The electrochemical study of oxidation-reduction properties of horseradish peroxidase

Oxidation-reduction properties of horseradish peroxidase (HRP) have been investigated by using direct electrochemical methods. Two successive separated distinct one-electron processes of HRP were obtained and the related physiological processes were described. The monolayer coverage of HRP at the electrode surface is about 50 pmol/cm(2). UV-Vis spectrophotometry and stable amperometry prove that the enzyme electrode possesses catalytic activity for H2O2 in the absence of a mediator and it might offer an opportunity to build the third generation of biosensors for analytes, such as H2O2, glucose and cholesterol etc. (C) 1997 Elsevier Science S.A.

毛竹茎木质化过程的组织细胞学研究

应用光学显微镜和透射电子显微镜，并结合组织化学和细胞化学方法，研究了毛竹（Phyllostachys pubescens Mazel）茎各组织中细胞壁的木质化过程、木质素异质性、酚酸类成分的分布、木质素在细胞壁中的沉积方式以及过氧化物酶的组织、细胞化学定位等。 研究结果表明：毛竹茎的原生木质部导管在维管束发育早期就已木质化;后生木质部导管和纤维细胞在维管束分化完成后，自胞间层和细胞角隅处开始木质化;基本薄壁组织细胞木质化的发生较晚，通常在茎的节间完成伸长生长后才开始，但也有少数薄壁组织细胞始终保持非木质化的薄壁状态。根据可见光显微分光光度的分析结果，纤维细胞壁在木质化的早期，主要形成愈创木基木质素（guaiacyl lignin）, 随着木质化过程的发展，紫丁得基木质素（syringyl lignin）含量不断增加，最后成为纤维细胞壁木质素的主要组成成分。导管分子的木质素主要成分为愈创木基木质素，基本薄壁组织细胞壁为愈创木基与紫丁香基两种。 毛竹茎各组织在紫外光激发下自发荧光的荧光显微分光光度分析表明，氨水处理可以有效地识别阿魏酸的分布，如在竹笋各种幼嫩组织中均分布有阿魏酸;而用过氧化氢／冰醋酸混合液处理，则可以区分木素与结合于半纤维素中的阿魏酸和对－香豆酸，随着毛竹茎的生长和细胞壁木质化的增加，阿魏酸的含量下降。 通过对毛竹茎纤维细胞壁木质化过程中超微结构的观察表明，高尔基体、高尔基小泡、内质网、壁旁体细胞器在木质素前体的形成和运输等方面均起着重要作用，而周质微管在细胞壁木质化过程中的具体作用方式尚不明确。木质素在细胞壁中的沉积方式分别为：胞间层的木质素呈分散的颗粒状沉积方式，导管次生壁的木质素为片层状沉积方式，而在纤维细胞次生壁Sl层中，木质素为团块状的沉积方式。木质素沉积方式与纤维素微纤丝的排列有密切关系。 在毛竹茎各组织的细胞壁尚未木质化之前，过氧化物酶仅分布于细胞角隅处，随着细胞次生壁的增厚和木质化的增强，过氧化物酶可大量出现在次生壁中;在纤维细胞次生壁中，木质素含量较高的St各层，过氧化物酶活性也较强，而木质素含量较低的Sl各层，过氧化物酶活性则较弱。由此表明，过氧化物酶直接参与了细胞壁木质素的合成。另外，在茎的部分基本薄壁组织细胞和韧皮部等未木质化的细胞壁中，过氧化物酶也同样表现出较强的活性，这说明在茎的不同组织中分布的这种酶，可能是几种不同功能的同工酶形式。

Effects of microcystins on the growth and the activity of superoxide dismutase and peroxidase of rape (Brassica napus L.) and rice (Oryza sativa L.)

Microcystins are naturally occurring hepatotoxic cyclic heptapeptides produced by some toxic freshwater cyanobacterial species. In this study, crude extract of toxic cyanobacterial blooms from Dianchi Lake in southwestern China was used to determine the effects of microcystins on rape (Brassica napus L.) and rice (Oryza sativa L.). Experiments were carried out on a range of doses of the extract (equivalent to 0, 0.024, 0.12, 0.6 and 3 mug MC-LR/ml). Investigations showed that exposure to microcystins inhibited the growth and development of both rice and rape seedlings, however, microcystins had more powerful inhibition effect on rape than rice in germination percentage of seeds and seedling height. Microcystins significantly inhibited the elongation of primary roots of rape and rice seedlings. Determination of the activities of peroxidase and superoxide dismutase demonstrated that microcystin stress was manifested as an oxidative stress. Using ELISA, microcystins were examined from the extract of exposed rape and rice seedlings, indicating that consumption of edible plants exposed to microcystins via irrigation route may have health risks. Significantly different levels of recovered microcystins between exposed rice and rape seedlings Suggested that there might be different tolerant mechanisms toward microcystins. (C) 2004 Elsevier Ltd. All rights reserved.

