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Single-enzyme kinetics with fluorogenic substrates: Lessons learnt and future directions

机译:含荧光底物的单酶动力学:经验教训和未来方向

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Single-molecule fluorescence techniques have developed into powerful tools for studying the kinetics of biological reactions at the single-molecule level. Using fluorogenic substrates, enzymatic reactions can be observed in real-time with single-turnover resolution. The turnover sequence contains all kinetic information, giving access to reaction substeps and dynamic processes such as fluctuations in the reaction rate. Despite their clearly proven potential, the accuracy of current measurements is limited by the availability of substrates with 1:1 stoichiometry and the signal-to-noise ratio of the measurement. In this review we summarize the state-of-the-art and discuss these limitations using experiments performed with α-chymotrypsin as an example. We are further providing an overview of recent efforts aimed at the improvement of fluorogenic substrates and the development of new detection schemes. These detection schemes utilize nanophotonic structures such as zero mode waveguides or nanoantennas. Nanophotonic approaches reduce the size of the effective detection volume and are a powerful strategy to increase the signal-to-noise ratio. We believe that a combination of improved substrates and novel detection schemes will pave the way for performing accurate single-enzyme experiments in biologically relevant conditions.
机译:单分子荧光技术已发展成为研究单分子水平生物反应动力学的强大工具。使用荧光底物,可以以单周转分辨率实时观察酶促反应。周转序列包含所有动力学信息,可以访问反应子步骤和动态过程,例如反应速率的波动。尽管具有明确的潜力,但电流测量的准确性受到化学计量比为1:1的底物的可用性以及测量的信噪比的限制。在这篇综述中,我们总结了最新技术,并以α-胰凝乳蛋白酶为例讨论了这些局限性。我们进一步概述了旨在改善荧光底物和开发新检测方案的最新努力。这些检测方案利用纳米光子结构,例如零模波导或纳米天线。纳米光子学方法减小了有效检测体积的大小,并且是增加信噪比的有效策略。我们相信,改进的底物和新颖的检测方案的结合将为在生物学相关条件下进行准确的单酶实验铺平道路。

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