Literature DB >> 22735543

STED microscopy with optimized labeling density reveals 9-fold arrangement of a centriole protein.

Lana Lau1, Yin Loon Lee, Steffen J Sahl, Tim Stearns, W E Moerner.   

Abstract

Super-resolution fluorescence microscopy can achieve resolution beyond the optical diffraction limit, partially closing the gap between conventional optical imaging and electron microscopy for elucidation of subcellular architecture. The centriole, a key component of the cellular control and division machinery, is 250 nm in diameter, a spatial scale where super-resolution methods such as stimulated emission depletion (STED) microscopy can provide previously unobtainable detail. We use STED with a resolution of 60 nm to demonstrate that the centriole distal appendage protein Cep164 localizes in nine clusters spaced around a ring of ∼300 nm in diameter, and quantify the influence of the labeling density in STED immunofluorescence microscopy. We find that the labeling density dramatically influences the observed number, size, and brightness of labeled Cep164 clusters, and estimate the average number of secondary antibody labels per cluster. The arrangements are morphologically similar in centrioles of both proliferating cells and differentiated multiciliated cells, suggesting a relationship of this structure to function. Our STED measurements in single centrioles are consistent with results obtained by electron microscopy, which involve ensemble averaging or very different sample preparation conditions, suggesting that we have arrived at a direct measurement of a centriole protein by careful optimization of the labeling density.
Copyright © 2012 Biophysical Society. Published by Elsevier Inc. All rights reserved.

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Year:  2012        PMID: 22735543      PMCID: PMC3379620          DOI: 10.1016/j.bpj.2012.05.015

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  47 in total

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Journal:  Nat Methods       Date:  2008-04-13       Impact factor: 28.547

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  38 in total

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Review 4.  Applications of STED fluorescence nanoscopy in unravelling nanoscale structure and dynamics of biological systems.

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Journal:  J Biosci       Date:  2018-07       Impact factor: 1.826

5.  Determining the Spatial Relationship of Membrane-Bound Aquaporin-4 Autoantibodies by STED Nanoscopy.

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6.  Super-Resolution Microscopy and Single-Protein Tracking in Live Bacteria Using a Genetically Encoded, Photostable Fluoromodule.

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7.  Super-resolution microscopy reveals that disruption of ciliary transition-zone architecture causes Joubert syndrome.

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Review 8.  Subdiffractive microscopy: techniques, applications, and challenges.

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9.  Hybrid Structured Illumination Expansion Microscopy Reveals Microbial Cytoskeleton Organization.

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Review 10.  Light Microscopy of Mitochondria at the Nanoscale.

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Journal:  Annu Rev Biophys       Date:  2020-02-24       Impact factor: 12.981

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