Structure and dynamics of multicellular assemblies measured by coherent light scattering

Benjamin Brunel; Carles Blanch; Aurélien Gourrier; Vanni Petrolli; Antoine Delon; Jean-François Joanny; Rémi Carminati; Romain Pierrat; Giovanni Cappello

doi:10.1088/1367-2630/aa7b0f

New Journal of Physics (Jan 2017)

Structure and dynamics of multicellular assemblies measured by coherent light scattering

Benjamin Brunel,
Carles Blanch,
Aurélien Gourrier,
Vanni Petrolli,
Antoine Delon,
Jean-François Joanny,
Rémi Carminati,
Romain Pierrat,
Giovanni Cappello

Affiliations

Benjamin Brunel: Université Grenoble Alpes , Laboratoire Interdisciplinaire de Physique, CNRS, F-38000 Grenoble, France
Carles Blanch: Institut Curie, CNRS, Université P. et M. Curie , UMR 168, F-75231 Paris, France
Aurélien Gourrier: ORCiD; Université Grenoble Alpes , Laboratoire Interdisciplinaire de Physique, CNRS, F-38000 Grenoble, France
Vanni Petrolli: Université Grenoble Alpes , Laboratoire Interdisciplinaire de Physique, CNRS, F-38000 Grenoble, France
Antoine Delon: Université Grenoble Alpes , Laboratoire Interdisciplinaire de Physique, CNRS, F-38000 Grenoble, France
Jean-François Joanny: Institut Curie, CNRS, Université P. et M. Curie , UMR 168, F-75231 Paris, France; ESPCI Paris, PSL Research University , 10 rue Vauquelin, F-75005 Paris, France
Rémi Carminati: ESPCI Paris, PSL Research University , CNRS, Institut Langevin, 1 rue Jussieu, F-75005 Paris, France
Romain Pierrat: ESPCI Paris, PSL Research University , CNRS, Institut Langevin, 1 rue Jussieu, F-75005 Paris, France
Giovanni Cappello: Université Grenoble Alpes , Laboratoire Interdisciplinaire de Physique, CNRS, F-38000 Grenoble, France

DOI: https://doi.org/10.1088/1367-2630/aa7b0f
Journal volume & issue: Vol. 19, no. 7
p. 073033

Abstract

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Determining the structure and the internal dynamics of tissues is essential to understand their functional organization. Microscopy allows for monitoring positions and trajectories of every single cell. Those data are useful to extract statistical observables, such as intercellular distance, tissue symmetry and anisotropy, and cell motility. However, this procedure requires a large and supervised computational effort. In addition, due to the large cross-section of cells, the light scattering limits the use of microscopy to relatively thin samples. As an alternative approach, we propose to take advantage of light scattering and to analyze the dynamical diffraction pattern produced by a living tissue illuminated with coherent light. In this article, we illustrate with a few examples that supra-cellular structures produce an exploitable diffraction signal. From the diffraction signal, we deduce the mean distance between cells, the anisotropy of the supra-cellular organization and, from its fluctuations, the mean speed of moving cells. This easy to implement technique considerably reduces analysis time, allowing real time monitoring.

Published in New Journal of Physics

ISSN: 1367-2630 (Online)
Publisher: IOP Publishing
Country of publisher: United Kingdom
LCC subjects: Science: Physics
Website: https://iopscience.iop.org/journal/1367-2630

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