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利用低污染表面等离子体共振生物传感器快速灵敏地检测细胞裂解液中的多种 microRNAs。

Rapid and sensitive detection of multiple microRNAs in cell lysate by low-fouling surface plasmon resonance biosensor.

机构信息

Institute of Photonics and Electronics, Academy of Sciences of the Czech Republic, Chaberská 57, 18251 Prague, Czech Republic.

Institute of Hematology and Blood Transfusion, U Nemocnice 1, 12820 Prague, Czech Republic.

出版信息

Biosens Bioelectron. 2015 Aug 15;70:226-31. doi: 10.1016/j.bios.2015.03.038. Epub 2015 Mar 17.

DOI:10.1016/j.bios.2015.03.038
PMID:25829219
Abstract

We report an ultra-low fouling surface plasmon resonance imaging (SPRi) biosensor for the rapid simultaneous detection of multiple miRNAs in erythrocyte lysate (EL) at subpicomolar levels without need of RNA extraction. The SPRi chips were coated with ultra-low fouling functionalizable poly(carboxybetaine acrylamide) (pCBAA) brushes having optimized thicknesses and directly functionalized with amino-modified oligonucleotide probes. We have characterized the effect of the brush thickness on the probe loading capacity: a loading capacity of ~9.8×10(12) probes/cm(2) was achieved for pCBAA having a thickness of ~40 nm. The probe-functionalized sensor also exhibited a high resistance to fouling from ~90% EL samples (<2 ng/cm(2)). A two-step detection assay was employed for multiplexed miRNA detection in EL. Specifically, the assay consisted of (i) a sandwich-type hybridization of the probe-functionalized pCBAA with target miRNA in EL (bound to biotinylated oligonucleotides) and (ii) the capture of streptavidin-functionalized gold nanoparticles to the aforementioned biotinylated probes. We have demonstrated that this approach enables the detection of miRNAs in EL at concentrations as low as 0.5 pM. Finally, we have confirmed the detection of four endogenous miRNAs representing a set of potential miRNA biomarkers of myelodysplastic syndrome (MDS) in clinical EL samples (miR-16, miR-181, miR-34a, and miR-125b). The results revealed significantly higher levels of miR-16 in all the clinical EL samples compared to the other measured miRNAs.

摘要

我们报道了一种超低污染的表面等离子体共振成像(SPRi)生物传感器,可在亚皮摩尔水平下无需 RNA 提取即可快速同时检测红细胞裂解液(EL)中的多种 miRNA。SPRi 芯片涂有超低污染的可功能化聚(羧基甜菜碱丙烯酰胺)(pCBAA)刷,其具有优化的厚度,并直接用氨基修饰的寡核苷酸探针功能化。我们已经研究了刷厚度对探针负载能力的影响:厚度约为 40nm 的 pCBAA 实现了约 9.8×10(12)个探针/cm(2)的负载能力。探针功能化的传感器还表现出对来自约 90%EL 样品(<2ng/cm(2))的污染的高抵抗力。采用两步检测法在 EL 中进行多重 miRNA 检测。具体而言,该检测法包括 (i)EL 中探针功能化的 pCBAA 与靶 miRNA(与生物素化寡核苷酸结合)的夹心型杂交,以及 (ii)链霉亲和素功能化的金纳米粒子对上述生物素化探针的捕获。我们已经证明,这种方法可以检测 EL 中低至 0.5pM 的 miRNA。最后,我们在临床 EL 样本中证实了四种内源性 miRNA 的检测,它们代表了骨髓增生异常综合征(MDS)的一组潜在 miRNA 生物标志物(miR-16、miR-181、miR-34a 和 miR-125b)。结果表明,与其他测量的 miRNA 相比,所有临床 EL 样本中的 miR-16 水平均显著升高。

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