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Three-Dimensional Single Molecule Localization Microscopy Reveals the Topography of the Immunological Synapse at Isotropic Precision below 15 nm
Author(s) -
Lukáš Veľas,
Mario Brameshuber,
Johannes B. Huppa,
Elke Kurz,
Michael L. Dustin,
Philipp Zelger,
Alexander Jesacher,
Gerhard J. Schütz
Publication year - 2021
Publication title -
nano letters
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 4.853
H-Index - 488
eISSN - 1530-6992
pISSN - 1530-6984
DOI - 10.1021/acs.nanolett.1c03160
Subject(s) - immunological synapse , biophysics , microscopy , lipid bilayer , synapse , fluorescence microscope , isotropy , bilayer , materials science , sted microscopy , t cell receptor , chemistry , nanotechnology , fluorescence , t cell , biology , optics , membrane , physics , biochemistry , laser , immune system , neuroscience , stimulated emission , immunology
T-cells engage with antigen-presenting cells in search for antigenic peptides and form transient interfaces termed immunological synapses. Synapse topography affects receptor binding rates and the mutual segregation of proteins due to size exclusion effects. It is hence important to determine the 3D topography of the immunological synapse at high precision. Current methods provide only rather coarse images of the protein distribution within the synapse. Here, we applied supercritical angle fluorescence microscopy combined with defocused imaging, which allows three-dimensional single molecule localization microscopy (3D-SMLM) at an isotropic localization precision below 15 nm. Experiments were performed on hybrid synapses between primary T-cells and functionalized glass-supported lipid bilayers. We used 3D-SMLM to quantify the cleft size within the synapse by mapping the position of the T-cell receptor (TCR) with respect to the supported lipid bilayer, yielding average distances of 18 nm up to 31 nm for activating and nonactivating bilayers, respectively.

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