Enhanced dSTORM imaging using fluorophores interacting with cucurbituril

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Advanced fluorescence microscopy including single-molecule localization-based super-resolution imaging techniques requires bright and photostable dyes orproteins asfluorophores.The photophysical properties of fluorophores have been proven to be crucial for super-resolution microscopy’s localization precision and imaging resolution.Fluorophores TAMRA and Atto Rho6 G,which can interact with macrocyclic host cucurbit[7]uril(CB7) to form host-guest compounds,were found to improve the fluorescence intensity and lifetimes of these dyes.We enhanced the localization precision of direct stochastic optical reconstruction microscopy(dSTORM) by introducing CB7 into the imaging buffer,and showed that the number of photons as well as localizations of both TAMRA and Atto Rho6 G increase over 2 times. Advanced fluorescence microscopy including single-molecule localization-based super-resolution imaging technique requires bright and photostable dyes orproteins as fluorophores. The photophysical properties of fluorophores have been proven to be crucial for super-resolution microscopy of localization precision and imaging resolution. Fluorophores TAMRA and Atto Rho 6 G, which can interact with macrocyclic host cucurbit [7] uril (CB7) to form host-guest compounds, were found to improve the fluorescence intensity and lifetimes of these dyes. We enhanced the localization precision of direct stochastic optical reconstruction microscopy (dSTORM) by introducing CB7 into the imaging buffer, and showed that the number of photons as well as localizations of both TAMRA and Atto Rho6 G increase over 2 times.
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