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Surface Functionalization by Stimuli-Sensitive Microgels for Effective Enzyme Uptake and Rational Design of Biosensor Setups

机译:表面功能化的刺激敏感的微凝胶有效吸收酶和生物传感器设置的合理设计。

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摘要

We highlight microgel/enzyme thin films that were deposited onto solid interfaces via two sequential steps, the adsorption of temperature- and pH-sensitive microgels, followed by their complexation with the enzyme choline oxidase, ChO. Two kinds of functional (ionic) microgels were compared in this work in regard to their adsorptive behavior and interaction with ChO, that is, poly(N-isopropylacrylamide-co-N-(3-aminopropyl)methacrylamide), P(NIPAM-co-APMA), bearing primary amino groups, and poly(N-isopropylacrylamide-co-N-[3-(dimethylamino) propyl]methacrylamide), P(NIPAM-co-DMAPMA), bearing tertiary amino groups. The stimuli-sensitive properties of the microgels in the solution were characterized by potentiometric titration, dynamic light scattering (DLS), and laser microelectrophoresis. The peculiarities of the adsorptive behavior of both the microgels and the specific character of their interaction with ChO were revealed by a combination of surface characterization techniques. The surface charge was characterized by electrokinetic analysis (EKA) for the initial graphite surface and the same one after the subsequent deposition of the microgels and the enzyme under different adsorption regimes. The masses of wet microgel and microgel/enzyme films were determined by quartz crystal microbalance with dissipation monitoring (QCM-D) upon the subsequent deposition of the components under the same adsorption conditions, on a surface of gold-coated quartz crystals. Finally, the enzymatic responses of the microgel/enzyme films deposited on graphite electrodes to choline were tested amperometrically. The presence of functional primary amino groups in the P(NIPAM-co-APMA) microgel enables a covalent enzyme-to-microgel coupling via glutar aldehyde cross-linking, thereby resulting in a considerable improvement of the biosensor operational stability.
机译:我们重点介绍了通过两个连续步骤沉积在固体界面上的微凝胶/酶薄膜,即对温度和pH敏感的微凝胶的吸附,然后与酶胆碱氧化酶ChO络合。在这项工作中,比较了两种功能性(离子)微凝胶的吸附行为和与ChO的相互作用,即聚(N-异丙基丙烯酰胺-co-N-(3-氨基丙基)甲基丙烯酰胺),P(NIPAM-co -APMA),带有伯氨基,和聚(N-异丙基丙烯酰胺-co-N- [3-(二甲基氨基)丙基]甲基丙烯酰胺),P(NIPAM-co-DMAPMA),带有叔氨基。通过电位滴定,动态光散射(DLS)和激光微电泳对溶液中微凝胶的刺激敏感特性进行了表征。通过结合表面表征技术,揭示了两种微凝胶的吸附行为的特殊性以及它们与ChO相互作用的特定特征。通过电动分析(EKA)对初始石墨表面和随后在不同吸附方式下沉积微凝胶和酶后的表面进行表征。湿微凝胶和微凝胶/酶膜的质量是由石英晶体微天平通过耗散监测(QCM-D)确定的,随后在相同的吸附条件下将组分沉积在镀金石英晶体的表面上。最后,通过安培法测试沉积在石墨电极上的微凝胶/酶膜对胆碱的酶促反应。 P(NIPAM-co-APMA)微凝胶中功能性伯氨基的存在能够通过戊二醛交联实现共价酶与微凝胶的偶联,从而大大改善了生物传感器的操作稳定性。

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