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Journal of Biomolecular Screening
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1087057106286210v1
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Article

Miniaturization and Validation of a Sensitive Multiparametric Cell-Based Assay for the Concomitant Detection of Microtubule-Destabilizing and Microtubule-Stabilizing Agents

Emilie Vassal1, Caroline Barette2, Xavier Fonrose3, Raphaël Dupont4, Emmanuelle Sans-Soleilhac5, Laurence Lafanechère6*

1 Université Joseph-Fourier, INSERM U366-CS/DRDC/CEA, Grenoble, Grenoble, France.
2 CEA, INSERM U366-CS/DRDC/CEA Grenoble, France.
3 Université Joseph-Fourier, INSERM U366-CS/DRDC/CEA, and Département de Biologie Intégrée, Grenoble, France.
4 Université Joseph-Fourier, Biopuces/DRDC/CEA, Grenoble, France.
5 INSERM, U366-CS/DRDC/CEA, Grenoble, France.
6 CNRS, INSERM U366-CS/DRDC/CEA, Grenoble, France.

* To whom correspondence should be addressed. E-mail: laurence.lafanechere{at}cea.fr.


   Abstract

The authors describe a cell-based assay for anti-microtubule compounds suitable for automation. This assay allows the identification, in a single screening campaign, of both microtubule-destabilizing and microtubule-stabilizing agents. Its rationale is based on the substrate properties of the tubulin-modifying enzymes involved in the tubulin tyrosination cycle. This cycle involves the removal of the C-terminal tyrosine of the tubulin {alpha}-subunit by an ill-defined tubulin carboxypeptidase and its readdition by tubulin tyrosine ligase. Because of the substrate properties of these enzymes, dynamic microtubules, sensitive to depolymerizing drugs, are composed of tyrosinated tubulin, whereas nondynamic, stabilized microtubules are composed of detyrosinated tubulin. Thus depolymerization or stabilization of the microtubule network can easily be detected with double-immunofluorescence staining using antibodies specific to tyrosinated and detyrosinated tubulin. The authors have scaled this assay to the 96-well plate format and adapted its process for an automated handling, including a readout using a microplate reader. They describe the different steps of this adaptation. This assay was validated using known compounds. This new cell-based assay represents an alternative to both global cytotoxicity assays and in vitro tubulin assembly assays commonly used for the detection of microtubule poisons.

Key Words: microtubules, tubulin posttranslational modifications, cell-based assay, anticancer drugs, high-content screening

First published on April 28, 2006, doi:10.1177/1087057106286210

Journal of Biomolecular Screening 2006;11:377.

A more recent version of this article appeared on June 1, 2006


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