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二维毛细管-井筛中 DNA 和蛋白质的连续流动电泳。

Continuous-Flow Electrophoresis of DNA and Proteins in a Two-Dimensional Capillary-Well Sieve.

机构信息

Department of Electronic and Computer Engineering, and ‡Division of Biomedical Engineering, The Hong Kong University of Science and Technology , Clear Water Bay, Hong Kong SAR, China.

出版信息

Anal Chem. 2017 Sep 19;89(18):10022-10028. doi: 10.1021/acs.analchem.7b02484. Epub 2017 Aug 29.

Abstract

Continuous-flow electrophoresis of macromolecules is demonstrated using an integrated capillary-well sieve arranged into a two-dimensional anisotropic array on silicon. The periodic array features thousands of entropic barriers, each resulting from an abrupt interface between a 2 μm deep well (channel) and a 70 nm capillary. These entropic barriers owing to two-dimensional confinement within the capillaries are vastly steep in relation to those arising from slits featuring one-dimensional confinement. Thus, the sieving mechanisms can sustain relatively large electric field strengths over a relatively small array area. The sieve rapidly sorts anionic macromolecules, including DNA chains and proteins in native or denatured states, into distinct trajectories according to size or charge under electric field vectors orthogonally applied. The baseline separation is achieved in less than 1 min within a horizontal migration length of ∼1.5 mm. The capillaries are self-enclosed conduits in cylindrical profile featuring a uniform diameter and realized through an approach that avoids advanced patterning techniques. The approach exploits a thermal reflow of a layer of doped glass for shape transformation into cylindrical capillaries and for controllably shrinking the capillary diameter. Lastly, atomic layer deposition of alumina is introduced for the first time to fine-tune the capillary diameter as well as to neutralize the surface charge, thereby suppressing undesired electroosmotic flows.

摘要

基于硅基二维各向异性毛细-井筛阵列,展示了用于大分子的连续流动电泳。该周期性阵列具有数千个熵屏障,每个熵屏障均由 2μm 深的井(通道)与 70nm 毛细之间的突然界面产生。由于毛细内的二维限制,这些熵屏障相对于具有一维限制的狭缝产生的熵屏障陡峭得多。因此,筛网机制可以在相对较小的阵列区域上维持相对较大的电场强度。在正交施加的电场矢量下,筛网根据大小或电荷将带负电荷的大分子(包括天然或变性状态的 DNA 链和蛋白质)快速分类成不同的轨迹。在水平迁移长度约 1.5mm 内,不到 1 分钟即可实现基线分离。毛细是自封闭的圆柱形通道,具有均匀的直径,采用避免先进图案化技术的方法实现。该方法利用掺杂玻璃的热回流将形状转化为圆柱形毛细,并可控制地缩小毛细直径。最后,首次引入氧化铝原子层沉积来微调毛细直径并中和表面电荷,从而抑制不需要的电渗流。

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