Spatiotemporally resolved mapping of extracellular proteomes via in vivo-compatible TyroID

蛋白质组 计算生物学 体内 细胞外 细胞生物学 生物 计算机科学 化学 生物信息学 遗传学
作者
Zijuan Zhang,Yankun Wang,Wenjie Lu,Xiaofei Wang,Hongyang Guo,Xuanzhen Pan,Zeyu Liu,Zhaofa Wu,Wei Qin
出处
期刊:Nature Communications [Springer Nature]
卷期号:16 (1) 被引量:2
标识
DOI:10.1038/s41467-025-57767-w
摘要

Extracellular proteins play pivotal roles in both intracellular signaling and intercellular communications in health and disease. While recent advancements in proximity labeling (PL) methods, such as peroxidase- and photocatalyst-based approaches, have facilitated the resolution of extracellular proteomes, their in vivo compatibility remains limited. Here, we report TyroID, an in vivo-compatible PL method for the unbiased mapping of extracellular proteins with high spatiotemporal resolution. TyroID employs plant- and bacteria-derived tyrosinases to produce reactive o-quinone intermediates, enabling the labeling of multiple residues on endogenous proteins with bioorthogonal handles, thereby allowing for their identification via chemical proteomics. We validate TyroID's specificity by mapping extracellular proteomes and HER2-neighboring proteins using affibody-directed recombinant tyrosinases. Demonstrating its superiority over other PL methods, TyroID enables in vivo mapping of extracellular proteomes, including mapping HER2-proximal proteins in tumor xenografts, quantifying the turnover of plasma proteins and labeling hippocampal-specific proteomes in live mouse brains. TyroID emerges as a potent tool for investigating protein localization and molecular interactions within living organisms. TyroID is a proximity labeling method that maps extracellular proteins with high spatiotemporal resolution through plant- and bacteria-derived tyrosinases. TyroID efficiently labels proteins in vivo to study of localization and interactions.
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