Abstract
BackgroundEmbryo implantation requires that uterine epithelium develops competence to bind trophoblast to its apical (free) poles. This essential element of uterine receptivity seems to depend on a destabilisation of the apico-basal polarity of endometrial epithelium. Accordingly, a reorganisation of the actin cytoskeleton regulated by the small GTPase RhoA plays an important role in human uterine epithelial RL95-2 cells for binding of human trophoblastoid JAR cells. We now obtained new insight into trophoblast binding using human uterine epithelial Ishikawa cells.MethodsPolarity of Ishikawa cells was investigated by electron microscopy, apical adhesiveness was tested by adhesion assay. Analyses of subcellular distribution of filamentous actin (F-actin) and RhoA in apical and basal cell poles were performed by confocal laser scanning microscopy (CLSM) with and without binding of JAR spheroids as well as with and without inhibition of small Rho GTPases by Clostridium difficile toxin A (toxin A). In the latter case, subcellular distribution of RhoA was additionally investigated by Western blotting.ResultsIshikawa cells express apical adhesiveness for JAR spheroids and moderate apico-basal polarity. Without contact to JAR spheroids, significantly higher signalling intensities of F-actin and RhoA were found at the basal as compared to the apical poles in Ishikawa cells. RhoA was equally distributed between the membrane fraction and the cytosol fraction. Levels of F-actin and RhoA signals became equalised in the apical and basal regions upon contact to JAR spheroids. After inhibition of Rho GTPases, Ishikawa cells remained adhesive for JAR spheroids, the gradient of fluorescence signals of F-actin and RhoA was maintained while the amount of RhoA was reduced in the cytosolic fraction with a comparable increase in the membrane fraction.ConclusionIshikawa cells respond to JAR contact as well as to treatment with toxin A with rearrangement of F-actin and small GTPase RhoA but seem to be able to modify signalling pathways in a way not elucidated so far in endometrial cells. This ability may be linked to the degree of polar organisation observed in Ishikawa cells indicating an essential role of cell phenotype modification in apical adhesiveness of uterine epithelium for trophoblast in vivo.
Highlights
Embryo implantation requires that uterine epithelium develops competence to bind trophoblast to its apical poles
We previously demonstrated that formation of stable cell-to-cell bonds depends in this model on RL95-2 cells' actin cytoskeleton (F-actin) and small GTPases of the Rho family, most likely RhoA
Data show that Ishikawa cells respond to JAR contact as well as to treatment with toxin A with rearrangement of Factin and a redistribution of the small GTPase RhoA
Summary
Embryo implantation requires that uterine epithelium develops competence to bind trophoblast to its apical (free) poles This essential element of uterine receptivity seems to depend on a destabilisation of the apico-basal polarity of endometrial epithelium. Organisation of the cell architecture and signalling systems seem to be changed [3,9,10,11,12,13,14,15,16] These modifications point to a reduction or destabilisation of apico-basal polarity of uterine epithelial cells in preparation for trophoblast adhesion during early embryo implantation [2,17,18,19]
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