First published online 29 August 2007
doi: 10.1242/dev.005868
Development 134, 3427-3436 (2007)
Published by The Company of Biologists 2007
A regulatory network involving Foxn4, Mash1 and delta-like 4/Notch1 generates V2a and V2b spinal interneurons from a common progenitor pool
Marta G. Del Barrio1,
Raquel Taveira-Marques1,
Yuko Muroyama2,*,
Dong-In Yuk2,
Shengguo Li3,
Mary Wines-Samuelson4,
Jie Shen4,
Hazel K. Smith1,
Mengqing Xiang3,
David Rowitch2,
and
William D. Richardson1,
1 Wolfson Institute for Biomedical Research and Department of Biology,
University College London, Gower Street, London WC1E 6BT, UK.
2 Department of Pediatric Oncology, Dana-Farber Cancer Institute, Dana 640D, 44
Binney Street, Boston, MA 02115, USA.
3 Center for Advanced Biotechnology and Medicine, UMDNJ-Robert Wood Johnson
Medical School, 679 Hoes Lane, Piscataway, NJ 08854, USA.
4 Center for Neurologic Diseases, Brigham and Women's Hospital, Program in
Neuroscience, Harvard Medical School, 77 Avenue Louis Pasteur, Boston, MA
02115, USA.
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Fig. 1. Foxn4 is sufficient to induce V2b and suppress V2a
interneurons. In this and subsequent figure legends, consecutive sections
are labelled A,A',A'' etc, and different fluorescence channels of
the same micrograph are labelled A,A1,A2 etc. (A-J') Chick
embryos were electroporated at st12-14 with
ß-actin-Foxn4-IRES-GFP and harvested after 24 or 48 hours.
Expression of the vector was confirmed by in situ hybridisation (ISH) for
Foxn4 or immunolabelling for GFP (panels marked Foxn4-GFP). Foxn4
induces robust ectopic expression of Gata2 at either 24 or 48 hours
post-electroporation (A',E',F). Foxn4 induced Gata3
(D',I') and Scl (J', note ventral induction,
arrowhead) only after 48 hours. Foxn4 does not induce ectopic expression of
Chx10 (B',G,H) or Lhx3 (C',E''). On the contrary,
Foxn4 represses endogenous Chx10 in the p2 domain (G,H).
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Fig. 2. Foxn4 lies upstream of Scl in V2b interneuron
development. (A) Double ISH for Scl (green) and
Foxn4 (red). Confocal image of wild-type E10.5 mouse spinal cord,
showing co-localisation of Scl and Foxn4 in some cells.
(B-C') Sections from chicken embryos electroporated at st12-14
with ß-actin-Foxn4-IRES-GFP and analysed after a further 24 (B)
or 48 (C) hours. Foxn4 does not induce Scl after 24 hours
(B'). At this stage, endogenous Scl is not expressed in the
chick neural tube (B'). Foxn4 does induce ectopic Scl
after 48 hours (C'). (D,D') Scl expression
in the p2 domain is dependant on functional Foxn4. Consecutive sections from
Foxn4-null mouse embryos at E10.5 were subjected to ISH for
lacZ (D) or Scl (D'). The row of Scl-positive
cells visible on the left of this section are endothelial cells. (E)
Scl-positive cells in a wild-type mouse embryo at E10.5.
(F,G) Foxn4 expression is not dependent on Scl.
Foxn4 expression was visualised by ISH at E11.5 in wild-type (F) and
Scl conditional null (G) mouse spinal cords (see Materials and
methods). Scale bar: 20 µm.
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Fig. 3. Foxn4 is expressed in common precursors of V2a and V2b
interneurons. (A,B) Foxn4+/- mouse
embryos were labelled by double immunohistochemistry for ß-galactosidase
(ß-gal, green) and either Chx10 or Gata3 (red). Confocal microscopy
reveals cells that are double labelled for ß-gal and either Chx10 (A) or
Gata3 (B), suggesting that Foxn4-expressing progenitors give rise to both V2a
and V2b interneurons (INs). (C-F) Consistent with this conclusion,
Foxn4-positive progenitors co-express Mash1 (C) and
Lhx3 (D), markers that later segregate into V2b and V2a INs
respectively. Individual Foxn4/Lhx3 double-positive cells
(boxes E and F) are reproduced, with fluorescence channels separated, in the
lower left and lower right corners, respectively, of D.
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Fig. 4. Foxn4 is necessary and sufficient to induce Dll4 in
the p2 domain. (A-D1) Double ISH for Dll4 (green) and
Foxn4 (red) in wild-type E10.5 mouse embryos, counter-stained with
Hoechst to visualise cell nuclei. A and B are transverse and longitudinal
sections, respectively, of spinal cord. Foxn4 is expressed in some of
the Dll4-positive cells within and outside the VZ (arrows). A
significant proportion of double-labelled cells at the ventricular surface are
pairs of cells in contact with each other, presumptive daughters of a recent
progenitor cell division (e.g. arrows in B). Examples of these are shown at
higher magnification in C,D; note the paired nuclei in C1,D1.
(E,E') Foxn4-null mouse embryos at E10.5. (E)
lacZ expression under Foxn4 control. (E')
Dll4 expression in the p2 domain is abolished. (F,F1)
Double ISH for Foxn4 (green) and Dll4 (red) showing that
Foxn4 induces ectopic expression of Dll4 in electroporated st11-13
chick neural tube.
