Three-dimensional Super Resolution Microscopy of F-actin Filaments by Interferometric PhotoActivated Localization Microscopy (iPALM)

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Cited by 10

11:57 min

December 1st, 2016

10.3791/54774-v

December 1st, 2016

10.1K views

We present a protocol for the application of interferometric PhotoActivated Localization Microscopy (iPALM), a 3-dimensional single-molecule localization super resolution microscopy method, to the imaging of the actin cytoskeleton in adherent mammalian cells. This approach allows light-based visualization of nanoscale structural features that would otherwise remain unresolved by conventional diffraction-limited optical microscopy.

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iPALM Microscopy

Chapters in this video

0:05

Title

0:55

Imaging Specimen Preparation

3:11

Sample Placement and iPALM Alignment

5:29

Calibration of the iPALM Setup

7:47

Data Acquisition

9:09

Results: Actin Cytoskeleton of Adherent Mammalian Cells Visualized by iPALM with Sub-20 nm Spatial Resolution in 3D

10:55

Conclusion

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