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Meso-Cellular Silicate Foam-Modified Reduced Graphene Oxide with a Sandwich Structure for Enzymatic Immobilization and Bioelectrocatalysis

机译:中间细胞硅酸盐泡沫改性的石墨烯氧化物,具有夹心结构,用于酶活化和生物电池分析

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An integrated composite of meso-cellular silicate foam (MCF)-modified reduced graphene oxide (MCF@rGO) was designed and synthesized based on polyethylene oxide-polypropylene oxide-polyethylene oxide (P123)-modified rGO (P123-rGO). As the polymeric template for the fabrication of mesoporous silicates, modified P123 greatly improved the affinity between the nanosheet and the in situ formed MCFs, resulting in the formation of thin layers of MCFs on both sides of rGO. Therefore, the MCFs@rGO formed exhibited a unique sandwich structure with an inner skeleton of rGO and two outer layers of MCFs. The outer modification by MCFs, with the presence of large mesopores, not only shifted the surface property of rGO from hydrophobic to hydrophilic but also offered immobilized enzymes a favorable microenvironment to maintain their bioactivity. Meanwhile, the inner skeleton of rGO compensated for the weak conductivity of MCFs, providing a pathway for the direct electron transfer (DET) of various redox enzymes or proteins, such as hemoglobin (Hb), horseradish peroxidase, glucose oxidase (GOD), and cholesterol oxidase. It was found that the DET signal obtained from Hb-MCFs@rGO/glassy carbon electrode (GCE) was much larger than the sum of the signals from two components-based modified electrodes of Hb-P123-rGO/GCE and Hb-MCFs/GCE. A similar improvement in DET signal was also observed using GOD-MCFs@rGO/GCE. The significant enhancement of DET signals for both protein electrodes can be ascribed to the synergistic effects generated from the integration of the two components, one of which enhances biocompatibility and the other enhances conductivity. The bioelectrocatalytic performance of Hb and GOD electrodes was further investigated. As for Hb-MCFs@rGO/GCE, the GOD electrode displayed excellent analytical performance for the detection of hydrogen peroxide (H2O2), including a good sensitivity of 0.25 mu A mu mol(-1) L cm(-2), a low detection limit of 63.6 nmol L-1 based on S/N = 3, and a low apparent Michaelis-Menten constant (K-M(app)) of 49.05 mu mol L-1. GOD-MCFs@rGO/GCE also exhibited good analytical performance for the detection of glucose, with a wide linear range of 0.25-8.0 mmol L-1. In addition, blood glucose detection in samples of human serum was successfully achieved using GOD-MCFs@rGO/GCE with a low quantification limit.
机译:基于聚环氧丙烷 - 聚丙烯氧化物 - 聚环氧乙烷(P123-RGO)设计并合成了中间细胞硅酸盐泡沫(MCF)硅酸盐泡沫(MCF)制备的石墨烯(MCF @ RGO)的整合复合物。作为制备介孔硅酸盐的聚合物模板,改性P123大大提高了纳米片和原位形成的MCF之间的亲和力,导致RGO两侧形成薄层MCF。因此,形成的MCFS @ Rgo展示了独特的夹心结构,其具有RGO的内骨架和两个外层的MCF。通过MCF的外部改性,具有大的中孔,不仅使RGO的表面特性从疏水移入亲水性,而且还提供了固定化的酶是一种良好的微环境,以保持其生物活性。同时,RGO的内骨架补偿了MCF的弱电导率,为各种氧化还原酶或蛋白质的直接电子转移(DET)提供了一种途径,例如血红蛋白(HB),辣根过氧化物酶,葡萄糖氧化酶(上帝)和胆固醇氧化酶。结果发现,从HB-MCFS @ rgo /玻璃电极(GCE)获得的DED信号远大于来自HB-P123-RGO / GCE和HB-MCF的两个组分的修改电极的信号之和/ GCE。使用GOD-MCFS @ RGO / GCE也观察到DED信号的类似改进。对于两个蛋白质电极的DEC信号的显着增强可以归因于从两种组分的整合产生的协同效果,其中一个是增强了生物相容性,另一个增强了导电性。进一步研究了Hb和神电极的生物电催化性能。至于HB-MCFS @ Rgo / GCE,神电极显示出优异的分析性能,用于检测过氧化氢(H2O2),包括0.25μmmol(-1)L cm(-2)的良好敏感性,低于基于S / N = 3的检出限为63.6nmol L-1,以及49.05μmol1-1的低表观迈克莱斯 - MENTEN常数(KM(APP))。 GoD-MCFS @ RGO / GCE还表现出良好的分析性能,用于检测葡萄糖,线性范围为0.25-8.0mmol L-1。此外,使用GOD-MCFS @ RGO / GCE具有低定量限制,成功实现了人血清样本中的血糖检测。

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