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

Renaud, Olivier; Viña, José; Yu, Yong; Machu, Christophe; Trouvé, Alain; Voort, Hans van der; Chalmond, Bernard; Shorte, Spencer

doi:10.1002/biot.200700188

Cited by 23 publications

(26 citation statements)

References 27 publications

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“…We thus explored the effect of Nef on T-cell shape in unfixed, living cells. We used a novel methodological approach, which allows visualization and axial tomography of living cells in suspension (41). A single living cell is immobilized in a cage by an electric field and then analyzed by high-resolution confocal microscopy.…”

Section: Resultsmentioning

confidence: 99%

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HIV-1 Nef Inhibits Ruffles, Induces Filopodia, and Modulates Migration of Infected Lymphocytes

Nobile

Rudnicka

Hasan

et al. 2010

J Virol

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The HIV-1 Nef protein is a pathogenic factor modulating the behavior of infected cells. Nef induces actin cytoskeleton changes and impairs cell migration toward chemokines. We further characterized the morphology, cytoskeleton dynamics, and motility of HIV-1-infected lymphocytes. By using scanning electron microscopy, confocal immunofluorescence microscopy, and ImageStream technology, which combines flow cytometry and automated imaging, we report that HIV-1 induces a characteristic remodeling of the actin cytoskeleton. In infected lymphocytes, ruffle formation is inhibited, whereas long, thin filopodium-like protrusions are induced. Cells infected with HIV with nef deleted display a normal phenotype, and Nef expression alone, in the absence of other viral proteins, induces morphological changes. We also used an innovative imaging system to immobilize and visualize living individual cells in suspension. When combined with confocal "axial tomography," this technique greatly enhances three-dimensional optical resolution. With this technique, we confirmed the induction of long filopodium-like structures in unfixed Nef-expressing lymphocytes. The cytoskeleton reorganization induced by Nef is associated with an important impairment of cell movements. The adhesion and spreading of infected cells to fibronectin, their spontaneous motility, and their migration toward chemokines (CXCL12, CCL3, and CCL19) were all significantly decreased. Therefore, Nef induces complex effects on the lymphocyte actin cytoskeleton and cellular morphology, which likely impacts the capacity of infected cells to circulate and to encounter and communicate with bystander cells.

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Section: Resultsmentioning

confidence: 99%

“…Cells were resuspended in Cytocon buffer II (Evotec Technologies/Perkin Elmer) at a final concentration of 10 6 cells/ml. Analysis was performed on single cells immobilized in a cage by a dielectric field and then visualized by high-resolution confocal microscopy as described previously (41).…”

Section: Methodsmentioning

confidence: 99%

HIV-1 Nef Inhibits Ruffles, Induces Filopodia, and Modulates Migration of Infected Lymphocytes

Nobile

Rudnicka

Hasan

et al. 2010

J Virol

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“…The image resolution for both z-stack slice and micro-rotation slice is set as 127 nm. More detail about image acquisition is found in [4,5]. Fig.…”

Section: Methodsmentioning

confidence: 99%

A Fast 3D Volume Reconstruction for Confocal Micro-rotation Cell Imaging

Trouvé

Chalmond

2008

2008 International Conference on BioMedical Engineering and Informatics

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We propose a fast reconstruction algorithm for nonadherent living cell images from micro-rotational confocal microscopy. This procedure is called bi-protocol. Its key point consists in coupling micro-rotation data and conventional z-stack. Doing so, the estimation of the microrotation slice positions becomes a slice-to-volume registration allowing to reduce drastically the computing time. The validation of our procedure is performed on real data which gives significant improvement compared with the conventional z-stacking imaging.

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“…In (Heintzmann & Cremer, ) tomography was applied to confocal fluorescence microscopy, by first obtaining several 3D projections by physical rotation of the sample and then combining the projections to a single sharp image. A similar technique was applied to living cells in (Renaud et al ., ). In (Swoger et al ., ; Verveer et al ., ; Krzic, ) the tomography approach to improve apparent axial resolution was applied to light‐sheet microscopy.…”

Section: Introductionmentioning

confidence: 99%

A software tool for tomographic axial superresolution in STED microscopy

Koho

Deguchi

Hänninen

2015

Journal of Microscopy

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A method for generating three-dimensional tomograms from multiple three-dimensional axial projections in STimulated Emission Depletion (STED) superresolution microscopy is introduced. Our STED< method, based on the use of a micromirror placed on top of a standard microscopic sample, is used to record a three-dimensional projection at an oblique angle in relation to the main optical axis. Combining the STED< projection with the regular STED image into a single view by tomographic reconstruction, is shown to result in a tomogram with three-to-four-fold improved apparent axial resolution. Registration of the different projections is based on the use of a mutual-information histogram similarity metric. Fusion of the projections into a single view is based on Richardson-Lucy iterative deconvolution algorithm, modified to work with multiple projections. Our tomographic reconstruction method is demonstrated to work with real biological STED superresolution images, including a data set with a limited signal-to-noise ratio (SNR); the reconstruction software (SuperTomo) and its source code will be released under BSD open-source license.

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

Cited by 23 publications

References 27 publications

HIV-1 Nef Inhibits Ruffles, Induces Filopodia, and Modulates Migration of Infected Lymphocytes

HIV-1 Nef Inhibits Ruffles, Induces Filopodia, and Modulates Migration of Infected Lymphocytes

A Fast 3D Volume Reconstruction for Confocal Micro-rotation Cell Imaging

A software tool for tomographic axial superresolution in STED microscopy

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