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荧光素酶调控蛋白相互作用。

Luciferase Controlled Protein Interactions.

机构信息

School of Chemistry and Biochemistry, Department of Organic Chemistry, NCCR Chemical Biology, Faculty of Science, University of Geneva, 30 quai Ernest-Ansermet, Geneva 12004, Switzerland.

School of Chemistry and Biochemistry, Department of Biochemistry, NCCR Chemical Biology, Faculty of Science, University of Geneva, 30 quai Ernest-Ansermet, Geneva 12004, Switzerland.

出版信息

J Am Chem Soc. 2021 Mar 17;143(10):3665-3670. doi: 10.1021/jacs.0c11016. Epub 2021 Mar 8.

Abstract

Protein trafficking and protein-protein interactions (PPIs) are central to regulatory processes in cells. Induced dimerization systems have been developed to control PPIs and regulate protein trafficking (localization) or interactions. Chemically induced dimerization (CID) has proven to be a robust approach to control protein interactions and localization. The most recent embodiment of this technology relies on CID conjugates that react with a self-labeling protein on one side and a photocaged ligand on the other side to provide spatiotemporal control of the interaction with the protein of interest. Advancing this technology further is limited by the light delivery problem and the phototoxicity of intense irradiation necessary to achieve photouncaging. Herein, we designed a novel chemically induced dimerization system that was triggered by bioluminescence, instead of external light. Protein dimerization showed fast kinetics and was validated by an induced change of localization of a target protein (to and from the nucleus or plasma membrane) upon trigger. The technology was used transiently to activate the phosphatidylinositol 3-kinase (PI3K)/mTOR pathway and measure the impact on lipid synthesis/metabolism, assessed by lipidomics.

摘要

蛋白质运输和蛋白质-蛋白质相互作用(PPIs)是细胞内调控过程的核心。已经开发了诱导二聚化系统来控制 PPI 并调节蛋白质运输(定位)或相互作用。化学诱导二聚化(CID)已被证明是一种控制蛋白质相互作用和定位的有效方法。该技术的最新体现形式依赖于 CID 缀合物,该缀合物在一侧与自标记蛋白反应,在另一侧与光笼化配体反应,以提供与感兴趣的蛋白质相互作用的时空控制。进一步推进这项技术受到光传输问题和实现光解笼所需的强烈辐照的光毒性的限制。在此,我们设计了一种新型的化学诱导二聚化系统,该系统由生物发光触发,而不是外部光触发。蛋白质二聚化表现出快速的动力学,并通过目标蛋白定位的诱导变化(从核或质膜到核或质膜)得到验证。该技术被用于瞬时激活磷脂酰肌醇 3-激酶(PI3K)/mTOR 途径,并通过脂质组学评估对脂质合成/代谢的影响。

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