4.8 Article

Fix Your Membrane Receptor Imaging: Actin Cytoskeleton and CD4 Membrane Organization Disruption by Chemical Fixation

Journal

FRONTIERS IN IMMUNOLOGY
Volume 10, Issue -, Pages -

Publisher

FRONTIERS MEDIA SA
DOI: 10.3389/fimmu.2019.00675

Keywords

super-resolution imaging; CD4; actin cortex; fixation; artefact analysis

Categories

Funding

  1. UK Biotechnology and Biological Sciences Research Council [BB/M022374/1, BB/P027431/1, BB/R000697/1, BB/S507532/1]
  2. UK Medical Research Council [MR/K015826/1]
  3. Wellcome Trust [203276/Z/16/Z]
  4. MRC Programme Grant [MC_UU12018/7, MC_U12016/1]
  5. European Research Council [649101-UbiProPox]
  6. European Union [750673]
  7. Commonwealth scholarship
  8. UK government
  9. Marie Curie Actions (MSCA) [750673] Funding Source: Marie Curie Actions (MSCA)
  10. BBSRC [BB/R000697/1, BB/M022374/1, BB/P027431/1] Funding Source: UKRI
  11. MRC [MC_UU_00012/1, MR/K015826/1] Funding Source: UKRI

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Single-molecule localization microscopy (SMLM) techniques allow near molecular scale resolution (similar to 20 nm) as well as precise and robust analysis of protein organization at different scales. SMLM hardware, analytics and probes have been the focus of a variety of studies and are now commonly used in laboratories across the world. Protocol reliability and artifact identification are increasingly seen as important aspects of super-resolution microscopy. The reliability of these approaches thus requires in-depth evaluation so that biological findings are based on solid foundations. Here we explore how different fixation approaches that disrupt or preserve the actin cytoskeleton affect membrane protein organization. Using CD4 as a model, we show that fixation-mediated disruption of the actin cytoskeleton correlates with changes in CD4 membrane organization. We highlight how these artifacts are easy to overlook and how careful sample preparation is essential for extracting meaningful results from super-resolution microscopy.

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