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Electrochemical behavior of ascorbate oxidase immobilized on graphite electrode modified with Au-nanoparticles

机译:纳米金修饰的石墨电极上固定的抗坏血酸氧化酶的电化学行为

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Direct electrochemistry of ascorbate oxidase was observed when immobilized on graphite modified with nano-sized gold structures. Au-structures were electrodeposited onto the graphite surface by means of cyclic voltammetry, then the enzyme was chemisorbed onto their surface. The electron transfer between the enzyme active center and the modified electrode surface was probed by square wave voltammetry (SWV) and cyclic voltammetry (CV). The dependence of the current maxima on the scan rate was found linear, suggesting that the redox process is controlled by surface chemistry. Bioelectrocatalytic oxidation of the enzyme substrate L-ascorbic acid was explored by constant potential amperometry over the potential range from 200 to 350 mV (vs. Ag/AgCl, 3 M KCl) at the pHs 5.6 and 7.0. At a potential as low as 200 mV, pH 7.0 and temperature 25 C following operational parameters were determined for the enzyme electrode: a sensitivity: 1.54μAmM~(-1) mm~2 (r~2 - 0.99s), linear dynamic range up to 3.3 mM, detection limit of 1.5μM, response time up to 20 s.
机译:当固定在用纳米金结构改性的石墨上时,观察到抗坏血酸氧化酶的直接电化学。通过循环伏安法将金结构电沉积在石墨表面上,然后将酶化学吸附在其表面上。通过方波伏安法(SWV)和循环伏安法(CV)探测酶活性中心和修饰电极表面之间的电子转移。发现电流最大值对扫描速率的依赖性是线性的,这表明氧化还原过程受表面化学作用的控制。通过恒定电位安培法在pH值5.6和7.0的200至350 mV(相对于Ag / AgCl,3 M KCl)的电位范围内,探索了酶底物L-抗坏血酸的生物电催化氧化。在低至200 mV的电位,pH 7.0和25°C的温度下,确定了酶电极的以下操作参数:灵敏度:1.54μAmM〜(-1)mm〜2(r〜2-0.99s),线性动态范围最高3.3 mM,检测极限为1.5μM,响应时间最高20 s。

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