Tight junction formation in early Xenopus laevis embryos: identification and ultrastructural characterization of junctional crests and junctional vesicles

How tight junctions (TJ) form during early amphibian embryogenesis is still an open question. We used time-lapse video microscopy, scanning electron microscopy (SEM), TEM and freeze-fracture to gain new insight into TJ biogenesis in early clevages of Xenopus laevis. Video analysis suggests three pha...

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Bibliographic Details
Published in:Cell and tissue research 2007-11, Vol.330 (2), p.247-256
Main Authors: Cardellini, Pietro, Cirelli, Alessandro, Citi, Sandra
Format: Article
Language:English
Subjects:
Animals
Cell Communication
Cell Differentiation - physiology
Cell Membrane - metabolism
Cell Membrane - ultrastructure
Cell Surface Extensions - metabolism
Cell Surface Extensions - ultrastructure
Cellular biology
Cytoplasmic Vesicles - metabolism
Cytoplasmic Vesicles - ultrastructure
Embryo, Nonmammalian - embryology
Embryo, Nonmammalian - metabolism
Embryo, Nonmammalian - ultrastructure
Female
Male
Microscopy
Microscopy, Electron, Scanning
Microscopy, Electron, Transmission
Molecular biology
Reptiles & amphibians
Tight Junctions - metabolism
Tight Junctions - ultrastructure
Xenopus laevis - embryology
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Summary:How tight junctions (TJ) form during early amphibian embryogenesis is still an open question. We used time-lapse video microscopy, scanning electron microscopy (SEM), TEM and freeze-fracture to gain new insight into TJ biogenesis in early clevages of Xenopus laevis. Video analysis suggests three phases in junction formation between blastomeres. A first "waiting" phase, where new unpigmented lateral membranes are generated. A second "mixing" phase, where the unpigmented lateral membrane is separated from the pigmented apical membrane by an area showing a limited degree of intermingling of cortical pigment. And a third "sealing" phase, characterized by the formation of cingulin-containing boundaries between membrane domains, and their rapid directional adhesion in a zipper-like fashion. By SEM, we characterized these boundaries ("junctional crests", JC) as arrays of villiform protrusions at the border between old and new membranes. In the 2-cell embryo, JC are deeply located, and thus not visible at the surface, but they become increasingly more superficial as cleavages progress. After adjacent blastomeres have adhered to each other, fractured JC display linear arrays of junctional vesicles (JV) of 1-3 mum diameter. TEM analysis shows that JV are symmetrically located near the apposed membranes of adjacent blastomeres, and that the membranes near the JV display focal sites of intimate contact, typical of TJ. Freeze-fracture analysis confirms that intramembrane fibrils, typical of TJ, are present at adhesion sites. We conclude that TJ are formed following the sealing of JC, through the recruitment, sorting and assembly of membrane and cytoplasmic proteins at or near JV.
ISSN:0302-766X
1432-0878
DOI:10.1007/s00441-007-0472-9