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玻璃上反应性烷氧基硅烷的蘸笔纳米光刻技术。

Dip-pen nanolithography of reactive alkoxysilanes on glass.

作者信息

Jung Hyungil, Kulkarni Rajan, Collier C Patrick

机构信息

Division of Chemistry and Chemical Engineering, California Institute of Technology, Pasadena, California 91125, USA.

出版信息

J Am Chem Soc. 2003 Oct 8;125(40):12096-7. doi: 10.1021/ja0363720.

Abstract

The use of organofunctional silane chemistry is a flexible and general method for immobilizing biomolecules on silicon oxide surfaces, including fabricating DNA, small-molecule, and protein microarrays. The biggest hurdle in employing dip-pen nanolithography (DPN) for extending this general approach to the nanoscopic domain is the tendency of trialkoxy- and trichlorosilanes to rapidly polymerize due to hydrolysis reactions. The control of the local water concentration between the substrate surface and the scanning AFM tip is critical, both to the physical and chemical processes involved in DPN writing and to the ability to form well-defined thin layers of reactive silanes without extensive polymerization induced disorder. We found that we could control the degree of polymerization through careful choice of the alkoxysilane used as the "ink" for DPN and through control of the relative humidity during inking and writing with the coated AFM tip. As a proof-of-principle, we demonstrate that areas patterned with an alkoxysilane on glass with DPN are functional for subsequent immobilization of fluorescently labeled streptavidin via covalent attachment of biotin. This preliminary result sets the stage for the ability to capture proteins in their fully hydrated state from buffered solution, by molecular recognition onto previously written reactive nanoscopic regions on oxidized silicon and glass.

摘要

利用有机官能硅烷化学是一种灵活通用的方法,可将生物分子固定在氧化硅表面,包括制造DNA、小分子和蛋白质微阵列。将蘸笔纳米光刻(DPN)用于将这种通用方法扩展到纳米领域的最大障碍是三烷氧基硅烷和三氯硅烷由于水解反应而迅速聚合的趋势。控制基底表面与扫描原子力显微镜(AFM)尖端之间的局部水浓度,对于DPN写入所涉及的物理和化学过程以及形成定义明确的反应性硅烷薄层而不产生广泛聚合诱导无序的能力至关重要。我们发现,可以通过仔细选择用作DPN“墨水”的烷氧基硅烷以及在使用涂覆AFM尖端进行上墨和写入过程中控制相对湿度来控制聚合程度。作为原理验证,我们证明了用DPN在玻璃上用烷氧基硅烷图案化的区域可通过生物素的共价连接用于随后固定荧光标记的链霉亲和素。这一初步结果为通过分子识别将处于完全水合状态的蛋白质从缓冲溶液中捕获到氧化硅和玻璃上先前写入的反应性纳米区域奠定了基础。

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