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Enzymatic activity of individual bioelectrocatalytic viral nanoparticles: dependence of catalysis on the viral scaffold and its length

机译:酶活性的个人bioelectrocatalytic病毒纳米颗粒:依赖的病毒脚手架和催化作用它的长度

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摘要

The enzymatic activity of tobacco mosaic virus (TMV) nanorod particles decorated with an integrated electro-catalytic system, comprising the quinoprotein glucose-dehydrogenase (PQQ-GDH) enzyme and ferrocenylated PEG chains as redox mediators, is probed at the individual virion scale by atomic force microscopy-scanning electrochemical atomic force microscopy (AFM-SECM). A marked dependence of the catalytic activity on the particle length is observed. This finding can be explained by electron propagation along the viral backbone, resulting from electron exchange between ferrocene moieties, coupled with enzymatic catalysis. Thus, the use of a simple 1D diffusion/reaction model allows the determination of the kinetic parameters of the virus-supported enzyme. Comparative analysis of the catalytic behavior of the Fc-PEG/PQQ-GDH system assembled on two differing viral scaffolds, TMV (this work) and bacteriophage-fd (previous work), reveals two distinct kinetic effects of scaffolding: An enhancement of catalysis that does not depend on the virus type and a modulation of substrate inhibition that depends on the virus type. AFM-SECM detection of the enzymatic activity of a few tens of PQQ-GDH molecules, decorating a 40 nm-long viral domain, is also demonstrated, a record in terms of the lowest number of enzyme molecules interrogated by an electrochemical imaging technique.
机译:烟草花叶病毒的酶活性(TMV)奈米棒颗粒装饰着一个综合electro-catalytic系统组成的quinoprotein葡糖脱氢酶(PQQ-GDH)氧化还原酶和ferrocenylated PEG链介质,在单个病毒粒子探测通过原子力microscopy-scanning规模电化学原子力显微镜(AFM-SECM)。活动粒子长度是观察。发现可以解释为电子传播沿着病毒骨干,造成电子交流二茂铁根,加上酶催化。扩散/反应模型允许的决心virus-supported的动力学参数酶。Fc-PEG / PQQ-GDH系统组装的行为在两个不同的病毒支架,烟草花叶病毒(这项工作)和bacteriophage-fd(以前的工作),揭示了两个不同的动力学影响脚手架:一个增强的催化作用不依赖于衬底的病毒类型和调制这取决于病毒抑制类型。AFM-SECM检测的酶活性几十PQQ-GDH分子,装修40nm长病毒领域,也证明,记录的最低数量的酶由电化学分子审问成像技术。

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