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A methodology for preparing nanostructured biomolecular interfaces with high enzymatic activity

机译:的方法制备纳米生物分子与高酶接口活动

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摘要

The development of a novel method for functionalizing nanopatterned surfaces with catalytically active proteins is reported. This method involves using dip-pen nanolithography (DPN) and polymer pen lithography (PPL) to generate nanoscale patterns of coenzyme A, followed by a phosphopantetheinyl transferase-mediated coupling between coenzyme A and proteins fused to the ybbR-tag. By exploiting the ability to generate protein features over large areas afforded by DPN and PPL, it was now possible to measure protein activity directly on these surfaces. It was found that proteins immobilized on the nanoscale features not only display higher activity per area with decreasing feature size, but are also robust and can be used for repeated catalytic cycles. The immobilization method is applicable to a variety of proteins and gives rise to superior activity compared to proteins attached in random orientations on the surface.
机译:一个新颖的方法的发展构建nanopatterned表面报告蛋白催化地活跃。方法涉及使用蘸水笔纳米(DPN)和聚合物笔光刻(PPL)生成纳米辅酶A的模式,随后phosphopantetheinyltransferase-mediated辅酶A之间的耦合和蛋白质ybbR-tag融合。生成蛋白质的能力特征提供大面积DPN PPL,这是现在可以直接测量蛋白质活性这些表面。不仅固定在纳米特性显示更高的活动单位面积减少功能尺寸,但也可以使用健壮和对重复催化循环。适用于各种蛋白质和方法相比产生优越的活动蛋白质附着在随机取向表面。

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