Automating multimodal microscopy with NanoJ-Fluidics

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Pedro Almada Pedro M Pereira Siân Culley Ghislaine Caillol Fanny Boroni-Rueda Christina Dix Guillaume Charras Buzz Baum Romain F Laine Christophe Leterrier Ricardo Henriques
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Abstract

Combining and multiplexing microscopy approaches is crucial to understand cellular events, but requires elaborate workflows. Here, we present a robust, open-source approach for treating, labelling and imaging live or fixed cells in automated sequences. NanoJ-Fluidics is based on low-cost Lego hardware controlled by ImageJ-based software, making high-content, multimodal imaging easy to implement on any microscope with high reproducibility. We demonstrate its capacity on event-driven, super-resolved live-to-fixed and multiplexed STORM/DNA-PAINT experiments.

Journal details

Journal Nature Communications
Volume 10
Issue number 1
Pages 1223
Publication date

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Publisher website (DOI) 10.1038/s41467-019-09231-9
Europe PubMed Central 30874553
Pubmed 30874553

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