Gap junctional intercellular communication capacity by gap-FRAP technique: A comparative study

Muriel Abbaci, Muriel Barberi-Heyob, Jean René Stines, Walter Blondel, Dominique Dumas, François Guillemin, Jacques Didelon

Résultats de recherche: Contribution à un journalArticleRevue par des pairs

54 Citations (Scopus)

Résumé

Gap junctions play an important role in vital functions, including the regulation of cell growth and cell differentiation. Connexins 43 (Cx43) are the most widely expressed gap junction proteins. Cellular localization of phosphorylated Cx43 has been implicated in the capacity of gap junctional intercellular communication (GJIC). To follow the functionality of GJIC of different cell types, in monolayer cultures, characterized by different patterns of phosphorylated Cx43, we used a fluorescence recovery after photobleaching (FRAP) technique, and compared two tracers, 5(6)-carboxyfluorescein diacetate (CFDA) and calcein acetoxym ethyl ester (AM). The GJIC capacity was quantified by estimating fluorescence redistribution parameters. The functionality of GJIC was in relation with the staining localization of phosphorylated Cx43 to the cell-cell contact areas, corresponding to gap junctions between contacting cells. GJIC involvement in fluorescence restitution after photobleaching was checked by a gap junction channel inhibition assay. We demonstrated that the choice of the dye did not significantly influence the fluorescence recovery percentages despite a cell line-dependent CFDA release, whereas it had an important impact on fluorescence kinetic profiles. This study reinforces the interest of the gap-FRAP approach to quantify modifications in the functionality of gap junctions and, above all, argues about the limits of CFDA for 3-D future approaches.

langue originaleAnglais
Pages (de - à)50-61
Nombre de pages12
journalBiotechnology Journal
Volume2
Numéro de publication1
Les DOIs
étatPublié - 1 janv. 2007
Modification externeOui

Contient cette citation