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将漆酶固定在接枝聚合物的聚四氟乙烯膜上用于生物传感器的构建。

Immobilization of laccase on polymer grafted polytetrafluoroethylene membranes for biosensor construction.

机构信息

Istanbul Technical University, Molecular Biology-Genetics and Biotechnology Program, MOBGAM, 34469 Maslak, Istanbul, Turkey.

出版信息

Talanta. 2011 Apr 15;84(2):524-30. doi: 10.1016/j.talanta.2011.01.031. Epub 2011 Jan 22.

Abstract

In this study, Trametes versicolor laccase was immobilized on polytetrafluoroethylene (PTFE) membranes using two different techniques, entrapment to gelatin and covalent immobilization to the surface. For surface immobilization, functional groups were formed on PTFE surface by radiofrequency (RF) plasma treatment followed by polymer grafting. Two different polymers, polyacrylamide (pAAm) and polyacrylic acid (pAAc) were tried. For polyacrylamide grafted PTFE, a two-step polymerization process was used. The membranes were first treated with hydrogen plasma and pAAm grafted PTFE (pAAm-g-PTFE) was then formed by argon plasma treatment. To produce pAAc grafted PTFE (pAAc-g-PTFE), the surface was first treated with argon plasma and AAc was then attached to the surface by heat treatment (70°C, 6h). For both cases, an optimized carbodiimide coupling reaction was used for laccase immobilization. Enzyme activity was measured by an oxygen electrode using guaiacol as substrate. All three biosensing membranes were characterized and compared in terms of optimum working conditions, storage stability and reusability. Our study concluded that although a higher activity was obtained by gelatin entrapped laccase, its mechanical instability and poor storage life makes the gelatin biosensor unattractive for multiple usages and for field measurements. pAAc-g-PTFE biosensor was found to be more stable and highly reusable (ca. 50 times) when compared with the other two biosensors. In addition, its sensitivity was suitable for field applications. Therefore, the pAAc-g-PTFE biosensor could be proposed as an alternative on-site detection tool for phenolic compound monitoring.

摘要

在这项研究中,使用两种不同的技术将彩绒革盖菌漆酶固定在聚四氟乙烯(PTFE)膜上,分别为明胶包埋和共价固定到表面。对于表面固定,通过射频(RF)等离子体处理在 PTFE 表面形成官能团,然后进行聚合物接枝。尝试了两种不同的聚合物,聚丙烯酰胺(pAAm)和聚丙烯酸(pAAc)。对于接枝到 PTFE 的聚丙烯酰胺,使用两步聚合过程。首先用氢气等离子体处理,然后用氩气等离子体处理形成接枝到 PTFE 的聚丙烯酰胺(pAAm-g-PTFE)。为了生成接枝到 PTFE 的聚丙烯酸(pAAc-g-PTFE),首先用氩气等离子体处理表面,然后通过热处理(70°C,6h)将 AAc 附着到表面。对于两种情况,都使用优化的碳二亚胺偶联反应进行漆酶固定。通过使用愈创木酚作为底物的氧电极测量酶活性。根据最佳工作条件、储存稳定性和可重复使用性对所有三种生物传感膜进行了表征和比较。我们的研究得出结论,尽管明胶包埋漆酶获得了更高的活性,但由于其机械不稳定性和较差的储存寿命,明胶生物传感器不适合多次使用和现场测量。与其他两种生物传感器相比,pAAc-g-PTFE 生物传感器更稳定且可高度重复使用(约 50 次)。此外,其灵敏度适合现场应用。因此,pAAc-g-PTFE 生物传感器可以作为酚类化合物监测的现场检测工具的替代方案。

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