Cryosectioning-enabled super-resolution microscopy for studying nuclear architecture at the single protein level

Author:

Stein JohannesORCID,Ericsson MariaORCID,Nofal MichelORCID,Magni LorenzoORCID,Aufmkolk SarahORCID,McMillan Ryan B.ORCID,Breimann LauraORCID,Herlihy Conor P.ORCID,Lee S. DeanORCID,Willemin AndréaORCID,Wohlmann JensORCID,Arguedas-Jimenez LauraORCID,Yin PengORCID,Pombo AnaORCID,Church George M.ORCID,Wu Chao-tingORCID

Abstract

AbstractDNA-PAINT combined with total Internal Reflection Fluorescence (TIRF) microscopy enables the highest localization precisions, down to single nanometers in thin biological samples, due to TIRF’s unique method for optical sectioning and attaining high contrast. However, most cellular targets elude the accessible TIRF range close to the cover glass and thus require alternative imaging conditions, affecting resolution and image quality. Here, we address this limitation by applying ultrathin physical cryosectioning in combination with DNA-PAINT. With “tomographic & kinetically-enhanced” DNA-PAINT (tokPAINT), we demonstrate the imaging of nuclear proteins with sub-3 nanometer localization precision, advancing the quantitative study of nuclear organization within fixed cells and mouse tissues at the level of single antibodies. We believe that ultrathin sectioning combined with the versatility and multiplexing capabilities of DNA-PAINT will be a powerful addition to the toolbox of quantitative DNA-based super-resolution microscopy in intracellular structural analyses of proteins, RNA and DNAin situ.

Publisher

Cold Spring Harbor Laboratory

Cited by 1 articles. 订阅此论文施引文献 订阅此论文施引文献,注册后可以免费订阅5篇论文的施引文献,订阅后可以查看论文全部施引文献

1. Spandrels of the cell nucleus;Current Opinion in Cell Biology;2024-10

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