4.3 Review

Three-dimensional imaging flow cytometry through light-sheet fluorescence microscopy

Journal

CYTOMETRY PART A
Volume 91A, Issue 2, Pages 144-151

Publisher

WILEY-BLACKWELL
DOI: 10.1002/cyto.a.23046

Keywords

light sheet fluorescence microscopy; high throughput microscopy; imaging flow cytometry

Funding

  1. Fundacao para a Ciencia e Tecnologia, Portugal [SFRH/BPD/80717/2011, EXPL/BBBIMG/0363/2013]
  2. MINECO/FEDER project [BIO2014-59614-JIN, RYC-2015-17935]
  3. Fundação para a Ciência e a Tecnologia [SFRH/BPD/80717/2011] Funding Source: FCT

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Flow cytometry is the tool of choice for high-speed acquisition and analysis of large cell populations, with the tradeoff of lacking intracellular spatial information. Although in the last decades flow cytometry systems that can actually acquire two-dimensional spatial information were developed, some of the limitations remained though, namely constrains related to sample size and lack of depth or dynamic information. The combination of fluidics and light-sheet illumination has the potential to address these limitations. By having cells travelling with the flowing sheath one can, in a controlled fashion, force them at constant speed through the light-sheet enabling the synchronized acquisition of several optical sections, that is, three-dimensional imaging. This approach has already been used for imaging cellular spheroids, plankton, and zebra-fish embryos. In this review, we discuss the known solutions and standing challenges of performing three-dimensional high-throughput imaging of multicellular biological models using fluidics, while retaining cell and organelle-level resolution. (c) 2017 International Society for Advancement of Cytometry

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