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电化学法检测乳腺癌细胞中的 microRNA,mir21。

Electrochemical based detection of microRNA, mir21 in breast cancer cells.

机构信息

Department of Biomedical Engineering, Faculty of Engineering and Architecture, Katip Celebi University, Izmir, Turkey.

出版信息

Biosens Bioelectron. 2012 Oct-Dec;38(1):195-201. doi: 10.1016/j.bios.2012.05.031. Epub 2012 Jun 16.

DOI:10.1016/j.bios.2012.05.031
PMID:22776181
Abstract

In this work, a novel electrochemical microRNA (miRNA) detection method based on enzyme amplified biosensing of mir21 from cell lysate of total RNA was demonstrated. The proposed enzymatic detection method was detailed and compared with the conventional guanine oxidation based assay in terms of detection limit and specificity. For the detection of mir21, capture probes and/or cell lysates were covalently attached onto the pencil graphite electrode (PGE) by coupling agents of N-(dimethylamino)propyl-N'-ethylcarbodiimide hydrochloride (EDC) and N-hydroxysulfosuccinimide (NHS). Having immobilized the capture probe onto the surface of PGE, hybridization was achieved with a biotinylated (from its 3' end) complementary target. Extravidin labeled alkaline phosphatase (Ex-Ap) binds to the biotinylated target due to the interaction between biotin-avidin and the enzyme converts electro-inactive alpha naphtyl phosphate (the substrate) to electro-active alpha naphtol (α-NAP, the product). α-NAP was oxidized at +0.23 V vs Ag/AgCl and this signal was measured by Differential Pulse Voltammetry (DPV). The signals obtained from α-NAP oxidation were compared for the probe and hybrid DNA. The specificity of the designed biosensor was proved by using non-complementary sequences instead of complementary sequences and the detection limit of the assay was calculated to be 6 pmol for cell lysates.

摘要

在这项工作中,展示了一种基于酶放大生物传感的新型电化学 microRNA (miRNA) 检测方法,用于从总 RNA 的细胞裂解物中检测 mir21。所提出的酶检测方法进行了详细描述,并与传统的基于鸟嘌呤氧化的测定方法在检测限和特异性方面进行了比较。为了检测 mir21,捕获探针和/或细胞裂解物通过偶联剂 N-(二甲氨基)丙基-N'-乙基碳二亚胺盐酸盐 (EDC) 和 N-羟基琥珀酰亚胺 (NHS) 共价附着在铅笔石墨电极 (PGE) 上。将捕获探针固定在 PGE 表面后,通过与生物素化(从其 3' 端)互补靶标进行杂交来实现。链霉亲和素标记的碱性磷酸酶 (Ex-Ap) 由于生物素-亲和素的相互作用与生物素化的靶标结合,并且该酶将非活性的α-萘基磷酸酯(底物)转化为活性的α-萘酚(α-NAP,产物)。α-NAP 在 +0.23 V 相对于 Ag/AgCl 被氧化,并且通过差分脉冲伏安法(DPV)测量该信号。通过使用非互补序列而不是互补序列来证明设计的生物传感器的特异性,并计算出该测定的检测限为 6 pmol 用于细胞裂解物。

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