Mechanical alterations of protein condensates are increasingly recognized in the etiology of several neurodegenerative diseases, yet their characterization remains technically challenging. Although Brillouin microscopy could offer a promising solution, its use is hindered by instrumental instabilities demanding frequent adjustments and manual calibrations with reference materials. Here, we present an enhanced Brillouin Microscope that incorporates an electro-optic modulator, serving simultaneously as frequency reference, spectrometer calibrator, and temporal stabilizer. This integration enables robust, real-time spectral stability over multiple days in a fully automated workflow. Using this system, we quantify Brillouin shifts of several protein condensates in living cells and validate our findings with FRAP. The correlation between techniques reveals a fractal internal architecture of the condensates, providing important insights into their physical nature while probing the mechanical behavior of entire compartments containing multiple protein species. Our method offers a unique framework for distinguishing physiological from pathological condensates, paving the way for long-term, user-independent, high-precision mechanical measurements in living cells.
Stabilized real-time Brillouin microscopy reveals fractal organization of protein condensates in living cells / Testi, Claudia; Pontecorvo, Emanuele; Bartoli, Chiara; Marzaro, Chiara; Gala, Fabrizio; Zhang, Li; Zanini, Giulia; D'Abbondanza, Noemi; Garone, Maria Giovanna; De Turris, Valeria; Giuliani, Andrea; Di Timoteo, Gaia; Bozzoni, Irene; Rosa, Alessandro; Ruocco, Giancarlo. - In: NATURE COMMUNICATIONS. - ISSN 2041-1723. - 17:1(2026), pp. 1-18. [10.1038/s41467-026-68984-2]
Stabilized real-time Brillouin microscopy reveals fractal organization of protein condensates in living cells
Testi, Claudia
;Pontecorvo, Emanuele;Bartoli, Chiara;Gala, Fabrizio;D'Abbondanza, Noemi;Garone, Maria Giovanna;de Turris, Valeria;Giuliani, Andrea;Di Timoteo, Gaia;Bozzoni, Irene;Rosa, Alessandro;Ruocco, Giancarlo
2026
Abstract
Mechanical alterations of protein condensates are increasingly recognized in the etiology of several neurodegenerative diseases, yet their characterization remains technically challenging. Although Brillouin microscopy could offer a promising solution, its use is hindered by instrumental instabilities demanding frequent adjustments and manual calibrations with reference materials. Here, we present an enhanced Brillouin Microscope that incorporates an electro-optic modulator, serving simultaneously as frequency reference, spectrometer calibrator, and temporal stabilizer. This integration enables robust, real-time spectral stability over multiple days in a fully automated workflow. Using this system, we quantify Brillouin shifts of several protein condensates in living cells and validate our findings with FRAP. The correlation between techniques reveals a fractal internal architecture of the condensates, providing important insights into their physical nature while probing the mechanical behavior of entire compartments containing multiple protein species. Our method offers a unique framework for distinguishing physiological from pathological condensates, paving the way for long-term, user-independent, high-precision mechanical measurements in living cells.| File | Dimensione | Formato | |
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