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荧光相关光谱法实时监测基于 Kai 蛋白的生物钟振荡。

Fluorescence correlation spectroscopy to monitor Kai protein-based circadian oscillations in real time.

机构信息

Medical Technology Research and Development Division, Advanced Analysis Technology Research and Development Department, Olympus Corporation, Tokyo 192-0904, Japan.

出版信息

J Biol Chem. 2012 Jan 27;287(5):3241-8. doi: 10.1074/jbc.M111.265777. Epub 2011 Dec 6.

Abstract

Dynamic protein-protein interactions play an essential role in cellular regulatory systems. The cyanobacterial circadian clock is an oscillatory system that can be reconstituted in vitro by mixing ATP and three clock proteins: KaiA, KaiB, and KaiC. Association and dissociation of KaiB from KaiC-containing complexes are critical to circadian phosphorylation and dephosphorylation of KaiC. We developed an automated and noninvasive method to monitor dynamic complex formation in real time using confocal fluorescence correlation spectroscopy (FCS) and uniformly labeled KaiB as a probe. A nanomolar concentration of the labeled KaiB for FCS measurement did not interfere with the oscillatory system but behaved similarly to the wild-type one during the measurement period (>5 days). The fluorescent probe was stable against repeated laser exposure. As an application, we show that this detection system allowed analysis of the dynamics of both long term circadian oscillations and short term responses to temperature changes (∼10 min) in the same sample. This suggested that a phase shift of the clock with a high temperature pulse occurred just after the stimulus through dissociation of KaiB from the KaiC complex. This monitoring method should improve our understanding of the mechanisms underlying this cellular circadian oscillator and provide a means to assess dynamic protein interactions in biological systems characterized by rates similar to those observed with the Kai proteins.

摘要

动态蛋白质-蛋白质相互作用在细胞调节系统中起着至关重要的作用。蓝藻生物钟是一个可以通过混合 ATP 和三种生物钟蛋白:KaiA、KaiB 和 KaiC 在体外重建的振荡系统。KaiB 与包含 KaiC 的复合物的结合和解离对于 KaiC 的生物钟磷酸化和去磷酸化至关重要。我们开发了一种自动且非侵入性的方法,使用共焦荧光相关光谱(FCS)和标记的 KaiB 作为探针实时监测动态复合物的形成。用于 FCS 测量的纳米摩尔浓度的标记 KaiB 不会干扰振荡系统,但在测量期间(>5 天)表现与野生型相似。荧光探针对重复激光暴露稳定。作为应用,我们表明,这种检测系统允许在同一样品中分析长期生物钟振荡和对温度变化(约 10 分钟)的短期反应的动力学。这表明,时钟的相位偏移伴随着高温脉冲发生,就在 KaiB 从 KaiC 复合物解离后立即发生。这种监测方法应该有助于我们理解这个细胞生物钟振荡器的机制,并提供一种评估具有与 Kai 蛋白相似速率的生物系统中动态蛋白质相互作用的手段。

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