Controlled Grafting Expansion Microscopy

Author:

Thielhorn Ria1,Heing‐Becker Isabelle2,Hümpfer Nadja1,Rentsch Jakob1,Haag Rainer2,Licha Kai2,Ewers Helge1ORCID

Affiliation:

1. Institut für Chemie und Biochemie Freie Universität Berlin Thielallee 63 14195 Berlin Germany

2. Institut für Chemie und Biochemie Freie Universität Berlin Takustr. 3 14195 Berlin Germany

Abstract

AbstractExpansion microscopy (ExM) is a recently developed technique that allows for the resolution of structures below the diffraction limit by physically enlarging a hydrogel‐embedded facsimile of the biological sample. The target structure is labeled and this label must be retained in a relative position true to the original, smaller state before expansion by linking it into the gel. However, gel formation and digestion lead to a significant loss in target‐delivered label, resulting in weak signal. To overcome this problem, we have here developed an agent combining targeting, fluorescent labeling and gel linkage in a single small molecule. Similar approaches in the past have still suffered from significant loss of label. Here we show that this loss is due to insufficient surface grafting of fluorophores into the hydrogel and develop a solution by increasing the amount of target‐bound monomers. Overall, we obtain a significant improvement in fluorescence signal retention and our new dye allows the resolution of nuclear pores as ring‐like structures, similar to STED microscopy. We furthermore provide mechanistic insight into dye retention in ExM.

Funder

Deutsche Forschungsgemeinschaft

Dahlem Research School, Freie Universität Berlin

Publisher

Wiley

Subject

General Chemistry,Catalysis

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