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In Situ Modification of a Semiconductor Surface by an Enzymatic Process: A General Strategy for Photoelectrochemical Bioanalysis

机译:通过酶法原位修饰半导体表面:光电化学生物分析的一般策略

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摘要

Usually, the photoelectrochemical (PEC) bioanalysis necessitates ready photoactive materials as signal sources to convert the specific biological events into electrical signals. Herein, the first PEC bioanalysis without the necessity of ready visible-light-active species was demonstrated. We use an enzyme catalytic process to couple with the unique surface chemistry of semiconductive nanocrystalline, whereby its electronic properties could be modified spontaneously during the enzymatic reaction. Specifically, the enzymatic hydrolysis of ascorbic acid 2-phosphate by alkaline phosphatase is allowed to interact on the TiO_2 nanoparticles (NPs) matrix. PEC tests reveal that the self-coordination of the biocatalyzed enediol-ligands onto the undercoordinated surface defect sites would in situ form a ligand-to-metal charge transfer (CT) complex, endowing the inert semiconductor with strong absorption bands in the visible region, and hence underlying a novel and general PEC bioanalysis strategy.
机译:通常,光电化学(PEC)生物分析需要使用现成的光敏材料作为信号源,以将特定的生物事件转换为电信号。在此,首次PEC生物分析得到证明,无需准备可见光活性物质。我们使用酶催化过程结合半导体纳米晶体的独特表面化学,从而可以在酶促反应过程中自发地改变其电子性能。具体而言,使碱性磷酸酶对2-磷酸抗坏血酸进行酶促水解,使其在TiO_2纳米颗粒(NPs)基质上相互作用。 PEC测试表明,生物催化的烯二醇配体在配位不足的表面缺陷位点上的自配位会原位形成配体到金属的电荷转移(CT)络合物,使惰性半导体在可见光区域具有强吸收带,因此,这是一种新颖而通用的PEC生物分析策略。

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