4.8 Article

Fast live-cell conventional fluorophore nanoscopy with ImageJ through super-resolution radial fluctuations

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NATURE COMMUNICATIONS
卷 7, 期 -, 页码 -

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NATURE PUBLISHING GROUP
DOI: 10.1038/ncomms12471

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资金

  1. Medical Research Council [MR/K015826/1]
  2. Biotechnology and Biological Sciences Research Council [BB/M022374/1]
  3. Engineering and Physical Sciences Research Council [EP/L504889/1]
  4. Marie-Curie grant [334303]
  5. European Research Council grant [337187]
  6. BBSRC [BB/M022374/1] Funding Source: UKRI
  7. MRC [MR/K015826/1] Funding Source: UKRI
  8. Biotechnology and Biological Sciences Research Council [BB/M022374/1] Funding Source: researchfish
  9. Engineering and Physical Sciences Research Council [1327852] Funding Source: researchfish
  10. Medical Research Council [MR/K015826/1] Funding Source: researchfish
  11. European Research Council (ERC) [337187] Funding Source: European Research Council (ERC)

向作者/读者索取更多资源

Despite significant progress, high-speed live-cell super-resolution studies remain limited to specialized optical setups, generally requiring intense phototoxic illumination. Here, we describe a new analytical approach, super-resolution radial fluctuations (SRRF), provided as a fast graphics processing unit-enabled ImageJ plugin. In the most challenging data sets for super-resolution, such as those obtained in low-illumination live-cell imaging with GFP, we show that SRRF is generally capable of achieving resolutions better than 150 nm. Meanwhile, for data sets similar to those obtained in PALM or STORM imaging, SRRF achieves resolutions approaching those of standard single-molecule localization analysis. The broad applicability of SRRF and its performance at low signal-to-noise ratios allows super-resolution using modern widefield, confocal or TIRF microscopes with illumination orders of magnitude lower than methods such as PALM, STORM or STED. We demonstrate this by super-resolution live-cell imaging over timescales ranging from minutes to hours.

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