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Dev Biol
1988 Oct 01;1292:380-9. doi: 10.1016/0012-1606(88)90385-5.
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Expression of Epi 1, an epidermis-specific marker in Xenopus laevis embryos, is specified prior to gastrulation.
London C
,
Akers R
,
Phillips C
.
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The induction of morphologically observable neural structures occurs as the result of tissue interactions between chordamesoderm and overlying ectoderm beginning at gastrulation. Since the future dorsal, and hence neural, side of the embryo is determined around the time of fertilization, we questioned whether the presumptive neural epithelium might have received some developmental instructions prior to contact with the migrating chordamesoderm. Epi 1, a cell surface antigen present only on epidermal epithelium was used as a marker to determine when epithelial cells have been programmed to express (or not express) this epidermal-specific molecule. We find that ligated animal halves of precleavage embryos already contain all the information necessary for expression of Epi 1 at the appropriate developmental time (early neurula). By at least the eight-celled stage, the epithelial cells derived from ventral animal blastomeres are much better at expressing the Epi 1 antigen than their dorsal counterparts. We suggest that the mechanisms responsible for expression of the Epi 1 antigen are localized within the animal hemisphere prior to the onset of cleavage. By the third cleavage division, dorsal animal cells appear to have received information which inhibits the subsequent expression of this epidermal antigen.
FIG. 1. In viwo expression pattern of Epi 1. (a) Cross section through
an early neural plate (stage 13) embryo. NP, neural plate. (b) Wholemount
of the dorsal anterior portion of a stage 15 embryo. CG, cement
gland. (a) 67X. (b) 428X.
FIG. 2. Detection of Epi 1 expression in cultured explants. Early
stage blastomeres were removed and cultured until control embryos
reached midneurula when they were fixed and assayed for Epi 1
expression. (a) Whole-mount stain of a cultured explant of the four
animal hemisphere blastomeres removed at the eight-cell stage. (b)
Whole-mount stain of the four vegetal blastomeres explanted at the
eight-cell stage and cultured to the equivalent of midneurula. (a)
168X. (b) 150x.
FIG. 3. The animal half of a precleavage embryo ligated free of the
vegetal half, cultured, and stained for the presence of Epi 1. 150x.
FIG. 4. Whole mounts of explants removed at midblastula (a) and
early gastrula (b), cultured until control embryos reached midneurula,
and stained for the presence of the Epi 1 antigen. The boundaries
between areas expressing or not expressing Epi 1 become sharper
when the cells are explanted later in development. (a) 150X. (b) 300X.
FIG. 5. A cultured, stained explant containing cells from the marginal
zone of the embryo. The area of non-Epi 1 expression normally
resides near the base of the protrusion. 150X.
FIG. 6. A whole-mount staining of a single cultured ventral animal
cell removed at the eight-cell stage. All ventral cell cultures show
nearly homogeneous expression of the Epi 1 antigen. 162X.
FIG. 7. Whole-mount staining of 40 cultured animal caps of uv-irradiated
embryos. Ninety percent of the stage 10 explanted caps expressed
the Epi 1 antigen completely (a). Four cultured explants
showed the same pattern of partial expression as observed from nonirradiated
stage 10 explants.
