Literature DB >> 27854362

A Bayesian cluster analysis method for single-molecule localization microscopy data.

Juliette Griffié1, Michael Shannon1, Claire L Bromley2, Lies Boelen3, Garth L Burn1, David J Williamson1, Nicholas A Heard4, Andrew P Cope5, Dylan M Owen1, Patrick Rubin-Delanchy6.   

Abstract

Cell function is regulated by the spatiotemporal organization of the signaling machinery, and a key facet of this is molecular clustering. Here, we present a protocol for the analysis of clustering in data generated by 2D single-molecule localization microscopy (SMLM)-for example, photoactivated localization microscopy (PALM) or stochastic optical reconstruction microscopy (STORM). Three features of such data can cause standard cluster analysis approaches to be ineffective: (i) the data take the form of a list of points rather than a pixel array; (ii) there is a non-negligible unclustered background density of points that must be accounted for; and (iii) each localization has an associated uncertainty in regard to its position. These issues are overcome using a Bayesian, model-based approach. Many possible cluster configurations are proposed and scored against a generative model, which assumes Gaussian clusters overlaid on a completely spatially random (CSR) background, before every point is scrambled by its localization precision. We present the process of generating simulated and experimental data that are suitable to our algorithm, the analysis itself, and the extraction and interpretation of key cluster descriptors such as the number of clusters, cluster radii and the number of localizations per cluster. Variations in these descriptors can be interpreted as arising from changes in the organization of the cellular nanoarchitecture. The protocol requires no specific programming ability, and the processing time for one data set, typically containing 30 regions of interest, is ∼18 h; user input takes ∼1 h.

Mesh:

Year:  2016        PMID: 27854362     DOI: 10.1038/nprot.2016.149

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  57 in total

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Journal:  Immunity       Date:  2011-11-04       Impact factor: 31.745

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Authors:  Dylan M Owen; Carles Rentero; Jérémie Rossy; Astrid Magenau; David Williamson; Macarena Rodriguez; Katharina Gaus
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Authors:  Dylan M Owen; David J Williamson; Astrid Magenau; Katharina Gaus
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Journal:  Nat Neurosci       Date:  2014-12-08       Impact factor: 24.884

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  14 in total

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4.  Parameter-free molecular super-structures quantification in single-molecule localization microscopy.

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Review 5.  Transcriptional Regulation of T-Cell Lipid Metabolism: Implications for Plasma Membrane Lipid Rafts and T-Cell Function.

Authors:  George A Robinson; Kirsty E Waddington; Ines Pineda-Torra; Elizabeth C Jury
Journal:  Front Immunol       Date:  2017-11-24       Impact factor: 7.561

6.  3D Bayesian cluster analysis of super-resolution data reveals LAT recruitment to the T cell synapse.

Authors:  Juliette Griffié; Leigh Shlomovich; David J Williamson; Michael Shannon; Jesse Aaron; Satya Khuon; Garth L Burn; Lies Boelen; Ruby Peters; Andrew P Cope; Edward A K Cohen; Patrick Rubin-Delanchy; Dylan M Owen
Journal:  Sci Rep       Date:  2017-06-22       Impact factor: 4.379

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8.  Mapping molecular assemblies with fluorescence microscopy and object-based spatial statistics.

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Journal:  Nat Commun       Date:  2018-02-15       Impact factor: 14.919

9.  Galectin-9 binds IgM-BCR to regulate B cell signaling.

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10.  Super Resolution Network Analysis Defines the Molecular Architecture of Caveolae and Caveolin-1 Scaffolds.

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