Theoretical analysis of the enzyme reaction processes within the multiscale porous biocatalytic electrodes

Mathematical model describing the oxidation of glucose in a multiscale porous biocatalytic electrode is discussed. The model considers herein is composed of two nonlinear differential equations accounting for reaction and diffusion within the hydrogel film. In this letter, approximate analytical expressions for the concentration of mediator, substrate and current have been obtained using the Adomian decomposition method (ADM). Furthermore, a comparison confirmed that our analytical result fitted very well with the numerical solution (Matlab). Sensitivity analysis of the parameters is also reported.     

采用磁性载体制备的固定化酶反应器的载体粒径对蛋白质酶解性能的影响

研究了以不同粒径的磁性颗粒为载体的固定化酶反应器在蛋白质酶解过程中,其粒径大小对团聚、酶解效率和漏切位点等的影响。实验结果表明,纳米级颗粒的酶负载量为亚微米级的3.5倍左右。但当酶固定量相同时,酶解效率基本相当。而在一定程度上加大磁性颗粒的粒径后,团聚现象得到明显改善。选择磁性载体粒径为20 nm的固定化酶反应器,对其性能进一步考察。结果显示胰蛋白酶与牛血清白蛋白(BSA)的质量比为1:1时,即能于1 min内实现快速酶解;当酶解10 min时,其零漏切位点肽段数和蛋白质序列覆盖率基本达到稳定,并明显优于溶液酶解水平。通过对漏切位点的统计分析比较,发现固定化酶解与溶液酶解时的漏切位点规律基本类似。因此,采用不同粒径磁性载体制备的固定化酶反应器均可在蛋白质组学研究中提供快速、高效的酶解。     

Development and evaluation of electrochemical glucose enzyme biosensors based on carbon film electrodes

Electrochemical glucose enzyme biosensors have been prepared on carbon film electrodes made from carbon film electrical resistors. Evaluation and characterisation of these electrodes in phosphate buffer saline solution has been carried out with and without pretreatment by cycling in perchloric acid or at fixed applied potential. Both pretreatments led to a reduction in the carbon surface oxidation peak and enabled better detection of hydrogen peroxide in the pH range of 5-7. Glucose oxidase enzyme was immobilised on the carbon surface by mixing with glutaraldehyde, bovine serum albumin and with and without Nafion. The performance of these two types of electrode was similar, that containing Nafion being more physically robust. Linear ranges were up to around 1.5 mM, with detection limits 60 μM, and pretreatment of the carbon film electrode at a fixed potential of +0.9 V versus SCE for 5 min was found to be the most beneficial. Michaelis-Menten constants between 5 mM and 10 mM were found under the different experimental conditions. Coating the immobilised enzyme layer with a thin layer of Nafion was found to give similar results in the determination of glucose to mixing it but with benefits against interferences for the analysis of complex matrices, such as wine. Potentialities, for a short-term-use or disposable sensors, are indicated.     

Nd-Fe-B permanent magnet electrodes. Theoretical evaluation and experimental demonstration of the paramagnetic body forces

Cyclic voltammetry with Nd-Fe-B disk magnet electrodes (3.2 mm diameter) at slow sweep rates (< or = 0.01 V s(-1)) in relatively concentrated solutions (e.g., 80 mM) of diamagnetic redox-active species (e.g., TMPD) is controlled by diffusion. Under similar conditions, cyclic voltammetry with conventional noble metal disk millielectrodes is characterized by the absence of diffusion waves and the presence of density gradient driven natural convection. Although the magnetic field in the vicinity of Nd-Fe-B electrodes is relatively strong (approximately 0.5 T at the surface of the magnet electrode), the absence of magnetohydrodynamic stirring effects is attributed to the fact that the i and B vectors are almost parallel, and therefore the magnetohydrodynamic force F(B) (=i x B) is very small. On the other hand, the absence of natural convection is attributed to the two possible paramagnetic body forces, F(inverted Delta B) and F(inverted Delta C), exerted by the magnet electrode on the diffusion layer. Of those two forces, the former depends on field gradients (F(inverted Delta B) approximately B x inverted Delta B), while the latter depends on concentration gradients (F(inverted Delta C) approximately inverted Delta C(j)) and is directed toward areas with higher concentration of paramagnetic j. Through thorough analysis of the magnetic field and its gradients, it is found that the average F(inverted Delta C) force acting upon the entire diffusion layer is approximately 1.75 times stronger than F(inverted Delta B). Nevertheless, it is calculated that either force independently is strong enough and would have been able to hold the diffusion layer by itself. Further evidence suggests that, integrated over the entire solution, F(inverted Delta B) is the dominant paramagnetic force when the redox-active species is paramagnetic, e.g., [Co(bipy)(3)](ClO(4))(2) (bipy = 2,2'-bipyridine). Finally, convective behavior with diamagnetic redox-active species and magnet millielectrodes can be observed by holding closely (2-3 mm away) a repelling second magnet that bends the induction B to the point that the i x B product is not equal to 0. with Nd-Fe-B disk ma     

Immobilized enzyme reactors in proteomics

Fast, efficient characterization of proteins is becoming one of the hottest topics in the bioanalytical community, especially for large-scale proteomic studies. As an attractive approach, protein digestion by enzymes supported on various matrices (referred to as immobilized enzyme reactors, IMERs) has recently attracted much attention.In this article, we present a critical overview of some highly efficient IMERs and related analytical systems. We give major coverage to applications of IMERs in proteomic analysis, including protein-expression profiling, characterization of proteins with post-translational modifications, and protein quantification. We also comment on promising trends for IMERs in proteomics.     

