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机械化学刻蚀

Mechanochemical Lithography.

机构信息

Collaborative Innovation Center of Advanced Microstructures, National Laboratory of Solid State Microstructure, Department of Physics, Nanjing University, Nanjing 210093, China.

Wenzhou Institute, University of Chinese Academy of Sciences, Wenzhou 325001, China.

出版信息

J Am Chem Soc. 2022 Jun 8;144(22):9949-9958. doi: 10.1021/jacs.2c02883. Epub 2022 May 30.

Abstract

Surfaces with patterned biomolecules have wide applications in biochips and biomedical diagnostics. However, most patterning methods are inapplicable to physiological conditions and incapable of creating complex structures. Here, we develop a mechanochemical lithography (MCL) method based on compressive force-triggered reactions. In this method, biomolecules containing a bioaffinity ligand and a mechanoactive group are used as mechanochemical inks (MCIs). The bioaffinity ligand facilitates concentrating MCIs from surrounding solutions to a molded surface, enabling direct and continuous printing in an aqueous environment. The mechanoactive group facilitates covalent immobilization of MCIs through force-triggered reactions, thus avoiding the broadening of printed features due to the diffusion of inks. We discovered that the ubiquitously presented amino groups in biomolecules can react with maleimide through a force-triggered Michael addition. The resulting covalent linkage is mechanically and chemically stable. As a proof-of-concept, we fabricate patterned surfaces of biotin and His-tagged proteins at nanoscale spatial resolution by MCL and verify the resulting patterns by fluorescence imaging. We further demonstrated the creation of multiplex protein patterns using this technique.

摘要

具有图案化生物分子的表面在生物芯片和生物医学诊断中有广泛的应用。然而,大多数图案化方法不适用于生理条件,并且无法创建复杂结构。在这里,我们开发了一种基于压缩力触发反应的机械化学光刻(MCL)方法。在这种方法中,含有生物亲和配体和机械活性基团的生物分子被用作机械化学墨水(MCIs)。生物亲和配体有助于将 MCIs 从周围溶液集中到成型表面,从而能够在水相环境中直接和连续打印。机械活性基团通过力触发反应促进 MCIs 的共价固定,从而避免由于墨水的扩散导致打印特征变宽。我们发现生物分子中普遍存在的氨基可以通过力触发迈克尔加成与马来酰亚胺反应。由此产生的共价键在机械和化学上都是稳定的。作为概念验证,我们通过 MCL 在纳米级空间分辨率下制造了生物素和 His 标记蛋白的图案化表面,并通过荧光成像验证了所得图案。我们还进一步展示了使用该技术创建多蛋白图案的能力。

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