The Role of gp130 in Cerebral Cortical Development: In Vivo Functional Analysis in a Mouse Exo Utero System

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The Journal of Neuroscience, July 1, 2002, 22(13):5516-5524

The Role of gp130 in Cerebral Cortical Development: In Vivo Functional Analysis in a Mouse Exo Utero System
Toshihisa Hatta¹, Kenji Moriyama¹, Kinichi Nakashima², Tetsuya Taga², and Hiroki Otani¹
¹ Department of Anatomy, Shimane Medical University, Izumo 693-8501, Japan, and ² Department of Cell Fate Modulation, Institute of Molecular Embryology and Genetics, Kumamoto University, Kumamoto 860-0811, Japan

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The role of gp130 in cerebral cortical histogenesis remains unknown. Mice lacking gp130 showed a hypoplastic cortical plateand decreased incorporation of 5-bromo-2'-deoxyuridine (BrdU)in progenitor cells of the developing cerebrum. In contrast, injectionof leukemia inhibitory factor (LIF), a gp130 ligand, into thelateral cerebral ventricle of wild-type embryos exo utero inducedhyperplasia of the cerebral cortex and increased the incorporationof BrdU in progenitor cells. Furthermore, chronologically controlledinjection of LIF followed or preceded by BrdU revealed that gp130-mediatedsignals promote the progenitor cells to reenter the stem cellcycle without affecting the duration of cell cycle and enhancethe migration of postmitotic neurons in the developingcerebrum.

Key words: gp130; leukemia inhibitory factor; cerebral cortex; neurogenesis; exo utero development; knock-out mouse

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

gp130 is a common signal transducer acting in association with ligand-specific receptors for the interleukin-6 (IL-6) familyof cytokines, including IL-6, IL-11, leukemia inhibitory factor(LIF), ciliary neurotrophic factor (CNTF), oncostatin-M (OSM),and cardiotrophin-1 (CT-1). Signals of IL-6 and IL-11 are transducedvia a homodimeric complex of gp130, and those of LIF, CNTF, OSM,and CT-1 are transduced via a heterodimeric complex of gp130 andthe LIF receptor (LIFR) (Taga et al., 1989; Hibi et al., 1990;Yin et al., 1993; Kishimoto et al., 1994; Pennica et al., 1995;Taga and Kishimoto 1997). gp130 thus acts as a common transducerand causes some redundancy in the functions of thesecytokines.

gp130-mediated signals play roles in a variety of cells (Taga et al., 1992; Kishimoto et al., 1994; Taga and Kishimoto, 1997).LIF and CNTF contribute to the survival and/or differentiationof neurons and glial cells in vitro (Ernsberger et al., 1989;Murphy et al., 1991, 1993; Ip et al., 1992; Mayer et al., 1994).In addition, their involvement in the survival of developing neuronsin the brainstem and spinal cord has been suggested in knock-outmice lacking the LIFR (Li et al., 1995; Ware et al., 1995) orthe CNTF receptor (CNTFR) (DeChiara et al., 1995). Disruptionof gp130 resulted in prenatal death with disorders of myocardialand hematological development. Development of cerebral cortexcould not be examined because prenatal death occurred before neuralhistogenesis in the cerebral cortex of gp130 ( $-$ / $-$ ) in the geneticbackground of a mixture of 129 and C57BL/6 (Yoshida et al., 1996).However, by generating mice that harbor a cardiac ventricularrestricted knock-out of gp130 via Cre-loxP-mediated recombination,it was revealed that conditional mutant mice had normal cardiacstructure and function and that the cardiac defect seen in conventionalgp130 ( $-$ / $-$ ) embryos likely represents a secondary effect of gp130deficiency (Hirota et al., 1999). Recently, some gp130 null mutantshave managed to be survived until birth after a change in thegenetic background from a mixture of 129 and C57BL/6 (Yoshidaet al., 1996) to ICR (Kawasaki et al., 1997). Using this strain,we reported that the survival of motor neurons in the brainstemand spinal cord and sensory neurons in the dorsal root ganglia(DRG), as well as the differentiation of astrocytes, were impairedin gp130-deficient mice (Nakashima et al., 1999a), which is consistentwith findings in knock-out mice lacking the LIFR or CNTFR. Inaddition, we showed that gp130, LIFR, and LIF are expressed incultured progenitor cells from embryonic day 14.5 (E14.5) wild-typecerebrum, and gp130-mediated signal transduction is stimulatedby exogenously added LIF in vitro (Nakashima et al., 1999a,b).However, the exact function of gp130 in the neurogenesis of thedeveloping cerebral cortex remainsunclear.

