| Literature DB >> 29672025 |
Mengfei Gao1, Riccardo Maraspini2, Oliver Beutel2, Amin Zehtabian1, Britta Eickholt3, Alf Honigmann2, Helge Ewers1.
Abstract
Stimulated emission depletion (STED) microscopy is routinely used to resolve the ultrastructure of cells with a ∼10-fold higher resolution compared to diffraction limited imaging. While STED microscopy is based on preparing the excited state of fluorescent probes with light, the recently developed expansion microscopy (ExM) provides subdiffraction resolution by physically enlarging the sample before microscopy. The expansion of the fixed cells by cross-linking and swelling of hydrogels easily enlarges the sample ∼4-fold and hence increases the effective optical resolution by this factor. To overcome the current limits of these complementary approaches, we combined ExM with STED (ExSTED) and demonstrated an increase in resolution of up to 30-fold compared to conventional microscopy (<10 nm lateral and ∼50 nm isotropic). While the increase in resolution is straightforward, we found that high-fidelity labeling via multi-epitopes is required to obtain emitter densities that allow ultrastructural details with ExSTED to be resolved. Our work provides a robust template for super-resolution microscopy of entire cells in the ten nanometer range.Keywords: actin ring; cilium; expansion microscopy; microtubule; stimulated emission depletion microscopy; super-resolution microscopy
Year: 2018 PMID: 29672025 DOI: 10.1021/acsnano.8b00776
Source DB: PubMed Journal: ACS Nano ISSN: 1936-0851 Impact factor: 15.881