Reactive fluorescent probe for covalent membrane-anchoring: enabling real-time imaging of protein aggregation dynamics in live cells

Aberrant aggregation of membrane proteins is a pathological hallmark of various diseases, including neurodegenerative disorders and cancer. The visualization of membrane protein aggregation has emerged as an important approach for investigating protein structure and function and for studying disease mechanisms and therapeutic interventions. While significant progress has been made in modifying membrane proteins and studying related biological processes, membrane protein aggregation remains underexplored, largely due to the lack of simple and effective methods for directly labeling native proteins and tracking this process in real time. With this research, we present a fluorescent probe equipped with a membrane-anchoring unit and a covalent reactive moiety for visualizing membrane protein dynamics, which operates via a two-stage mechanism: first, rapid electrostatic interaction-mediated localization to the cell membrane, followed by chemoselective macrocyclization with thiol and amine groups on membrane proteins to form a fluorescent conjugate, whose emission is substantially enhanced due to restriction of twisted intramolecular charge transfer (TICT) within the confined microenvironment induced by protein aggregation. Leveraging this mechanism, the probe successfully reports membrane protein aggregation triggered by diverse stressors, such as redox imbalance and chemotherapeutic agents, while also capturing distinct membrane reorganization dynamics. With features of biocompatibility, wash-free performance, and long-term membrane retention, this probe provides an alternative tool for evaluating the complex structural dynamics of membrane proteins and offers potential for developing targeted therapeutic strategies.