Determination of some reactive oxygen species scavengers based on the peroxidase-oxidase oscillator

This paper reports a new method for detection of ROS scavengers including superoxide dismutase, ascorbic acid and glutathione based on a 'probe' of peroxidase-oxidase biochemical oscillator. The oscillation period and amplitude change with different concentrations of scavengers. The linear ranges of superoxide dismutase, ascorbic acid and glutathione are respectively 1.56 x 10(-4)-1.56 x 10(-3) mg mL(-1), 1.75 x 10(-7) -1.75 x 10(-5) mol L-1 and 9.38 x 10(-7) -7.5 x 10(-5) mol L-1. The selectivity, linearity and precision for superoxide dismutase, ascorbic acid, and glutathione are presented and discussed. The results compared well with other standard methods for determination of superoxide dismutase, ascorbic acid and glutathione. Some possible steps in the overall reaction mechanisms are discussed.

Hydrogen peroxide biosensor based on horseradish peroxidase-Au nanoparticles at viologen grafted glassy carbon electrode

A novel hydrogen peroxide biosensor was fabricated that is based on horseradish peroxidase-Au nanoparticles immobilized on a viologen-modified glassy carbon electrode (GCE) by amino cation radical oxidation in basic solution. The immobilized BAPV acts as a mediator and a covalent linker between GCE and the Au nanoparticles. The biosensor exhibited fast response, good reproducibility, and long-term stability.

Fe3O4 magnetic nanoparticles as peroxidase mimetics and their applications in H2O2 and glucose detection

Artificial enzyme mimetics are a current research interest because natural enzymes bear some serious disadvantages, such as their catalytic activity can be easily inhibited and they can be digested by proteases. A very recently study reported by Yan et al. has proven that Fe3O4 magnetic nanoparticles (MNPs) exhibit an intrinsic enzyme mimetic activity similar to that found in natural peroxidases, though MNPs are usually thought to be biological and chemical inert (Gao, L. Z.; Zhuang, J.; Nie, L.; Zhang, J. B.; Zhang, Y.; Gu, N.; Wang, T. H.; Feng, J.; Yang, D. L.; Perrett, S.; Yan, X. Y. Nat. Nanotechnol. 2007, 2, 577-583).

Selective, peroxidase substrate based "signal-on" colorimetric assay for the detection of chromium (VI)

Due to the potentially adverse effects of the chromium (VI) on the human health and also on the environment, the quantitative determination of Cr(VI) is of particular interest. This work herein reports a facile, selective and rapid colorimetric determination of Cr(VI) based on the peroxidase substrate-2,2'-azino-bis(3-ethylbenzo-thiazoline-6-sulfonic acid) diammonium salt (ABTS) as the color developing agent. ABTS, which was usually acted as peroxidase substrate for the enzyme linked immunosorbent assay, is used here for the first time to fabricate the "signal-on" colorimetric Assay for Cr(VI).

Direct electrochemistry of horseradish peroxidase immobilized in calcium carbonate microsphere doped with phospholipids

Protein electrochemistry affords a direct method to study the biological electron transfer processes. However, supplying a biocompatible environment to maintain the native state of protein is all-important and challengeable. Here, we chose vaterite, one of the crystalline polymorphs of calcium carbonate, with highly porous nature and large specific surface area, which was doped with phospholipids, as the matrix to immobilize horseradish peroxidase (HRP). The integrity of HRP was kept during the simple immobilization procedure. By virtue of this organic/inorganic complex matrix, the direct electrochemistry of HRP was realized, and the activity of HRP for catalyzing reduction of O-2 and H2O2 was preserved.

Direct electron transfer of horseradish peroxidase and its electrocatalysis based on carbon nanotube/thionine/gold composites

Horseradish peroxidase (HRP) was incorporated into multiwalled carbon nanotube/thionine/Au (MTAu) composite film by electrostatic interactions between positively charged HRP and negatively charged MTAu composite. The results of electrochemical impedance spectroscopy (EIS) confirmed adsorption of HRP on the surface of MTAu modified GC electrode.

Hydrogen peroxide biosensor based on direct electrochemistry of soybean Peroxidase immobilized on single-walled carbon nanohorn modified electrode

Single-walled carbon nanohorns (SWCNHs) were used as a novel and biocompatible matrix for fabricating biosensing devices. The direct immobilization of acid-stable and thermostable soybean peroxidase (SBP) on SWCNH modified electrode surface can realize the direct electrochemistry of enzyme. Cyclic voltammogram of the adsorbed SBP displays a pair of redox peaks with a formal potential of -0.24V in pH 5 phosphate buffer solution.