Ion-selective electrodes and enzyme electrodes in environmental and clinical studies.

Electrodes have been developed for the assay of glucose, urea, amino acids, uric acid, phosphate, nitrate and perchlorate. The electrodes for the organic compounds are enzyme electrodes which are prepared by chemically immobilizing an enzyme over the outside of a conventional ion-selective electrode. These electrodes will be discussed in depth. The progress and the development of the electrodes that show sensitivity and selectivity for phosphate, nitrate and perchlorate will be outlined. The basis of these sensors is a complex of a transition metal of either an analog of thiourea or an organic chelator, such as 1,10-phenanthraline. Such electrodes respond linearly to phosphate, nitrate or perchlorate, and show selectivity over sulphate, halides and acetate. The linear range of all these electrodes is approx. 10(-1)-10(-5) M with a near Nernstian slope and a reproducibility of 1%. The electrodes are stable and can be used continuously.     

Electrochemical performance evaluation of template-assisted and morphology-modified ultra-small-sized NiO as electrodes for supercapacitors

Journal of Solid State Electrochemistry - Nickel oxide is a significant candidate for the supercapacitor electrode application due to its high theoretical capacitance. This work demonstrates the...     

A study of gelled enzyme ultrafiltration reactors

Experiments were carried out in UF reactors with dynamically formed gelled enzyme artificial membranes. Unstirred batch systems and UF reactors with continuous recirculation of the substrate on the membrane were investigated. A significant increase in enzyme stability was tested in both systems. The enzymes used were acid phosphatase, urease, and β-glucosidase. The agreement between the experimental results and the predictions of a simple analytical model for the two classes of UF heterogeneous enzymatic reactors is generally satisfactory.     

Amperometric enzyme electrodes for the determination of l-glutamate

Electrodes for amperometric measurement of l-glutamate were prepared by immobilization of l-glutamate oxidase on an Immobilon-AV Affinity membrane and attachment to an oxygen/hydrogen peroxide sensor. The response of the hydrogen peroxide sensor was linear over the concentration range 5.0 x 10(-8)-5.0 x 10(-4)Ml-glutamate, with a limit of detection of 35nM. Attachment of a size-exclusion membrane (cut-off for molecular weight > 100) or of a hydrophobic oxygen membrane eliminated electro-oxidizable interferences, but the response was attenuated by a factor of 2-3. The response may be amplified 10-fold by co-immobilizing l-glutamate dehydrogenase with the l-glutamate oxidase. The electrode initially lost 25% of its activity but was then stable for more than 320 days and at least 200 assays. The electrode was successfully used to assay glutamate in a protein tablet and in several food products. A flow-injection system was assembled for the continuous assay of l-glutamate.     

Kinetics of redox polymer-mediated enzyme electrodes

Oxygen-reducing enzyme electrodes are prepared from laccase of Trametes versicolor and a series of osmium-based redox polymer mediators covering a range of redox potentials from 0.11 to 0.85 V. Experimentally obtained current density generated by the film electrodes is analyzed using a one-dimensional numerical model to obtain kinetic parameters. The bimolecular rate constant for mediation is found to vary with mediator redox potential from 250 s(-1) M(-1) when mediator and enzyme are close in redox potential to 9.4 x 10(4) s(-1) M(-1) when the redox potential difference is large. The value of the bimolecular rate constant for the simultaneously occurring laccase-oxygen reaction is found to be 2.4 x 10(5) s(-1) M(-1). The relationship between mediator-enzyme overpotential and bimolecular rate constant is used to determine the optimum mediator redox potential for maximum power output of a hypothetical biofuel cell with a planar cathode and a reversible hydrogen anode. For laccase of T. versicolor (E(e)(0) = 0.82), the optimum mediator potential is 0.66 V (SHE), and a molecular structure is presented to achieve this result.     

Rapid and efficient proteolysis through laser-assisted immobilized enzyme reactors

In this report, laser radiation (808nm) for the first time was employed to enhance the efficiency of proteolysis through immobilized enzyme reactor (IMER). IMER based monolithic support was prepared in the fused-silica capillary via a simple two-step procedure including acryloylation on trypsin surface and in situ aqueous polymerization/immobilization. The feasibility and high efficiency of the laser-assisted IMER were demonstrated by the digestion of bovine serum albumin (BSA), cytochrome c (Cyt-c) and β-casein. The digestion process was achieved in 60s. The peptides were identified by MALDI-TOF-MS, yielding the sequence coverage of 33% for BSA, 73% for Cyt-c and 22% for β-casein. The comparisons between the in-solution digestion and on IMER reaction with/without laser assistance were made. To further confirm its efficiency in proteome analysis, the laser-assisted IMER was also applied to the analysis of one fraction of human serum sample through two-dimensional (2-D) separation of strong anion exchange/reversed-phase liquid chromatography (SAX/RPLC). After a database search, 49 unique peptides corresponding to 5 proteins were identified. The results showed that the laser-assisted IMER provides a promising platform for the high-throughput protein identification.     

