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Targeted activation in localized protein environments via deep red photoredox catalysis

化学 光催化 催化作用 小分子 叠氮化物 生物物理学 纳米技术 光化学 组合化学 光催化 生物化学 生物 有机化学 材料科学
作者
Nicholas E. S. Tay,Keun Ah Ryu,John L. Weber,Aleksandra Olow,David C. Cabanero,David R. Reichman,Rob Oslund,Olugbeminiyi Fadeyi,Tomislav Rovis
出处
期刊:Nature Chemistry [Nature Portfolio]
卷期号:15 (1): 101-109 被引量:95
标识
DOI:10.1038/s41557-022-01057-1
摘要

State-of-the-art photoactivation strategies in chemical biology provide spatiotemporal control and visualization of biological processes. However, using high-energy light (λ < 500 nm) for substrate or photocatalyst sensitization can lead to background activation of photoactive small-molecule probes and reduce its efficacy in complex biological environments. Here we describe the development of targeted aryl azide activation via deep red-light (λ = 660 nm) photoredox catalysis and its use in photocatalysed proximity labelling. We demonstrate that aryl azides are converted to triplet nitrenes via a redox-centric mechanism and show that its spatially localized formation requires both red light and a photocatalyst-targeting modality. This technology was applied in different colon cancer cell systems for targeted protein environment labelling of epithelial cell adhesion molecule (EpCAM). We identified a small subset of proteins with previously known and unknown association to EpCAM, including CDH3, a clinically relevant protein that shares high tumour-selective expression with EpCAM. Technologies for profiling biological environments with high spatiotemporal resolution are in demand to enable the discovery of new targets for addressing unmet clinical needs. Now, a deep red light-mediated photocatalytic strategy for the targeted activation of aryl azides has been developed. This platform enables mapping of protein microenvironments in physiologically relevant systems.
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