Research Article

High-resolution 3-D imaging of living cells in suspension using confocal axial tomography

  1. Olivier Renaud1,
  2. Jose Viña2,
  3. Yong Yu3,
  4. Christophe Machu1,
  5. Alain Trouvé3,
  6. Hans Van der Voort2,
  7. Bernard Chalmond3,
  8. Spencer L. Shorte Dr.1,*

Article first published online: 16 NOV 2007

DOI: 10.1002/biot.200700188

Issue

Biotechnology Journal

Biotechnology Journal

Special Issue: Methods and Advances in Biotech

Volume 3, Issue 1, pages 53–62, January 2008

Additional Information

How to Cite

Renaud, O., Viña, J., Yu, Y., Machu, C., Trouvé, A., Van der Voort, H., Chalmond, B. and Shorte, S. L. (2008), High-resolution 3-D imaging of living cells in suspension using confocal axial tomography. Biotechnology Journal, 3: 53–62. doi: 10.1002/biot.200700188

Author Information

  1. 1

    Institut Pasteur, Plate-forme d'Imagerie Dynamique, Imagopole, Paris, France

  2. 2

    Scientific Volume Imaging, Hilversum, The Netherlands

  3. 3

    C.M.L.A, CNRS (UMR 8536), ENS-Cachan, Cachan, France

*Institut Pasteur, Plate-forme d'Imagerie Dynamique, Imagopole, 25–28 rue du Dr Roux, 75015 Paris, France, Fax: +33-1-4568-8949

Publication History

  1. Issue published online: 15 JAN 2008
  2. Article first published online: 16 NOV 2007
  3. Manuscript Accepted: 1 OCT 2007
  4. Manuscript Revised: 21 SEP 2007
  5. Manuscript Received: 14 AUG 2007

Funded by

  • Institut Pasteur, European Commission
  • Agence Nationale de la Recherche
  • La Région Ile-de-France

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Keywords:

  • 3-D reconstruction;
  • Deconvolution;
  • Dielectric field caging;
  • Flow cytometry;
  • Micro-rotation

Abstract

Conventional flow cytometry (FC) methods report optical signals integrated from individual cells at throughput rates as high as thousands of cells per second. This is further combined with the powerful utility to subsequently sort and/or recover the cells of interest. However, these methods cannot extract spatial information. This limitation has prompted efforts by some commercial manufacturers to produce state-of-the-art commercial flow cytometry systems allowing fluorescence images to be recorded by an imaging detector. Nonetheless, there remains an immediate and growing need for technologies facilitating spatial analysis of fluorescent signals from cells maintained in flow suspension. Here, we report a novel methodological approach to this problem that combines micro-fluidic flow, and microelectrode dielectric-field control to manipulate, immobilize and image individual cells in suspension. The method also offers unique possibilities for imaging studies on cells in suspension. In particular, we report the system's immediate utility for confocal “axial tomography” using micro-rotation imaging and show that it greatly enhances 3-D optical resolution compared with conventional light reconstruction (deconvolution) image data treatment. That the method we present here is relatively rapid and lends itself to full automation suggests its eventual utility for 3-D imaging cytometry.

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