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基于表面特性调制的创新型 microRNA 纯化。

Innovative microRNA purification based on surface properties modulation.

机构信息

Fondazione Bruno Kessler, Laboratory of Biomolecular Sequence and Structure Analysis for Health, via Sommarive 18, I-38123 Povo, Trento, Italy.

Fondazione Bruno Kessler, Laboratory of Biomolecular Sequence and Structure Analysis for Health, via Sommarive 18, I-38123 Povo, Trento, Italy; CNR - Consiglio Nazionale delle Ricerche, Istituto di Biofisica, via alla Cascata 56/C, I-38123 Povo, Trento, Italy.

出版信息

Colloids Surf B Biointerfaces. 2014 Apr 1;116:160-8. doi: 10.1016/j.colsurfb.2013.12.033. Epub 2014 Jan 6.

DOI:10.1016/j.colsurfb.2013.12.033
PMID:24463152
Abstract

The increasing interest in circulating microRNAs (miRNAs) as potential non-invasive cancer biomarkers has prompted the rapid development of several extraction techniques. However, current methods lack standardization and are costly and labor intensive. In light of this, we developed a microRNA solid-phase extraction strategy based on charge and roughness modulation on substrate surfaces. PECVD treated silicon oxide (PECVD-SO) and thermally grown silicon oxide (TG-SO) surfaces were functionalized with positively charged 3-aminopropyltriethoxysilanes (APTES) and neutral poly(ethylene glycol) silanes (PEG-s) mixed in different proportions to modulate the density of net positive charges and the roughness of the substrate. Characterization of the surfaces was performed by atomic force microscopy (AFM), X-ray photoelectron spectroscopy (XPS) and s-SDTB (sulfosuccinimidyl-4-o-(4,4-dimethoxytrityl) butyrate) assay in order to investigate the surface morphology and chemical composition, respectively. Adsorption and elution efficiency were assessed by fluorescence microscopy by means of synthetic fluorescently labeled microRNAs. We identified PECVD-SO functionalized with 0.1% APTES and 0.9% 21-24 units long PEG-s as a promising surface able to selectively bind microRNAs and release them in the presence of a basic buffer (pH=9) compatible with downstream analyses. MicroRNA integrity was assessed by reverse transcription and real-time PCR and confirmed by electrophoresis (Agilent 2100 Bioanalyzer), while binding competition from circulating DNA and proteins was excluded by fluorescence analyses and real-time PCR. On the contrary, total RNA slightly decreased miRNA adsorption. In conclusion, we showed an innovative and easy solid-state purification method for circulating miRNAs based on charge interaction, which could pave the path to future diagnostic and prognostic assays feasible as a routine test.

摘要

循环 microRNAs(miRNAs)作为潜在的非侵入性癌症生物标志物的兴趣日益浓厚,这促使了几种提取技术的快速发展。然而,目前的方法缺乏标准化,且成本高、劳动强度大。有鉴于此,我们基于基底表面的电荷和粗糙度调制开发了一种 miRNA 固相提取策略。PECVD 处理的氧化硅(PECVD-SO)和热生长氧化硅(TG-SO)表面通过正电荷 3-氨丙基三乙氧基硅烷(APTES)和中性聚(乙二醇)硅烷(PEG-s)以不同比例混合进行功能化,以调节基底的净正电荷密度和粗糙度。通过原子力显微镜(AFM)、X 射线光电子能谱(XPS)和 s-SDTB(琥珀酰亚胺-4-O-(4,4-二甲氧基三苯甲基)丁酸酯)测定分别对表面形貌和化学组成进行了表征。通过荧光显微镜评估了吸附和洗脱效率,分别采用合成的荧光标记 miRNA。我们发现,PECVD-SO 经 0.1%APTES 和 0.9%21-24 个单位长的 PEG-s 功能化后是一种很有前途的表面,能够选择性地结合 microRNAs,并在碱性缓冲液(pH=9)存在下释放,该缓冲液与下游分析兼容。通过反转录和实时 PCR 评估了 microRNA 的完整性,并通过电泳(Agilent 2100 Bioanalyzer)进行了确认,而通过荧光分析和实时 PCR 排除了循环 DNA 和蛋白质的结合竞争。相反,总 RNA 略微降低了 miRNA 的吸附。总之,我们展示了一种基于电荷相互作用的新型简单循环 miRNA 固相纯化方法,为未来基于诊断和预后的可行常规检测铺平了道路。

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