In the present study, we observed histologically that the cerebral cortex is hypoplastic and that 5-bromo-2'-deoxyuridine(BrdU) incorporation decreased in the gp130-deficient embryos.We then analyzed the role of gp130-mediated signals in cerebralcortical development by injecting LIF as an exogenous ligand intothe embryonic cerebral ventricle and observed effects on progenitorcells in the ventricular zone (VZ), as well as on postmitoticneurons in the cortical plate (CP). The experiment was based onthe mouse exo utero development system (Muneoka et al., 1986;Hatta et al., 1994; Zhang et al., 1998). This experimental systemcan set "gain of function" conditions in a spatiotemporally controlledand readily modifiable manner, which is difficult to attain usingthe conventional transgenic or even the latest Cre-loxP strategy(Hirota et al., 1999; Li et al., 2000). Thus, we could functionallydissect and analyze the effects of LIF/gp130-mediated signalson the developingcerebrum.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals
Jcl:ICR female mice aged 8-20 weeks old (CLEA Japan, Tokyo, Japan) were used. A female mouse was housed with a potent maleovernight, and the day a vaginal plug was recognized was designatedE0. For exo utero surgery, dams were anesthetized with pentobarbital.All treatments involving experimental animals were performed inaccordance with the guidelines for animal experiments of ShimaneMedical University (Izumo, Japan). The gp130-deficient mice usedin this study had the genetic background of ICR, and some of thenull embryos survived until birth: the original strain, whosegenetic background is a mixture of 129 and C57BL/6, is embryoniclethal (Yoshida et al., 1996; Kawasaki et al., 1997).

Exo utero surgery and microinjection of LIF
On E14, exo utero surgery was performed as described previously (Hatta et al., 1994). Briefly, after making a longitudinalincision along the myometrium on the opposite side of the placenta,we injected 1 µl of LIF solution into the left cerebral ventricleof the embryos with a fine glass needle through the embryonicmembrane. Recombinant murine LIF (R & D Systems, Minneapolis,MN) was dissolved at 10 ng/µl in sterilized saline with 0.1% bovineserum albumin as a carrier and injected into embryos in the leftuterine horn, whereas control embryos in the right horn of thesame dam were injected with the vehicle. The dose of LIF (10 ng/embryo,40-50 µg/kg body weight) was determined based on a pilot studyand a previous report (Akita et al., 1996). The embryos togetherwith the uterus were placed back in the abdominal cavity of thedams. On E14, E15, E16, and E18, dams were killed by an overdoseof diethyl ether, and the embryos wereobtained.

Semiquantitative study on cerebral cortical neurons
For the morphometric study of the number of cortical neurons in gp130 ( $-$ / $-$ ) embryos on E15 and LIF-injected embryos on E18,we applied a nonstereological but semiquantitative analysis (Satriotomoet al., 2000) with a random and systematic sampling. In brief,the left cerebral cortex was divided into three parts: anterior,intermediate, and posterior parts. The initial section of theanterior part was determined as the most rostral one in whichthe pallidal fork of the lateral ventricle clearly divided theelevated ganglionic eminence (GE) into medial (pallidum) and lateral(striatum) parts on E15 and the anterior commissure crossing themidline on E18. The initial section of the intermediate part wasdetermined as the most rostral one in which the interventricularforamen of Monroe appeared on both E15 and E18. The initial sectionof the posterior segment was determined as the caudal end of GE,at which the elevation of GE into the lateral ventricle was flattened.Each initial section was numbered as 1, with all subsequent sectionsbeing numbered sequentially rostral to caudal. In each embryo,a number between 1 and 5 was selected at random to determine thefirst section. Every third section for E15 brains and fifth sectionfor E18 was chosen for semiquantitative analysis (for example,sections 2, 5, 8, etc. for E15 were selected and sections 2, 7,12, etc. for E18). Five and six sections at E15 and E18, respectively,were chosen from each of the anterior, intermediate, and posteriorparts and used for the subsequent analysis. Photographs of theleft hemisphere were taken with a light microscope (model BX50;Olympus Optical, Tokyo, Japan) at 1-4× magnification dependingon the size of the area, using a CCD camera (model CS520MD; OlympusOptical). The boundary of the cerebral cortex was drawn on thecaptured images (Vaccarino et al., 1999), and the area of theleft cerebral cortex per section was measured using the ScionImage software (Beta 4.0.2; Scion, Frederick, MD). The cell densityof the cerebral cortex in each section was estimated as follows.Several regions of the left cerebral cortex, the margins of whichshould overlap, were captured at 20 or 40× magnification. Thetransformed images were used to reconstruct the whole left cortexon the section using Adobe Photoshop (version 5.0; Adobe Systems,San Jose, CA). Then the grid was superimposed on the reconstructedimages using the grid function of the software. The distance betweenadjacent cross points of the grid lines was 25 µm, so that thearea of a square (counting box) determined by the grid line was25 × 25 µm². The counting box located in the most medial and most dorsalregion was numbered 1. The other boxes were then numbered seriallymedial to lateral in the dorsoventral dimension. Every 15th boxwas selected for cell counting, and ~20 boxes per section on E15and 50 boxes on E18 were used (in total, ~300 boxes at E15 and750 boxes at E18 per brain). The average number of cells in acounting box was obtained, and the estimated density of cellsper 1 µm² was calculated. The total number of cells was calculated by multiplyingthe mean cell density by area in each section, and then the averageof the total number of cells per section was calculated in theanterior, central, and posterior parts in the cerebral cortexas a representative value for each part. Three embryos were usedin the LIF-injected and control groups on E18, and three and sixembryos were used in gp130 ( $-$ / $-$ ) and (+/+) on E15,respectively.

