Synthesis,characterization of naphthalene‐based polyimides,and their use as immobilized enzyme membrane

A new monomer, 1,5‐bis(p‐dimethylaminophenylimino)naphthalene, was prepared through Schiff‐base condensation reaction of 1,5‐diaminonaphthalene and 4‐(dimethylamino)benzaldehyde in the presence of ethanol. A series of aromatic polyimides bearing naphthalene and ? CH?N? groups were synthesized from the diamine with five kinds of commercial dianhydrides via a conventional one‐stage process. The resulting naphthalene based polyimides (NBPs) showed good solubilities in N‐methyl‐2‐pyrrolidone and m‐cresol. NBPs had glass‐transition temperatures at 139–174°C and 10% weightloss temperatures above 430 °C in nitrogen atmospheres. Excellent properties of NBPs are attributed to the incorporation of the naphthalene and ? CH?N? group in 1,5‐bis(p‐dimethylaminophenylimino)naphthalene. Moreover, chemically prepared polyimides were used for immobilization of glucose oxidase (GOx). The amperometric responses of the NBPs‐GOx‐Pt electrodes toward glucose were examined at a potential of 0.7 V in PBS solution by means of time‐base (TB) technique. Results show that NBPs bearing ? O? group membrane (PI‐3) has many advantages in the immobilization of glucose oxidase because of its strong adherence to electrode surface and chemical stability and selectivity. Copyright © 2010 John Wiley & Sons, Ltd.     

黄嘌呤氧化酶－乙醛－吖啶酯化学发光分析新体系

乙醛在黄嘌呤氧化酶催化作用下，被空气氧化生成乙酸和过氧化氢，酶反应生成的过氧化氢氧化新吖啶酯试剂［１０－甲基－９－（对甲酰苯基）吖啶羧酸酯氟磺酸盐］产生化学发光，化学发光强度与己醛浓度在一定范围内成线性关系．由此建立了一种化学发光分析新体系，用于测定乙醇含量．线性范围２．０×１０－７～１．２×１０－３ｍｏｌ／Ｌ，测定５．０×１０－７ｍｏｌ／Ｌ乙醛，相对标准偏差为６．８％，检测限为１．２×１０－７ｍｏｌ／Ｌ，测定环境水样中乙醇含量，取得满意结果，回收率为９５～１０６％．     

O2 binding to cytochrome c oxidase-inspired nanomaterials

We investigate O₂ binding to cytochrome c oxidase (CcO)-inspired nanomaterials using ab initio density functional calculations. We consider iron-porphyrin (FeP) and copper-(imidazole)₃ [Cu(Im)₃] as a representative of the active binuclear center, and explore the effect of the Cu(Im)₃ on the FeP-O₂ adduct in relation to the geometric, vibrational, electronic and energetic properties. We find that the Cu(Im)₃ induces the weak O-O and Fe-O bonds mainly because of the electron transfer to the O₂ and the spin polarization of the Fe and O₂ by bridging the O₂ between the Fe and Cu, possibly resulting in the facile O₂ dissociation.     

A Novel Cholesterol Oxidase Biosensor Based on Pt-nanoparticle /Carbon Nanotube Modified Electrode

A variety of electrochemical biosensors for cholesterol detection have been proposed because of its importance in clinic and food analysis 1-2. Classical devices for the detection were based on monitoring either the consumption of oxygen or the production of H2O2. The amperometric determination of H2O2 oxidation is sensitive and stable, but it requires a high anodic potential (over 0.6 V vs Ag/AgCl) and is affected by co-oxidable substances such as ascorbic acid and uric acid usually presen…     

Glucose Measurement Using an Enzymatic Oscillatory Reaction

In biological systems, oscillatory reactions are often found. These reactions, so‐called biological oscillators, have a characteristic oscillation period ranging from seconds to years [1]. For the oscillation in which an enzyme is involved, the reaction has been studied both experimentally [2–5] and theoretically [6–10]. In many cases, temperature control, stirring, or continuous flow of the reactant is necessary to observe continuous oscillation. No trial has been made yet to control the oscillation period or waveform. Here, we report an enzymatic oscillation reaction using catalase and glucose oxidase in which the oscillation period and waveform can be changed by the addition of glucose. We achieved good reproducibility with an oscillation period and waveform change that was sufficient to be applied to the glucose quantification. The effect of coexisting chemicals such as ascorbic acid, urea, or acetamidophenol on the oscillation is examined.     

