Stridfeldt Fredrik, Pandey Vikash, Kylhammar Hanna, Talebian Gevari Moein, Metem Prattakorn, Agrawal Vipin, Görgens André, Mamand Doste R, Gilbert Jennifer, Palmgren Lukas, Holme Margaret N, Gustafsson Oskar, El Andaloussi Samir, Mitra Dhrubaditya, Dev Apurba
Department of Applied Physics, Kungliga Tekniska Högskolan Royal Institute of Technology, Stockholm 11419, Sweden.
Nordita, Kungliga Tekniska Högskolan Royal Institute of Technology and Stockholm University, Stockholm 11419, Sweden.
Proc Natl Acad Sci U S A. 2025 Apr 22;122(16):e2414174122. doi: 10.1073/pnas.2414174122. Epub 2025 Apr 18.
The elastic properties of nanoscale extracellular vesicles (EVs) are believed to influence their cellular interactions, thus having a profound implication in intercellular communication. However, accurate quantification of their elastic modulus is challenging due to their nanoscale dimensions and their fluid-like lipid bilayer. We show that the previous attempts to develop atomic force microscopy-based protocol are flawed as they lack theoretical underpinning as well as ignore important contributions arising from the surface adhesion forces and membrane fluctuations. We develop a protocol comprising a theoretical framework, experimental technique, and statistical approach to accurately quantify the bending and elastic modulus of EVs. The method reveals that membrane fluctuations play a dominant role even for a single EV. The method is then applied to EVs derived from human embryonic kidney cells and their genetically engineered classes altering the tetraspanin expression. The data show a large spread; the area modulus is in the range of 4 to 19 mN/m and the bending modulus is in the range of 15 to 33 [Formula: see text], respectively. Surprisingly, data for a single EV, revealed by repeated measurements, also show a spread that is attributed to their compositionally heterogeneous fluid membrane and thermal effects. Our protocol uncovers the influence of membrane protein alterations on the elastic modulus of EVs.
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