BrdU injection schedules
Dams were injected intraperitoneally with 50 mg/kg body weight of BrdU (Sigma, St. Louis, MO) in distilled water. The schedulesof BrdU injections are asfollows.
The effects on the proliferative activity of progenitor cells in the VZ. Progenitor cells at S phase in the VZ of gp130 ( $-$ / $-$ )[( $-$ / $-$ ), n = 3; (+/+), n = 6)], and LIF-injected embryos were labeledwith an intraperitoneal injection of BrdU given to the dams onE15 (24 hr after LIF injection) (see Fig. 3c) (LIF, n = 3; control,n = 3), and embryos were removed 2 hr after BrdUinjection.
The effects on the nuclear translocation of progenitor cells. BrdU was injected 2 hr before LIF, and embryos were killed 6,10, and 14 hr later on E14 (see Fig. 4j). In the exo utero systemon E14, the inner subset of the labeled cell population (distributedaround bin 4) reached the ventricular surface (bin 1) ~6 hr afterBrdU injection. Most of the labeled cells accumulated there (bin1-2) at 10 hr after BrdU injection, exited M phase, and movedupward ~14 hr after BrdU injection (Hatta et al., 1994). Threeembryos were used for each time point in the LIF-injected andcontrolgroups.
The effects on the migration of the postmitotic neurons. BrdU was injected 12 hr before LIF on E14 (see Fig. 5a). When LIFwas injected 12 hr after BrdU on E14, the labeled cell populationhad finished M phase and was migrating upward from the ventricularsurface to the cerebral cortex (Fig. 4h,i) (for details, see Results).Thus, the initial number of labeled progenitor cells was the samebetween the LIF-injected and control groups. At 60 hr after BrdUinjection (48 hr after LIF injection), BrdU-labeled cells appearedin the CP. In the control embryos, labeled neurons derived fromthe first cell division after BrdU injection had entered the CPbut were still migrating to the pial surface across the CP, aswas determined in a pilot study performed exo utero. In the presenttime range, whereas the first generation of labeled daughter cellsreached the CP, the later (second or third) generation of labeledcells had not yet reached the CP. Therefore, the number of BrdU-labeledcells in the CP was equal between LIF-injected and control groups(for details, see Results), and the number and distribution ofBrdU-labeled cells along the ventrodorsal dimension in the CPshould reflect the migration of first generation of postmitoticneurons. They were examined semiquantitatively as described belowin three embryos each for the LIF-injected and controlgroups.

Tissue preparation
Whole embryos on E11-E13 were fixed by immersion for 6-12 hr at 4°C in a mixture of 4% formaldehyde and 70% methanol. On E14and E15, embryos were decapitated and fixed in the manner describedabove. On E16 and E18, the brains were dissected out in physiologicalsaline at 4°C under a dissecting microscope and fixed as describedabove. Specimens were embedded in paraffin and sectioned at 5µm coronally or sagittally. The brains of gp130 ( $-$ / $-$ ) and (+/+)embryos on E15 and of LIF-treated and control embryos on E18 weresectioned in the coronal plane. In the first several sectionsthrough the olfactory bulb and the anterior part of the cerebralventricle in the coronal plane, the cutting angle was adjustedright-left symmetrically and as perpendicular as possible by adjustingthe microtome. Then serial sections were prepared throughout thecerebrum and stained with hematoxylin-eosin (HE) for general histologyand cresyl violet for the counting of cerebral cortical neurons.For BrdU analysis, serial paramedian sagittal sections of theleft cerebrum were prepared at 5 µm.

Semiquantitative study on BrdU-labeled cells
The number and distribution of BrdU-labeled cells were analyzed semiquantitatively based on the bin method used by Takahashiet al. (1993, 1995, 1996a,b) with some modifications. The paramediansagittal section in which the olfactory bulb had disappeared wasdesignated as the first section, and subsequent sections werenumbered serially in the mediolateral dimension. The first andevery third sections were selected, and five sections per brainwere examined. The distribution of the BrdU-labeled cells wasanalyzed in the sector, which was settled in the dorsomedial cerebralwall, corresponding to the intermediate cortex in the coronalplane described above. The region of analysis was 360 µm in itsrostrocaudal dimension and was composed of 18 sectors, 20 µm inwidth. Sectors were numbered in the rostrocaudal dimension, andevery second sector (nine sectors per section) was selected. Sectorswere then divided into bins, 20 µm in height in the ventrodorsaldimension. The bins were numbered 1, 2, 3, and so on, from theventricular surface outward for analyzing the number and distributionof BrdU-labeled cells in the VZ and from the pial surface inwardfor those in the CP (Takahashi et al., 1993, 1995, 1996a,b). Thenumber of BrdU-positive cells per bin per sector was obtainedin each experiment and was shown by ahistogram.

