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生物界面连接化学对用于蛋白质检测的硅纳米线灵敏度的影响。

Effect of biointerfacing linker chemistries on the sensitivity of silicon nanowires for protein detection.

作者信息

Dorvel Brian, Reddy Bobby, Bashir Rashid

机构信息

Center for Biophysics and Computational Biology, University of Illinois at Urbana-Champaign , Urbana, Illinois 61801, United States.

出版信息

Anal Chem. 2013 Oct 15;85(20):9493-500. doi: 10.1021/ac400955f. Epub 2013 Oct 3.

Abstract

Point-of-care diagnostics show promise in removing reliance on centralized lab testing facilities and may help increase both the survival rate for infectious diseases as well as monitoring of chronic illnesses. CMOS compatible diagnostic platforms are currently being considered as possible solutions as they can be easily miniaturized and can be cost-effective. Top-down fabricated silicon nanowires are a CMOS-compatible technology which have demonstrated high sensitivities in detecting biological analytes, such as proteins, DNA, and RNA. However, the reported response of nanowires to these analytes has varied widely since several different functionalization protocols have been attempted with little characterization and comparison. Here we report protocols for fabrication and functionalization of silicon nanowires which yield highly stable nanowires in aqueous solutions and limits of detection to ∼1 pg/mL of the model protein used in the study. A thorough characterization was done into optimizing the release of the silicon nanowires using combined dry and wet etch techniques, which yielded nanowires that could be directly compared to increase output statistics. Moreover, a range of different linker chemistries were tried for reacting the primary antibody, and its response to target and nonspecific antigens, with polyethylene glycol based linker BS(PEG)5 providing the best response. Consequently, this chemistry was used to characterize different oxide thicknesses and their responses to the mouse IgG antigen, which with the smallest oxide thickness yielded 0.1-1 pg/mL limits of detection and a dynamic range over 3 orders of magnitude.

摘要

即时诊断在消除对集中式实验室检测设施的依赖方面显示出前景,并且可能有助于提高传染病的存活率以及慢性病的监测水平。与互补金属氧化物半导体(CMOS)兼容的诊断平台目前被视为可能的解决方案,因为它们可以轻松小型化且具有成本效益。自上而下制造的硅纳米线是一种与CMOS兼容的技术,在检测生物分析物(如蛋白质、DNA和RNA)方面已显示出高灵敏度。然而,由于尝试了几种不同的功能化方案,且几乎没有表征和比较,因此报道的纳米线对这些分析物的响应差异很大。在此,我们报告了硅纳米线的制造和功能化方案,该方案可在水溶液中产生高度稳定的纳米线,并将检测限降低至研究中使用的模型蛋白质的约1 pg/mL。通过结合干法和湿法蚀刻技术对硅纳米线的释放进行了全面表征,以优化其释放,从而获得可直接比较以增加输出统计数据的纳米线。此外,尝试了一系列不同的连接化学方法来使一抗与靶抗原和非特异性抗原反应,基于聚乙二醇的连接剂BS(PEG)5提供了最佳响应。因此,这种化学方法被用于表征不同的氧化物厚度及其对小鼠IgG抗原的响应,其中最小的氧化物厚度产生了0.1 - 1 pg/mL的检测限和超过3个数量级的动态范围。

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