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Fig. 5. Dll4 inhibits V2a lineage progression. Chick embryos were
electroporated with human DLL4 (hDll4) in the form of
hDll4-Myc at st14-16 and analysed after 48 hours. (A-B) Double
immunolabelling for Chx10 (red) and hDll4-Myc (green) showing repression of
Chx10-positive cells. (B) Quantification of Chx10-labelled cells showed a
 50% decrease on the hDll4-electroporated side compared with the
contralateral, control side. (C) Some hDll4-electroporated
cells co-express Chx10, consistent with the idea that Dll4 can suppress V2a
generation in a non-cell-autonomous fashion. (D) Immunolabelling for
hDll4-Myc (green). (D') Dll4 exceptionally can induce
Gata2 (arrowhead). (D'') Dll4 does not affect
Scl expression. (E) Dll4 does not greatly affect
generation of V2b INs, judging by ISH. Quantification of V2b markers
Gata2 and Scl by pixel-counting software showed no
significant effect on V2b production (see text for statistics).
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Fig. 6. Foxn4 controls Mash1 expression. (A) Double ISH for
Foxn4 (red) and Mash1 (green) in E10.5 mouse cord. Note the
extensive overlap in the p2 domain. (B,B') Foxn4 induces
ectopic expression of Cash1 in chick electroporation experiments.
(C,D) Foxn4 expression does not depend on
Mash1; there is no noticeable change in the Foxn4 ISH signal
in Mash1-null mice compared with wild type.
(E,E') Electroporation of
ß-actin-Mash1-IRES-GFP in the st13-14 chick neural tube induces
Dll4 after 24 hours. Mash1 expression was confirmed by GFP
immunolabelling (E) and Dll4 by ISH (E'). (F-G) Mash1
did not induce ectopic Chx10, but repressed endogenous Chx10 V2a INs in the p2
domain. G is a magnified view of the ventral part of panel F'.
(H-H'') Also, Mash1 did not induce ectopic V2b markers
Gata2 or Scl. (I,J) Despite the fact that
Mash1 is sufficient to induce Dll4 in chick (see E,E'), Mash1
is not required for Dll4 expression in mice; Dll4 is
expressed as normal in the ventral spinal cord of Mash1-null
mice.
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Fig. 7. Notch1 is required for specification of V2b interneurons. Mice
carrying a floxed allele of Notch1 and a Nestin-Cre
transgene (Notch1 cKO mice) were analysed at E10.5 and E11.5 by ISH
and double immunolabelling for V2a and V2b IN markers. (A-D) There is a
two-fold increase in the number of Chx10 immunopositive V2a INs in the
Notch1 cKO compared with wild type, whereas Gata3 immunopositive V2b
INs are abolished. In addition, the Chx10-positive V2a INs accumulate near the
midline of the spinal cord instead of migrating into the parenchyma.
(E,F) Double immunolabelling for Olig2 (magenta) and Hb9
(green). In the Notch1 cKO, Olig2-positive cells are missing and the
Hb9 population is similar to that in the control. Therefore, Notch1 activity
is needed for V2b IN production; in the absence of Notch1, V2b INs are
respecified as V2a INs with little or no influence on MN fate. (G-J) In
the Notch1 cKO, expression of Foxn4 is increased at E10.5
relative to wild type (compare G with H), but is almost extinguished by E11.5
(I,J). (K-N) Scl (V2b INs) is reduced at E10.5 (K,L) and
absent at E11.5 (M,N) in the Notch1 cKO. Note that the ventral half
of the central canal (and the VZ) is lost in the Notch1 cKO mouse
between E10.5 and E11.5.
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Fig. 9. Generation of V2a and V2b INs from common progenitors in the p2
domain. Multipotent neuroepithelial (radial) progenitors (A), which
do not express Foxn4, generate a population of V2a/V2b (p2) progenitors
(B). All V2a/V2b progenitors express Foxn4, which induces the
expression of Dll4, Gata2 and Mash1. These common progenitors also start to
express Lhx3 at their final division (C). Notch1 is expressed in all p2
progenitors (Lindsell et al.,
1996 ), so Notch1/Dll4 reciprocal cell-cell interactions are
initiated (opposing arrows in C). This situation resolves into two populations
of progenitors, one with activated Notch1 (Notch1*) and the other
with Dll4 (D). Notch1* blocks the V2a fate and, in
cooperation with Foxn4 and Mash1, specifies V2b IN fate (E). The
complementary set of p2 progenitors (Dll4-positive) that fails to activate
Notch1 adopts the V2a fate instead, possibly under the control of Lhx3
(Tanabe et al., 1998) (E). In
this way, V2a and V2b INs are generated in a salt-and-pepper fashion during
the same time window from a homogeneous population of p2 progenitors.
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© The Company of Biologists Ltd 2007
(?) Dll4, which is speculative. Black
arrows denote speculative interactions proposed in the present study. Blue
arrows depict interactions demonstrated in previous studies (see below). The
dashed red line represents the proposed intercellular Dll4/Notch1 interaction
between sibling V2 progenitors, which results in Notch1 being activated
(yellow star) in the cells that develop subsequently as V2b INs. The grey
arrow signifies the requirement of Mash1 for proper V2b development
(Li et al., 2005