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Literature DB >> 28580376

Reversible Cryo-arrests of Living Cells to Pause Molecular Movements for High-resolution Imaging.

Jan Huebinger¹, Martin E Masip¹, Jens Christmann^1,2, Frank Wehner¹, Philippe I H Bastiaens^1,2.

Abstract

Fluorescence live-cell imaging by single molecule localization microscopy (SMLM) or fluorescence lifetime imaging microscopy (FLIM) in principle allows for the spatio-temporal observation of molecular patterns in individual, living cells. However, the dynamics of molecules within cells hamper their precise observation. We present here a detailed protocol for consecutive cycles of reversible cryo-arrest of living cells on a microscope that allows for a precise determination of the evolution of molecular patterns within individual living cells. The usefulness of this approach has been demonstrated by observing ligand-induced clustering of receptor tyrosine kinases as well as their activity patterns by SMLM and FLIM (Masip et al., 2016).

Entities: Chemical

Keywords: Cryo-arrest; FLIM; Fixation; Single molecule localization; Superresolution

Year: 2017 PMID： 28580376 PMCID： PMC5450929 DOI： 10.21769/BioProtoc.2236

Source DB: PubMed Journal: Bio Protoc ISSN： 2331-8325

18 in total

1. Imaging phosphorylation dynamics of the epidermal growth factor receptor.

Authors: Martin Offterdinger; Virginie Georget; Andreas Girod; Philippe I H Bastiaens
Journal: J Biol Chem Date: 2004-06-23 Impact factor: 5.157

2. Membrane molecules mobile even after chemical fixation.

Authors: Kenji A K Tanaka; Kenichi G N Suzuki; Yuki M Shirai; Shusaku T Shibutani; Manami S H Miyahara; Hisae Tsuboi; Miyako Yahara; Akihiko Yoshimura; Satyajit Mayor; Takahiro K Fujiwara; Akihiro Kusumi
Journal: Nat Methods Date: 2010-10-03 Impact factor: 28.547

Reversible Cryo-arrests of Living Cells to Pause Molecular Movements for High-resolution Imaging.

1. Imaging phosphorylation dynamics of the epidermal growth factor receptor.

2. Membrane molecules mobile even after chemical fixation.

3. Oligomerization of the EGF receptor investigated by live cell fluorescence intensity distribution analysis.

4. Global analysis of time correlated single photon counting FRET-FLIM data.

Review 5. Origins of regulated cell-to-cell variability.

6. Cholesterol dictates the freedom of EGF receptors and HER2 in the plane of the membrane.

7. Single-molecule diffusion study of activated EGFR implicates its endocytic pathway.

8. Reversible cryo-arrest for imaging molecules in living cells at high spatial resolution.

9. Conformational coupling across the plasma membrane in activation of the EGF receptor.

10. Direct Measurement of Water States in Cryopreserved Cells Reveals Tolerance toward Ice Crystallization.

1. Quantification of protein mobility and associated reshuffling of cytoplasm during chemical fixation.