Comparing lifeact and phalloidin for superresolution imaging of actin in fixed cells

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Abstract

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 dSTORM 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.

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Mazloom-Farsibaf, H., Farzam, F., Fazel, M., Wester, M. J., Meddens, M. B. M., & Lidke, K. A. (2021). Comparing lifeact and phalloidin for superresolution imaging of actin in fixed cells. PLoS ONE, 16(1 January). https://doi.org/10.1371/journal.pone.0246138

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