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基于电化学分子陷阱的单细胞内低丰度酶的检测。

Electrochemical Molecule Trap-Based Sensing of Low-Abundance Enzymes in One Living Cell.

机构信息

The State Key Lab of Analytical Chemistry for Life Science, School of Chemistry and Chemical Engineering, Nanjing University, Nanjing 210093, Jiangsu, P. R. China.

School of Chemical Sciences, University of Chinese Academy of Science, Beijing 100190, P. R. China.

出版信息

J Am Chem Soc. 2022 Sep 28;144(38):17558-17566. doi: 10.1021/jacs.2c06962. Epub 2022 Sep 16.

Abstract

Measuring the activity of low-abundance enzymes, down to a few molecules in one living cell, is important but challenging to elucidate their biological function. Here, an electrochemical molecule trap is established at the tip of a nanopipette with an electrochemical detector, in which the diffusion of the molecules away from the electrochemical detector is prevented by electro-osmotic flow (EOF). Accordingly, a limited amount of enzymes is trapped to continuously catalyze the conversion of the substrate to generate a sufficient amount of the byproduct hydrogen peroxide for electrochemical measurements. The resistive pulse sensing of the enzymes in single liposomes validates the detection sensitivity down to 15 molecules. Using this ultrasensitive electrochemical strategy, the activity of 60 sphingomyelinase molecules inside single unstimulated living J774 cells is measured, which was hardly detected by previous methods. The established electrochemical molecule trap-based sensing approach opens the door toward single-molecule electrochemical detection in one living cell. This success will solve the long-standing problem regarding the study of the activity of low-abundance proteins in cells in their native physiological state and greatly enhance the understanding of the roles of proteins in cellular behavior.

摘要

测量低丰度酶的活性,低至一个活细胞中的几个分子,对于阐明其生物学功能很重要,但也具有挑战性。在这里,在带有电化学检测器的纳米移液器尖端建立了电化学分子陷阱,其中电渗流 (EOF) 阻止分子从电化学检测器扩散。因此,将有限量的酶捕获以连续催化底物的转化,以产生足够量的副产物过氧化氢进行电化学测量。在单个脂质体中的酶的电阻脉冲感应验证了检测灵敏度低至 15 个分子。使用这种超灵敏的电化学策略,测量了单个未受刺激的活 J774 细胞内 60 个神经鞘磷脂酶分子的活性,这是以前的方法很难检测到的。所建立的基于电化学分子陷阱的传感方法为在单个活细胞中的单分子电化学检测开辟了道路。这一成功将解决长期以来关于在其天然生理状态下研究细胞中低丰度蛋白质活性的问题,并极大地增强对蛋白质在细胞行为中的作用的理解。

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