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Fig. 2. Mis-expression of eng3 results in an anterior shift of the
position of the DMB. Mis-expression of 500 pg eng3 mRNA in one cell
at the two blastomere stage (A-D). The broken line indicates the midline; the
upper side is the control side (con) and the lower side is the injected side
(inj). At 1 ss, pax6.1 expression is strongly diminished in the
injected side (black arrowheads). The expression of otx2 is not
altered. To localize the experimental side, lacZ mRNA was co-injected
and detected with a secondary, FITC-coupled antibody (B). At 26hpf,
efna4 is suppressed at the injected side (C). The mis-expression of
eng3 results in an altered formation (n=36, out of 84) or in
a loss of the posterior commissure (n=23, out of 84; D, white
arrowheads). To follow the fate of small cell clones in
eng3-mRNA-injected embryos, caged fluorescein was co-injected with
lacZ-mRNA in control embryos or together with eng3-mRNA
(E-J). For this experiment, a microscope was used that was provided with an
nitrogen laser unit (E) and a grid (raster size 0.05 mm). At shield stage, the
embryos were orientated dorsal side up with the shield to the left. The
fluorescein dye was uncaged with a laser beam (365 nm) at the position of the
grid: x-axis, –4; y-axis, –3 (F). A picture of a
living embryo at shield stage was superimposed on a dark field picture to
visualize the clone, and a grid was overlaid. `sh' marks the position of the
shield. At 15 ss, the cell clones are visible in the eye or in the posterior
diencephalon visualized by a superimposed pseudo lateral picture of the same
living wild-type embryo with a darkfield-fluorescence picture (G). In situ
hybridization for pax6.1 expression on the same embryo shows that the
clone is located in the pax6.1-positive domain (encircled by red
dots, H). Small cell clones that were uncaged in embryos injected with 500 pg
eng3-mRNA are located in the pax6.1-negative region,
suggesting a transformation of cell identity (I,J). (K-M) Injection of
different amounts of eng3-mRNA (300 pg and 600 pg, indicated by the
red triangle below) show concentration-dependent reduction of pax6.1
expression and of the size of the eye anlage (arrowheads). After the injection
of 600 pg eng3-mRNA, the forebrain expression of pax6.1 is
completely abolished and the eye anlage was not detectable (M). DMB,
diencephalic-mesencephalic boundary; eye, eye anlage; hb, hindbrain; mb,
midbrain; PC, posterior commissure; sh, shield.
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10 cell wide gap is shown between the
expression domains (O,P). At 6 ss the gap increases in size to 20 cells (Q).
At 24hpf, the expression of fgf8 is refined to the posterior part of
the MHB (R). Arrowheads demarcate the gap between the expression domains of
pax6.1 and the indicated marker (D-R). Asterisks mark the
pax6.1 free territory (E,J,O). dd, dorsal diencephalon; eye, eye
anlage; fb, forebrain; fec, facial ectoderm; DMB, diencephalic-mesencephalic
boundary; mb, midbrain; MHB, midbrain-hindbrain boundary; ost, optic stalk;
PC, posterior commissures, somites per stage; tb, tailbud stage; tec, tectum
opticum. Percentage specifications are percent of epiboly indicated in the
figures.
-Phosphohistone 3 antibody and in situ hybridization with
pax6.1 probe of wild-type and eng2/eng3 morphant embryos at
the indicated stages (G-L). The expanded pax6.1 territory is marked
by red arrows. (M,N) In eng2/eng3 morphants Engrailed protein is not
detectable by the 
