble, bifunctional enzyme complex has been prepared by crosslinking lactate dehydrogenase and alcohol dehydrogenase with glutaraldehyde. The crosslinking was performed on a solid phase while the active sites of alcohol dehydrogenase and lactate dehydrogenase were held adjacent to one another with the aid of a bis-NAD analog. Subsequently, the enzyme complex was released from the solid phase. The soluble enzyme complex was then purified by using NAD-Sepharose as an affinity adsorbent. Based on gel filtration experiments, the complex was estimated to consist of one of each dehydrogenase. By using a third enzyme, lipoamide dehydrogenase, which competes with lactate dehydrogenase for NADH produced by alcohol dehydrogenase, the effect of site-to-site orientation was studied. It was found that about 83% of the NADH produced by alcohol dehydrogenase was oxidized by site-to-site oriented lactate dehydrogenase compared to a figure of only about 61% obtained in an identical system of separate enzymes. This indicates that given two alternative routes, the preference for the one to lactate dehydrogenase over the one to lipoamide dehydrogenase is enhanced when lactate dehydrogenase and alcohol dehydrogenase are site-to-site oriented.