Automating multimodal microscopy with NanoJ-Fluidics

Author:

Almada PedroORCID,Pereira Pedro M.ORCID,Culley SiânORCID,Caillol Ghislaine,Boroni-Rueda Fanny,Dix Christina L.,Laine Romain F.ORCID,Charras GuillaumeORCID,Baum BuzzORCID,Leterrier ChristopheORCID,Henriques RicardoORCID

Abstract

AbstractFluorescence microscopy can reveal all aspects of cellular mechanisms, from molecular details to dynamics, thanks to approaches such as super-resolution and live-cell imaging. Each of its modalities requires specific sample preparation and imaging conditions to obtain high-quality, artefact-free images, ultimately providing complementary information. Combining and multiplexing microscopy approaches is crucial to understand cellular events, but requires elaborate workflows involving multiple sample preparation steps. We present a robust fluidics approach to automate complex sequences of treatment, labelling and imaging of live and fixed cells. Our open-source NanoJ-Fluidics system is based on low-cost LEGO hardware controlled by ImageJ-based software and can be directly adapted to any microscope, providing easy-to-implement high-content, multimodal imaging with high reproducibility. We demonstrate its capacity to carry out complex sequences of experiments such as super-resolved live-to-fixed imaging to study actin dynamics; highly-multiplexed STORM and DNA-PAINT acquisitions of multiple targets; and event-driven fixation microscopy to study the role of adhesion contacts in mitosis.

Publisher

Cold Spring Harbor Laboratory

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