EphB receptor tyrosine kinases control morphological development of the ventral midbrain

EphB receptor tyrosine kinases and ephrin-B ligands regulate several types of cell–cell interactions during brain development, generally by modulating the cytoskeleton. EphB/ephrinB genes are expressed in the developing neural tube of early mouse embryos with distinct overlapping expression in the v...

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Bibliographic Details
Published in:Mechanisms of development 2005-04, Vol.122 (4), p.501-512
Main Authors: Altick, Amy L., Dravis, Christopher, Bowdler, Tracey, Henkemeyer, Mark, Mastick, Grant S.
Format: Article
Language:English
Subjects:
Animals
Body Patterning
Cell Proliferation
Development
Eph
EphB2
EphB3
Ephrin
Ephrin-B3
Gene Expression Regulation, Developmental - genetics
Mesencephalon - embryology
Mesencephalon - metabolism
Mice
Midbrain
Morphology
Mutation - genetics
Neural tube
Neuroepithelium
Receptor, EphB2 - deficiency
Receptor, EphB2 - genetics
Receptor, EphB2 - metabolism
Receptor, EphB3 - deficiency
Receptor, EphB3 - genetics
Receptor, EphB3 - metabolism
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Summary:EphB receptor tyrosine kinases and ephrin-B ligands regulate several types of cell–cell interactions during brain development, generally by modulating the cytoskeleton. EphB/ephrinB genes are expressed in the developing neural tube of early mouse embryos with distinct overlapping expression in the ventral midbrain. To test EphB function in midbrain development, mouse embryos compound homozygous for mutations in the EphB2 and EphB3 receptor genes were examined for early brain phenotypes. These mutants displayed a morphological defect in the ventral midbrain, specifically an expanded ventral midline evident by embryonic day E9.5–10.5, which formed an abnormal protrusion into the cephalic flexure. The affected area was comprised of cells that normally express EphB2 and ephrin-B3. A truncated EphB2 receptor caused a more severe phenotype than a null mutation, implying a dominant negative effect through interference with EphB forward (intracellular) signaling. In mutant embryos, the overall number, size, and identity of the ventral midbrain cells were unaltered. Therefore, the defect in ventral midline morphology in the EphB2; EphB3 compound mutant embryos appears to be caused by cellular changes that thin the tissue, forcing a protrusion of the ventral midline into the cephalic space. Our data suggests a role for EphB signaling in morphological organization of specific regions of the developing neural tube.
ISSN:0925-4773
1872-6356
DOI:10.1016/j.mod.2004.11.013