Immunohistochemistry
Sections were incubated with 10% normal goat serum (Dako, Glostrup, Denmark) in Tris-buffered saline (TBS) (100 mM Tris-Cland 150 mM NaCl, pH 7.5) for 30 min at room temperature, the rabbitpolyclonal anti-human gp130 antibody (1:500; 8.5 µg/ml; UpstateBiotechnology, Lake Placid, NY) in TBS at 4°C overnight, and thealkaline phosphatase-conjugated anti-rabbit IgG (1:500; VectorLaboratories, Burlingame, CA) in TBS for 30 min at room temperature.Sections were visualized with a mixture of 4-nitroblue tetrazoliumchloride (Boehringer Mannheim, Mannheim, Germany) and 5-bromo-4-chloro-3-indolyl-phosphate(Boehringer Mannheim) containing 1 mM levamisole (Sigma) as aninhibitor for nonspecific phosphatase reactions. Non-immunizednormal rabbit IgG (8.5 µg/ml; Zymed, San Francisco, CA) was usedas an immunohistochemical control forgp130.
To detect the BrdU-labeled cells, sections were digested with 0.1% trypsin in 0.1% CaCl₂ for 8-10 min at 37°C, denatured with2N HCl for 30 min, and neutralized with 0.1 M borax-borate buffer,pH 8.8, for 5 min at room temperature. Sections were pretreatedwith a mixture of 0.3% hydrogen peroxide and 99% methanol for15 min. They were incubated in the 10% normal goat serum for 30min, in anti-BrdU antibody (1: 50) (Dako) overnight at 4°C, andthen in Dako Envision polymer (Dako, Carpinteria, CA) for 1 hrat room temperature. Sections were visualized with 0.05% 3,3'-diaminobenzidine-tetrahydrochloride(Wako, Osaka, Japan) and 0.01% hydrogen peroxide. Adjacent sectionswere incubated in TBS without primary antibody as a negative controlof BrdUimmunostaining.

Statistical analysis
All data in this study are presented as the mean ± SD. An ANOVA was used for comparisons of groups and a post hoc pairwisecomparison (Fisher's post hoc test) for each factor between groups.The difference in the total number of cells per sector betweengroups was analyzed by Student's ttest.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression of gp130 in the developing cerebrum of the wild-type embryo

On E11, the expression of gp130 in the cerebral wall was faint compared with that in the other parts of the CNS and DRG (Fig.1a,e) in the wild-type embryo. On E13, gp130 was expressed throughoutthe cerebral wall (Fig. 1b). Most cells showed staining of moderateintensity, but some cells in the VZ, intermediate zone (IZ), andpreplate (PP) were heavily stained (Fig. 1f). On E14, the stainingof the progenitor cells became more intense in the VZ, and thenumber of heavily stained neurons increased in the CP (Fig. 1g).On E15, the number of neurons in the CP and progenitor cells thatwere heavily stained increased, and most cells were strongly positivefor gp130 (Fig. 1c,h,i). Mitotic cells on the ventricular surfacewere not stained for gp130 (Fig. 1i, arrowheads). On E18, cellsin the CP and subventricular zone (SVZ) and fibers in the SVZwere heavily stained, whereas the staining intensity was decreasedin the VZ (Fig. 1d,j). Negative controls were incubated with non-immunizedrabbit IgG and showed no staining (data not shown).

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Figure 1. Expression of gp130 in the developing cerebral wall. On E11, the staining intensity is faint in the cerebral wall (Cer) (a, e). On E13, gp130 staining is generally positive in the cerebral wall (b). Some heavily stained cells appear among the many lightly stained cells in the VZ, IZ, and PP (f). On E14, the staining of the progenitor cells became more intense in the VZ, and the number of heavily stained neurons increased in the CP (g). On E15, cells and fibers in the CP, IZ, and VZ are stained heavily (c, h, i). Note that the mitotic cells on the ventricular surface are not stained for gp130 (arrowheads in i). On E18, gp130 staining is strongly positive in cells and fibers in the CP and SVZ (d, arrows in j); in contrast, the staining intensity was decreased in the VZ (j). Negative controls were incubated with normal rabbit IgG and showed no staining (data not shown). MZ, Marginal zone; LV, lateral ventricle; fourth, fourth ventricle. Scale bars: a-d, 1 mm; e-j, 100 µm.

Characteristic phenotypes in the cerebrum of gp130 ( $-$ / $-$ ) and LIF-injected embryos

Cellularity in the CP was characteristically lower in gp130 ( $-$ / $-$ ) than gp130 (+/+) embryos on E15 (Fig. 2, compare a, b).Semiquantitative analysis revealed that gp130 ( $-$ / $-$ ) embryos differedsignificantly from gp130 (+/+) embryos in the number of corticalneurons per section in the left hemisphere (ANOVA; p < 0.001;F = 52.9). Post hoc test (Fisher's post hoc test) revealed significanteffects of genotype on the number of neurons per section in theanterior, intermediate, and posterior parts of the cerebral cortexin the left hemisphere (p < 0.01) (Fig. 2c). In contrast, histologicalobservation revealed that wild-type embryos injected with LIFon E14 showed higher cellularity in the CP than controls on E18(Fig. 2, compare d, e). Semiquantitative analysis revealed thatLIF-injected embryos differed significantly from controls in thenumber of cortical neurons per section in the left hemisphere(ANOVA; p < 0.001; F = 32.7). Post hoc test (Fisher's post hoctest) revealed significant effects of LIF on the number of neuronsper section in the anterior, intermediate, and posterior partsof the cortex in the left hemisphere (p < 0.05) (Fig. 2f). Glialfibrillary acidic protein-immunostaining for astrocytes was negativein the CP on E15 and E16 (data not shown). Apoptotic cells wererare in the cerebral wall and indistinguishable between gp130( $-$ / $-$ ) and (+/+) embryos or between LIF-injected and control groupsstained by HE or cresyl violet or by the terminal deoxynucleotidyltransferase-mediated biotinylated UTP nick end labeling method(Gavrieli et al., 1992) (data not shown).

