Published September 1, 2020 | Version v1
Dataset Open

Comparing Lifeact and Phalloidin for super-resolution imaging of actin in fixed cells

  • 1. University of New Mexico
  • 2. The University of Texas Southwestern Medical Center
  • 3. University of Massachusetts Medical School
  • 4. Arizona State University
  • 5. University Medical Center Utrecht

Description

Visualizing actin filaments in fixed cells is of great interest for a variety of topics in cell biology such as cell division, cell movement, and cell signaling. We investigated the possibility of replacing phalloidin, the standard reagent for super-resolution imaging of F-actin in fixed cells, with the actin binding peptide `lifeact'. We compared the labels for use in single molecule based super-resolution microscopy, where AlexaFluor 647 labeled phalloidin was used in a (d)STORM modality and Atto 655 labeled lifeact was used in a single molecule imaging, reversible binding modality. We found that imaging with lifeact had a comparable resolution in reconstructed images and provided several advantages over phalloidin including lower costs, the ability to image multiple regions of interest on a coverslip without degradation, simplified sequential super-resolution imaging, and more continuous labeling of thin filaments.

Notes

All related notes are included in the methods section above or in README files included with files in the collection.

Funding provided by: NIH*
Crossref Funder Registry ID: http://dx.doi.org/10.13039/100000002
Award Number: 1R21EB019589

Funding provided by: NIH*
Crossref Funder Registry ID: http://dx.doi.org/10.13039/100000002
Award Number: P50GM085273

Funding provided by: NIH*
Crossref Funder Registry ID: http://dx.doi.org/10.13039/100000002
Award Number: R01GM109888

Funding provided by: NIH
Crossref Funder Registry ID: http://dx.doi.org/10.13039/100000002
Award Number: 1R21EB019589

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