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基于 l-Cys-血红素/G-四链体的高效电化学自催化平台及其在生物测定中的应用。

Efficient Electrochemical Self-Catalytic Platform Based on l-Cys-hemin/G-quadruplex and Its Application for Bioassay.

机构信息

Key Laboratory of Luminescent and Real-Time Analytical Chemistry (Southwest University), Ministry of Education, College of Chemistry and Chemical Engineering , Southwest University , Chongqing 400715 , China.

出版信息

Anal Chem. 2018 Aug 7;90(15):9109-9116. doi: 10.1021/acs.analchem.8b01526. Epub 2018 Jul 18.

Abstract

Commonly, in the artificial enzyme-involved signal amplification approach, the catalytic efficiency was limited by the relatively low binding affinity between artificial enzyme and substrate. In this work, substrate l-cysteine (l-Cys) and hemin were combined into one molecule to form l-Cys-hemin/G-quadruplex as an artificial self-catalytic complex for the improvement of the binding affinity between l-Cys-hemin/G-quadruplex and l-Cys. The apparent Michaelis-Menten constant ( K = 2.615 μM) on l-Cys-hemin/G-quadruplex for l-Cys was further investigated to assess the affinity, which was much lower than that of hemin/G-quadruplex ( K = 8.640 μM), confirming l-Cys-hemin/G-quadruplex possessed better affinity to l-Cys compared with that of hemin/G-quadruplex. Meanwhile, l-Cys bilayer could be further assembled onto the surface of l-Cys-hemin/G-quadruplex based on hydrogen-bond and electrostatic interaction to concentrate l-Cys around the active center, which was beneficial to the catalytic enhancement. Through this efficient electrochemical self-catalytic platform, a sensitive thrombin aptasensor was constructed. The results exhibited good sensitivity from 0.1 pM to 80 nM and the detection limit was calculated to be 0.032 pM. This self-catalytic strategy with improved binding affinity between l-Cys-hemin/G-quadruplex and l-Cys could provide an efficient approach to improve artificial enzymatic catalytic efficiency.

摘要

通常,在人工酶参与的信号放大方法中,由于人工酶与底物之间的结合亲和力相对较低,因此催化效率受到限制。在这项工作中,将底物 l-半胱氨酸(l-Cys)和血红素结合到一个分子中,形成 l-Cys-血红素/G-四链体作为人工自催化复合物,以提高 l-Cys-血红素/G-四链体与 l-Cys 之间的结合亲和力。进一步研究了 l-Cys-血红素/G-四链体对 l-Cys 的表观米氏常数(K = 2.615 μM),以评估亲和力,其明显低于血红素/G-四链体(K = 8.640 μM),证实了 l-Cys-血红素/G-四链体与 l-Cys 的亲和力比血红素/G-四链体更好。同时,l-Cys 双层可以进一步基于氢键和静电相互作用组装到 l-Cys-血红素/G-四链体的表面上,以将 l-Cys 浓缩在活性中心周围,这有利于催化增强。通过这种高效的电化学自催化平台,构建了一种灵敏的凝血酶适体传感器。结果显示,从 0.1 pM 到 80 nM 具有良好的灵敏度,检测限计算为 0.032 pM。这种提高 l-Cys-血红素/G-四链体与 l-Cys 之间结合亲和力的自催化策略可以为提高人工酶催化效率提供一种有效的方法。

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