“…Selective staining of intact EVs remains a challenge to understand their biological roles, including physiological and pathological functions, clinical potential, and the intracellular fate of their molecular components [ 7 , 9 , 10 ]. Current fluorescent EV staining strategies have limitations, including low selectivity and throughput [ 10 , 11 , 12 , 13 ]. For instance, prevailing fluorescent and other labeling or staining strategies for isolated EVs utilize lipid membrane-, surface protein-, luminal-, nucleic acid-, radionuclide-, and quantum dot (QD)-labels for visualization and characterization of EVs [ 10 , 14 ].…”