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Figure 2. Histological changes of the cortical plate in LIF-injected or gp130-deficient embryos. a-c, The cortical plate in gp130 ( $-$ / $-$ ) and (+/+) embryos on E15. Coronal sections of the dorsal region of the left anterior cortex in gp130 ( $-$ / $-$ ) (a) and (+/+) (b) (cresyl violet staining). c, Semiquantitative analysis revealed that the gp130 ( $-$ / $-$ ) embryos differed significantly from gp130 (+/+) embryos in the number of cells in the cerebral cortex (p < 0.001; F = 52.9; ANOVA). The number of cells per section in the anterior, intermediate, and posterior parts of the cortex was significantly decreased by disruption of gp130 (*p < 0.01; Fisher's post hoc test). d-f, LIF-injected and control brains on E18. The cellularity of the CP is greater in the LIF group (d) than in the control group (e) (anterior part of the cerebral cortex in the coronal plane on E18, HE staining). f, Semiquantitative analysis revealed that LIF-treated animals differed significantly from controls in the number of cells in the cerebral cortex per section (p < 0.001; F = 32.7; ANOVA). The number of cells per section in the anterior, intermediate, and posterior parts of the cortex was significantly increased by the LIF-treatment (**p < 0.05; Fisher's post hoc test). MZ , Marginal zone. Scale bars, 100 µm.

Proliferation of progenitor cells in the cerebral ventricular zone of gp130 ( $-$ / $-$ ) and LIF-injected embryos

On E15, gp130 ( $-$ / $-$ ) embryos differed significantly from gp130 (+/+) embryos in the number of BrdU-positive cells per sector(ANOVA; p < 0.001; F = 33.5) (Fig. 3a). The total number of BrdU-positivecells per sector was significantly decreased by the gp130 disruption[(+/+), 12.6 ± 3.56; ( $-$ / $-$ ), 7.0 ± 1.21; p < 0.05; Student's ttest], indicating a reduction in the proliferation of progenitorcells on disruption of gp130. We then examined the changes ofBrdU incorporation in progenitor cells after LIF injection intothe cerebral ventricle of wild-type embryos. BrdU was injectedinto dams on E15, 24 hr after LIF treatment (Fig. 3c), and embryoswere analyzed 2 hr after the injection. The LIF-injected groupdiffered significantly from the control in the number of BrdU-positivecells per sector (ANOVA; p < 0.001; F = 61.0) (Fig. 3b). The totalnumber of labeled cells per sector was significantly increasedby LIF injection (LIF, 20.1 ± 3.71; control, 10.0 ± 0.71; p <0.01; Student's t test), indicating that the LIF induced progenitorcells to reenter the cell cycle, and then, as a result, the numberof progenitor cells at S phase increased.

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Figure 3. Mitotic labeling in the ventricular zone after gp130 deletion and activation. a, Progenitor cells were labeled by single injection of 50 mg/kg BrdU in gp130 ( $-$ / $-$ ) embryos and gp130 (+/+) littermates on E15. Embryos were analyzed 2 hr after the injection. Semiquantitative analysis revealed that gp130 ( $-$ / $-$ ) differed significantly from gp130 (+/+) in the number of labeled cells (p < 0.001; F = 33.5; ANOVA). Total number of BrdU-positive cells per sector was significantly decreased in gp130 ( $-$ / $-$ ) compared with gp130 (+/+) [( $-$ / $-$ ), 7.0 ± 1.21; (+/+), 12.6 ± 3.56; p < 0.05; Student's t test]. b, Progenitor cells were labeled by single injection of 50 mg/kg BrdU in LIF-injected and control embryos on E15. BrdU was injected into dams 24 hr after LIF, and embryos were analyzed at 2 hr after BrdU injection, as shown in c. Semiquantitative analysis revealed that the LIF-injected embryos differed significantly from the controls in the number of labeled cells (p < 0.001; F = 61.0; ANOVA). The total number of BrdU-positive cells per sector was significantly increased in the LIF-injected group compared with the control (LIF, 20.1 ± 3.71; control, 10.0 ± 0.71; p < 0.01; Student's t test).

