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Blank peak current-suppressed electrochemical aptameric sensing platform for highly sensitive signal-on detection of small molecule

机译:空白峰值电流抑制电化学适体传感平台,用于小分子的高灵敏信号检测

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摘要

In this contribution, an electrochemical aptameric sensing scheme for the sensitive detection of small molecules is proposed using adenosine as a target model. A ferrocene (Fc)-functionalized thiolated aptamer probe is adapted and immobilized onto an electrode surface. Introducing a recognition site for EcoRI into the aptamer sequence not only suppresses the peak current corresponding to blank sample but also provides a signal-on response mechanism. In the absence of adenosine, the aptamer can fold into a hairpin structure and form a cleavable double-stranded region. Fc is capable of being removed from electrode surface by treatment with endonuclease, and almost no peak current is observed. The adenosine/aptamer binding induces the conformational transition of designed aptamer, dissociating the cleavable double-stranded segment. Therefore, the integrated aptamer sequence is maintained when exposing to endonuclease, generating a peak current of Fc. Utilizing the present sensing scheme, adenosine even at a low concentration can give a detectable current signal. Thus, a detection limit of 10−10 M and a linear response range from 3.74 × 10−9 to 3.74 × 10−5 M are achieved. The proposed proof-of-principle of a novel electrochemical sensing is expected to extend to establish various aptameric platforms for the analysis of a broad range of target molecules of interest.
机译:在此贡献中,提出了使用腺苷作为目标模型的用于敏感地检测小分子的电化学适体传感方案。将二茂铁(Fc)-官能化的硫醇化适体探针适配并固定在电极表面上。在适体序列中引入EcoRI的识别位点不仅抑制了与空白样品相对应的峰值电流,而且还提供了信号响应机制。在没有腺苷的情况下,适体可折叠成发夹结构并形成可裂解的双链区。 Fc能够通过核酸内切酶处理而从电极表面去除,几乎未观察到峰值电流。腺苷/适体结合诱导设计的适体的构象转变,解离可裂解的双链区段。因此,当暴露于核酸内切酶时,整合的适体序列得以维持,从而产生Fc的峰值电流。利用本发明的传感方案,即使在低浓度的腺苷也可以给出可检测的电流信号。这样,检测极限为10-10 M,线性响应范围为3.74××10-9至3.74××10-5×M。预期所提出的新颖电化学传感的原理证明将扩展以建立用于分析广泛范围的目标靶分子的各种适体平台。

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