Enzymatic reactions in supercritical gases

The enzyme polyphenol oxidase has been found to be catalytically active in supercritical carbon dioxide and fluoroform: it readily oxidizesp-cresol andp-chlorophenol to their correspondingo-benzoquinones.     

Mechanistic studies of reactions catalysed by diamine oxidase using isotope effects

Diamine oxidase (DAO), the enzyme that is responsible for amine biodegradation in animals, plants and humans, catalyses the biotransformation of amines such as histamine (HA), putrescine, 1-phenylethylamine, tyrosine, tryptamine, serotonine and spermine. The kinetic and solvent isotope effects (SIEs) were applied to study the mechanism of the biotransformation using HA and its methylderivatives. The SIE for the biotransformation of HA, N^τ-methylhistamine and N^π-methylhistamine was found to be 3.58, 2.22 and 5.70 on V_max, and 1.58, 1.06 and 1.14 on V_max/K_M, respectively. On the other hand, the kinetic isotope effect for oxidation of stereospecifically deuterium-labelled [(α R)-²H]-N^τ-methylhistamine and [(α R)-²H]-N^π-methylhistamine was 0.69 and 0.62 on V_max, and 15.06 and 7.50 on V_max/K_M, respectively. These results demonstrate that DAO catalyses amine biotransformation by stereospecifically cleaving the αC\bond H bond in the pro-S position. Moreover, the oxidation of amine to aldehyde involves several transition states, including hybridisation change from sp³ (Schiff base) to sp² (imine), then back again to sp³ to give a final product with hybridisation sp² (aldehyde).     

A novel amperometric glucose biosensor based on reconstitution of glucose oxidase on thiophene-3-boronic acid polymer layer

The biosensor was constructed for determination of glucose by using glucose oxidase enzyme immobilized on poly(thiophene-3-boronic acid) (PTBA). Boronic acid functionalized polythiophene layer was obtained by electrochemical polymerization of Thiophene (Th) and thiophene-3-boronic acid (TBA) with different monomer rations. The reconstitution of the apo-glucose oxidase (apo-GOx) on a complexed flavin adenine dinucleotide (FAD) linked to polythiophene boronic acid (PTBA) monolayer yields an electrically contacted enzyme monolayer. The GOx-reconstituted enzyme electrode exhibited excellent electrocatalytic activities toward the reduction and oxidation of hydrogen peroxide as well. The PTBA/FAD/GOx biosensor shows an excellent performance for glucose at +0.4 V with a high sensitivity (2.14 μA/mM) and lower response time (～5 s) in a wide concentration range of 0.5–18 mM (correlation coefficient of 0.9952). Furthermore, the effects of applied potential, pH, temperature, electroactive interference, stability and reusability of the biosensors were discussed.     

Interaction between isoamyl adenine and rice cytokinin oxidase

Cytokinin (CTK) dehydrogenase is responsible for regulating the endogenous CTK content by oxidative removal of the side chain. Herein, we have applied fluorescence method to study the interaction between CTK dehydrogenase and CTK in vitro and obtain some parameters of their interaction. We found that addition of isopentenyl adenine can quench the fluorescence of CTK dehydrogenase, and the quenching mechanism was to be a static quenching procedure. We have measured the number of binding sites n and the apparent binding constant K and have calculated the thermodynamics parameter ΔH, ΔG, and ΔS by fluorescence quenching method. Based on thermodynamics parameter’s results, we concluded that their binding reaction was both entropy driven and the enthalpy driven, and the Van der Waals force and hydrogen bond force played a major role in the interaction. Based on the synchronous fluorescence spectrometry results, we demonstrated that the binding site between isopentenyl adenine and CTK dehydrogenase is in the microenvironment of both tryptophan and tyrosine. The fluorescence signal of coenzyme, flavin adenine dinucleotide, decreases gradually with the addition of isopentenyl adenine. And this method can be used for isopentenyl adenine routine assay. Under optimized experimental parameters, the linear segment increases from 0.6 µM to 100 µM with a regression equation of ΔF = 0.04 + 0.15c_ip (r = 0.999, c_ip in µM) with the detection limit of 0.15 µM iP.     

Erythrina alkaloids from leaves of Erythrina arborescens

Continued interest in Erythrina alkaloids resulted in the isolation of 38 alkaloids including 7 undescribed ones from the leaves of Erythrina arborescens Roxburgh. Among the new compounds, erythrivarines H-I were two dimeric alkaloids, while others were Erythrina alkaloid glucosides. Dimeric Erythrina alkaloids and monomers, turcomanidine and isoboldine, showed medium xanthine oxidase inhibition.