Effects of LIF on the elevator movement of progenitor cells

To clarify the mechanisms underlying the changes described above, we further analyzed the effects of LIF on the progenitorcell kinetics known as elevator movement. Elevator movement andassociated production of neurons is divided into the followingphases: (1) downward nuclear translocation to the ventricularsurface (S to G₂/M phase and mitosis), (2) upward nuclear translocation(G₁ phase) of a daughter cell, which reenters the stem cell cycleas described above and also later in the next section, and (3)migration of another daughter cell, which exits the stem cellcycle (G₀), up to the CP as a postmitotic neuron (Fujita, 1963;Jakobson, 1991).

We first analyzed the effects of LIF on the downward nuclear translocation of progenitor cells (duration of S to G₂/M phase).We injected BrdU into dams 2 hr before LIF to eliminate possibleeffects of LIF on the labeling efficiency and then evaluated thenumber and localization of BrdU-positive nuclei of progenitorcells at 6, 10, and 14 hr after BrdU injection (Fig. 4j). Theinterpeak of the BrdU-positive cell distribution in both LIF-treatedand control groups moved from bin 4 (60-80 µm from the ventricularsurface) to bin 1 (0-20 µm from the ventricular surface) at 6hr (Fig. 4a,d,g), and a majority of the labeled cells had accumulatedon the ventricular surface (bin 1) at 10 hr after BrdU injection(Fig. 4b,e,h). At 14 hr after BrdU injection, most of the labeledcells were distributed through bin 1 to bin 3, and the interpeakof the distribution was in bin 2 for both groups. When observedclosely, the inner half of bin 1 was found to be occupied by unlabeledcells, indicating that the labeled cells had already passed throughM phase and changed position to the deeper area of the VZ at 14hr after BrdU injection in both groups (Fig. 4c,f,i). Semiquantitativeanalysis revealed that there were no significant interactionsbetween treatment (LIF injection or control) and bin in the numberof labeled cells per sector or no significant differences in thenumber of BrdU-positive cells for any bin between LIF-injectedand control groups (Fig. 4g-i).

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Figure 4. Effect of LIF on the downward nuclear translocation of the progenitor cells. Progenitor cell cells were labeled with BrdU 2 hr before injection of LIF on E14, and the distribution of BrdU-positive nuclei was analyzed 6, 10, and 14 hr after BrdU injection (j). The interpeak of the BrdU-positive cell distribution in both groups shifted from bin 4 (60-80 µm from the ventricular surface) (see Fig. 3) to bin 1 (0-20 µm from the ventricular surface) at 6 hr (a, d, g). Most cells had accumulated on the ventricular surface (bin 1) at 10 hr after BrdU injection (b, e, h), when the cells had entered or just finished M phase. At 14 hr after BrdU injection, the interpeak of the labeled cells shifted from bin 1 to bin 2. When observed closely, the inner half of bin 1 was found to be occupied by unlabeled cells in both groups, indicating that the labeled cell population had already passed through M phase and was changing position to a deeper area of VZ (c, f, i). Statistical analysis revealed that there were no significant differences between LIF-injected and control embryos in the number of labeled cells (ANOVA) and no significant interactions between treatment (LIF injection or control) and bin in the number of labeled cells for each time point (ANOVA) (g-i). Sac, Sacrifice. Scale bar, 100 µm.

Then the total number of BrdU-positive cells per sector was plotted for each time point (Fig. 5a). The number increased at2 hr after BrdU injection and was twice the initial value at 14hr in the LIF-injected and control groups (not significantly differentbetween the groups by ANOVA). The percentage of increased ratioin BrdU-positive cells relative to the initial value (2 hr afterBrdU) was calculated for each time point (Fig. 5b). There wereno significant differences between LIF-injected and control embryosin the percentage of increase in BrdU-positive cells and no significantinteractions between treatment and time point (ANOVA). When thelabeled population had finished mitosis, the number of labeledcells was twice the initial value (represented as 100%). The labeledpopulation finished mitosis at 10.5 and 10.7 hr in the LIF-injectedgroup and control group, respectively, as estimated from a simpleregression (LIF, r² = 0.95; control, r² = 0.95) (Fig. 5b). The percentage of labeled nuclei at M phasereached 100% at 6 hr after BrdU injection in both LIF-injectedand control groups. The duration of G₂ + M + 1/2S in both groupscan, therefore, be estimated as ~6 hr (Jakobson, 1991), whichis in the range of that established by Takahashi et al. (1993,1995).

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Figure 5. Effects of LIF on the cell cycle of progenitor cells. The total number of BrdU-positive cells on E14 was calculated from data obtained in the analysis of downward nuclear translocation. a, The number of labeled cells per sector was plotted for each time point: 6, 10, and 14 hr after BrdU injection. The number of labeled cells at 2 hr after BrdU injection without LIF was used as the initial value. In this experiment, the number of initially labeled cells was not affected by LIF injection, as shown in Figure 4j. The initial number of cells at 2 hr was ~10 per sector, increased, and then doubled between 10 and 14 hr in both groups. There were no significant differences between LIF-injected and control embryos (ANOVA) and no significant interaction between treatment and time point (ANOVA). b, The percentage of increase in BrdU-positive cells relative to the initial value was calculated for each time point. When the population completed mitosis, the number of labeled cells was twice the initial value (represented as 100%). There were no significant differences between LIF-injected and control embryos in the percentage of increase of BrdU-positive cells and no significant interaction between treatment and time point (ANOVA). The labeled population finished mitosis at 10.5 and 10.7 hr after BrdU injection in the LIF-injected and control groups, respectively. The values were obtained using linear models (simple regression; LIF, r² = 0.95; control, r² = 0.95).

