Time-lapse Contact Microscopy of Cell Cultures Based on Non-coherent Illumination

Overview

Journal Sci Rep

Specialty Science

Date 2015 Oct 14

PMID 26459014

Citations 2

Authors

Marion Gabriel

Dorothee Balle

Stephanie Bigault

Cyrille Pornin

Stephane Getin

Francois Perraut

Marc R Block

Francois Chatelain

Nathalie Picollet-Dhahan

Xavier Gidrol

Vincent Haguet

Affiliations

Soon will be listed here.

Abstract

Video microscopy offers outstanding capabilities to investigate the dynamics of biological and pathological mechanisms in optimal culture conditions. Contact imaging is one of the simplest imaging architectures to digitally record images of cells due to the absence of any objective between the sample and the image sensor. However, in the framework of in-line holography, other optical components, e.g., an optical filter or a pinhole, are placed underneath the light source in order to illuminate the cells with a coherent or quasi-coherent incident light. In this study, we demonstrate that contact imaging with an incident light of both limited temporal and spatial coherences can be achieved with sufficiently high quality for most applications in cell biology, including monitoring of cell sedimentation, rolling, adhesion, spreading, proliferation, motility, death and detachment. Patterns of cells were recorded at various distances between 0 and 1000 μm from the pixel array of the image sensors. Cells in suspension, just deposited or at mitosis focalise light into photonic nanojets which can be visualised by contact imaging. Light refraction by cells significantly varies during the adhesion process, the cell cycle and among the cell population in connection with every modification in the tridimensional morphology of a cell.

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