Comparison of immobilized enzyme reactors for flow-injection systems

Straight, coiled, beaded, and packed-bed reactors containing immobilized glucose oxidase or l-(+)-lactate dehydrogenase were compared in terms of reaction rate, sensitivity, sample throughput, and sample dispersion. The enzymes were covalently attached to the inside walls of 5.0-cm long, 1.12-mm i.d. nylon tubes, and the resulting reactors were tested in a flow-injection system. The beaded enzymatically-active reactors (BEARs) were filled with solid glass beads of 0.5-mm or 1.0-mm diameter. Reactors with the larger beads had 2–4 times the activity, twice the sensitivity, and better throughput than the open reactors; they also minimized the physical and chemical contributions to dispersion. Packed-bed reactors were superior in the lactate determination, but the beaded reactors were better for the determination of glucose. With BEARs containing 1.0-mm beads, glucose was determined in the range 10–800 μM with a conversion efficiency of 0.056 mol of product per mole of substrate; for lactate, the range was 8–64 μM with a conversion efficiency of 0.13 mol mol^?1.     

Screen-printed tyrosinase-containing electrodes for the biosensing of enzyme inhibitors

Disposable amperometric inhibition biosensors have been microfabricated by screen printing a tyrosinase-containing carbon ink. The decrease in the substrate (catechol) steady-state current, caused by the addition of various pesticides and herbicides, offers convenient quantitation of micromolar levels of these pollutants. Unlike esterasebased disposable strips, the tyrosinase thick-film devices can be fabricated by incorporating the enzyme within the carbon ink. and do not require a prolonged incubation step in the presence of the inhibitor. The effect of experimental variables, such as the enzyme loading or substrate concentration, is assessed. Applicability to an untreated river water sample is illustrated. Such use of single-use devices for monitoring toxins addresses the problem of irreversible enzyme inhibition, and holds great promise for on-site field analysis.     

Metal-metal oxide enzyme electrodes for the determination of urea

Enzyme electrodes for urea assay based on metal-metal oxide (Sb, Bi, W, Ti + RuO₂) with urease immobilized in gelatin gel were examined. It was shown that the best electrodes were obtained for tungsten. The urea response of the electrodes was influenced by the pH and concentration of the buffer used. Increasing additions of inert salt (potassium chloride) change the pH characteristic of the tungsten electrode and buffer capacity, thus influencing the urea response of the electrode.     

Conducting polymer based amperometric enzyme electrodes

The construction and the properties of conducting-polymer based amperometric enzyme electrodes are reviewed. The main aim is to focus on the properties of conducting polymer films which are important for the construction of amperometric enzyme electrodes. Additionally, the review is focused on electron-transfer pathways between conducting-polymer integrated immobilized enzyme molecules and the modified electrode using free-diffusing redox mediators as well as direct electron transfer via the conducting-polymer wires. Possible future applications using microstructured conducting-polymer films will be discussed.     

Amperometric enzyme electrodes in analytical chemistry

Summary An overview is given of works on the construction and application of amperometric enzyme electrodes for the determination of metabolites in biological solutions. The following electrodes are dealt with: monoenzyme and polyenzyme electrodes involving amperometric detection of hydrogen peroxide, bienzyme electrodes with oxidase-peroxidase, electrodes based on organic metals and chemically modified electrodes, dehydrogenase electrodes, amperometric hydrolase electrodes and highly sensitive electrodes involving chemical amplification. Biocatalytic stripping and macrokinetic behaviour of the electrodes are discussed.

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Amperometrische Enzymelektroden in der analytischen Chemie

     

Performance of fixed and fluidized bed reactors with immobilized enzyme

Applied Biochemistry and Biotechnology - Saccharification of α-amylase liquefied cassava starch was carried out at pH 4.5 and 45?C, in both fixed and fluidized bed reactors, using...     

Silicone-grease-based immobilisation method for the preparation of enzyme electrodes

An approach to the construction of amperometric biosensors based on the incorporation of an enzyme in silicone grease and using the grease to fill micropores on a graphite surface is described. The enzyme-grease electrode concept, illustrated with the enzyme tyrosinase, offers a very simple, rapid and inexpensive approach to the fabrication of enzyme electrodes. The tyrosinase electrode responds very rapidly to dynamic changes in the concentration of phenolic compounds. A response time (t95%) as low as 5 s has been determined. With flow injection, 120 samples per hour can be processed with a relative standard deviation of 2.4%. The electrode remains active for about 12 d. The detection limit for dopamine is 6 x 10(-6) M. This method of biosensor construction should be applicable to other enzyme-substrate systems.