These findings suggest that LIF does not affect the downward nuclear translocation or duration of the 1/2S-G₂-M phases inprogenitor cells. The upward nuclear translocation could not beexamined because of a lack of appropriate markers for differentiatingbetween overlapping BrdU-positive progenitor cells and postmitoticneurons in theVZ.

The effect of LIF on the postmitotic migration of the BrdU-positive cells

We further examined the effects of LIF on the postmitotic migration of the BrdU-positive cells. Dams were injected with BrdUon E13, at 12 hr later on E14, they were injected with LIF, andthen the distribution of BrdU-positive neurons was analyzed inthe cerebral wall of the wild-type embryos on E16 (at 60 hr afterBrdU injection, 48 hr after LIF injection) (Fig. 6a). The totalnumber of BrdU-positive cells in the VZ, SVZ/IZ, and CP per sectorwas calculated by accumulating the number of cells per bin persector in each zone and revealed that the BrdU-positive cellsin the LIF-injected group significantly differed from those incontrols in the VZ (LIF, 16.9 ± 0.59; control, 8.8 ± 0.68) andSVZ/IZ (LIF, 20.8 ± 1.06; control, 11.3 ± 0.55) (Fisher's posthoc test; p < 0.01). However, there was no significant differencein the CP between LIF-injected and control groups (LIF, 12.1 ±0.60; control, 11.3 ± 0.55) (Fig. 6b), indicating that, at 60hr after BrdU injection, the first generation of labeled neuronshad reached the CP, but the next generation of labeled neuronshad not yet arrived.

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Figure 6. Change of the number and distribution of BrdU-labeled cells at 60 hr elapse. Dams were injected with BrdU on E13 (12 hr before LIF injection), and the number and distribution of BrdU-positive cells was analyzed in the cerebral wall of the wild-type embryos 60 hr after BrdU on E16 (a). The total number of BrdU-labeled cells per sector in the cerebral wall was significantly increased in the LIF-injected group than that in the control (ANOVA; p < 0.01) (b). Post hoc analysis revealed that the number of labeled cells in the VZ and SVZ/IZ significantly increased in the LIF-injected group (p < 0.01; Fisher's post hoc test) but that, in the CP, did not significantly differ between the LIF-injected and control groups (b). This result indicates that the labeled neurons derived from the first cell division after BrdU labeling had reached to the CP, but the later generation had not yet arrived. It is also suggested that LIF directed the postmitotic labeled daughter cells to reenter the cell cycle to increase the stem cell pool in the VZ and SVZ, because the number of labeled migrating neurons in SVZ/IZ increased. The histogram demonstrates the distribution pattern of BrdU-positive cells per sector in each bin (c). Note that, although the total number of BrdU-positive cells in the CP did not differ between LIF-injected and control groups (b), BrdU-positive cells were localized significantly more in bins 21 and 23 (p < 0.05) and less in bins 17 (p < 0.05) and 18 (p < 0.1) in the LIF-injected group than in the control (Fisher's post hoc test) (c). This finding indicates that the first generation of the BrdU-positive neurons was localized more in the outer and less in the inner region of the CP in the LIF-injected group than in the control group, suggesting that LIF promoted the migration of postmitotic neurons. *p < 0.05; **p < 0.1.

The distribution pattern of the BrdU-positive cells in the CP was analyzed, as represented in the histograms of the BrdU-positivecells per sector in the bins (bins 17-22) (Fig. 6c). It was demonstratedthat the BrdU-positive cells in the CP were localized more inpial side (bin 22 and bin 21; p < 0.05) and less in bin 17 (p< 0.1) and bin 18 (p < 0.05) in the LIF-injected embryos thanin the control (Fisher's post hoc test), suggesting that LIF promotedthe migration of postmitotic neurons to theCP.

In contrast to the CP, the number of BrdU-positive cells significantly increased in the VZ and SVZ/IZ (Fig. 6b,c) in the LIF-injectedembryos than that in the control, indicating that LIF inducedprogenitor cells to reenter the stem cell cycle as described above(Fig. 3b).

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Do gp130-mediated signals play roles in the developing brain?

In contrast to the mild changes in the CNS induced by gene disruption of LIF (Escary et al., 1993) and/or CNTF (Masu et al.,1993), knock-out mice lacking LIFR, CNTFR, or gp130 showed hypoplasiaof motor nuclei in the brainstem and spinal cord, as well as aloss of astrocytes (DeChiara et al., 1995; Li et al., 1995; Nakashimaet al., 1999a). Therefore, it has been suggested that gp130-mediatedsignals contribute to the survival of postmitotic neurons anddifferentiation of astrocytes during development. However, thefunction of gp130 in neurogenesis and cerebral cortical histogenesisremainsunknown.

The present results regarding the expression pattern of gp130 suggest a contribution of gp130 to neuronal production. Theexpression of gp130 in the VZ of the wild-type embryos was detectedon E11, when the production of neurons had started (Angevine andSidman, 1961), increased as development proceeded, peaked at approximatelyE15, and decreased in the VZ but increased in the SVZ on E18.This chronological change in the expression of gp130 well correspondsto the change in the distribution of cells with neuronal productionin the VZ/SVZ and suggests that gp130-mediated signals are involvedin the production in the VZ for cerebral cortical histogenesis.These results further suggest that gp130 plays roles in the progenitorcells of the cerebral wall at approximately E14, when LIF wasused to stimulate the gp130 signal transduction in the developingcerebral wall in the presentstudy.

gp130 signals affect the proliferation of the progenitor cell

In the present study, gp130 ( $-$ / $-$ ) showed a hypoplastic CP, and BrdU-labeling experiments revealed that neuronal productionwas impaired among progenitor cells in gp130 ( $-$ / $-$ ). We next examinedthe in vivo effects of the gp130-mediated signals on the neurogenesisof the cerebral cortex using mouse exo utero system. Consequently,it was clearly revealed that hyperplasia of the CP is inducedby injection of LIF, allowing additional detailed analyses ofthe effects of LIF on the neuronalproduction.

First, the effect of LIF was analyzed by injecting LIF on E14, BrdU at 24 hr later on E15, and examining the number of BrdU-positivecells at 2 hr after BrdU injection. In the VZ, the number of BrdU-positivecells significantly increased in the LIF-injected group than inthe control. Furthermore, when BrdU was injected 12 hr beforethe LIF injection and the number of labeled cells was analyzed60 hr after BrdU (48 hr after LIF) injection, the number of BrdU-positivecells in the VZ significantly increased in the LIF-injected groupcompared with that in the control. In this experimental model,the initial frequency of BrdU incorporation was equal betweenthe LIF and control groups. The cell cycle of progenitor cellswas not affected by LIF and was in the range of that establishedin normal mouse embryos by Takahashi et al. (1993, 1995, 1996a,b,1999). These findings suggest that LIF increased the stem cellpool by directing the postmitotic cells, which normally exit thecycle, to reenter S phase of the stem cellcycle.

We could not detect any significant differences in the number of apoptotic cells in the CP between LIF-injected and controlgroups or between gp130 ( $-$ / $-$ ) and gp130 (+/+) embryos. Thus, itis suggested that the present changes in the number of cerebralcortical neurons were induced by the LIF effect on neuron productionrather than on cellsurvival.

LIF enhances the migration of postmitotic neurons

For analyzing the migration of postmitotic neurons, LIF was injected 12 hr after BrdU, when the labeled progenitor cells hadalready finished the first M phase. Therefore, the injection ofLIF did not affect the number of the labeled postmitotic neuronsderived from the first cell division after BrdU-labeling. In fact,the number of BrdU-positive cells per sector in the CP 60 hr afterBrdU injection, when only the first generation of BrdU-positivecells reached the CP, did not differ significantly between theLIF-injected and control groups. However, in the CP, the numberof BrdU-positive cells was significantly larger on the pial side(bins 21 and 22) and smaller on the ventricular side (bins 17and 18) in the LIF-injected group than that in the control. Thisindicates that the labeled cortical neurons at 60 hr after BrdUinjection were derived from the initial cell division after BrdUlabeling and did not include the second wave of migrating neuronsfrom the later generation and that the BrdU-positive neurons reachedthe upper part of the CP faster in the LIF-injected group thanin the control. The second wave of BrdU-positive neurons was observedin the SVZ/IZ, which were increased in number in the LIF-injectedgroup than in the control, but had not yet reached the CP. Thesefindings suggest that the migration of postmitotic neurons tothe CP was accelerated by the LIF-triggered activation of gp130.The migration of postmitotic neurons is closely related to theirdifferentiation, and therefore gp130 signals may also contributeto the differentiation of cortical neurons in vivo, as reportedin the sensory neurons of embryonic DRG (Murphy et al., 1991,1993) or sympathetic neurons (Yamamori et al., 1989) in vitro.

In conclusion, we revealed that the LIF/gp130 signal plays important roles in producing neurons and also in the migrationof postmitotic neurons in the presentstudy.

  FOOTNOTES

Received March 20, 2001; revised April 15, 2002; accepted April 16, 2002.

This study was supported by a grant from the Ministry of Education, Science, Sports, and Culture of Japan. We thank Dr. TakumiTakizawa and Dr. Wataru Ochiai for BrdU labeling and genotypingof the gp130 knock-outs and Dr. Takanori Miki and Prof. YoshihiroFukui for their suggestion of the quantitative analysis. We alsothank Yumiko Takeda for her help in histologicalpreparations.

Correspondence should be addressed to Dr. Toshihisa Hatta, Department of Anatomy, Shimane Medical University, Izumo, Shimane693-8501, Japan. E-mail: thatta{at}shimane-med.ac.jp

K. Moriyama's present address: Department of Medicine and Clinical Science, Kyoto University Graduate School of Medicine,Kyoto 606-8507,Japan.

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