Sonic Hedgehog and Bone Morphogenetic Protein Regulate Interneuron Development from Dorsal Telencephalic Progenitors In Vitro

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The Journal of Neuroscience, October 29, 2003, 23(30):9862-9872

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Sonic Hedgehog and Bone Morphogenetic Protein Regulate Interneuron Development from Dorsal Telencephalic Progenitors In Vitro
Alexandra Gulacsi and Laura Lillien
Department of Neurobiology and Pittsburgh Cancer Institute, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania 15261

   Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Cortical progenitors are competent to produce interneurons,but do not generate large numbers of interneurons in vivo undernormal circumstances. This could reflect the absence of an inductivesignal in the environment of the dorsal telencephalon and/orthe presence of an inhibitory signal. To determine whether eitheror both mechanisms regulate interneuron generation, progenitorsin dorsomedial and dorsolateral wall explants of mouse telencephalonwere marked with a retrovirus and cultured under several conditions.When cultured separately, progenitors in dorsomedial wall explantsproduced fewer GABAergic interneurons than progenitors in dorsolateralwall explants. When cocultured with ventral telencephalic cells,however, dorsomedial wall progenitors produced more GABAergicinterneurons than in dorsomedial wall explants alone. The inductiveeffect of ventral telencephalon depended on sonic hedgehog (Shh)and could be mimicked by exogenous Shh. In contrast, exogenousbone morphogenetic protein 4 (BMP4) reduced the production ofinterneurons in dorsolateral wall explants and inhibited theinduction by exogenous Shh. Moreover, inhibiting BMP signalingin dorsomedial wall progenitors with a dominant-negative BMPreceptor Ib (dnBMPIb) virus increased their production of interneurons,even if Shh was blocked. Shh and dnBMPRIb increased proliferationand the generation of interneurons, but FGF2 did not induceinterneurons, although it increased proliferation. This suggeststhat proliferation per se does not control the production ofinterneurons. Our findings suggest that the generation of interneuronsby dorsal telencephalic progenitors is normally limited by excesslevels of BMPs. Shh may promote the generation of interneuronsby antagonizing BMP, but may not be required directly for thegeneration of interneurons.

Key words: cortex; progenitor; FGF; glutamate; GABA; neuronal differentiation

   Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

There are two major classes of neurons in the neocortex andhippocampus: glutamatergic excitatory projection neurons andGABAergic inhibitory interneurons. Retroviral lineage analysisand several transgenic models revealed that distinct progenitorcells give rise to cortical projection neurons and interneurons,and that there is a relationship between cell phenotype andmigration pattern (Parnavelas et al., 1991; Luskin et al., 1993;Mione et al., 1994, 1997; Tan et al., 1998). Most cortical pyramidalcells arise from progenitors in the cortical ventricular zone(VZ) and migrate radially to form the cortical plate (Sidmanand Rakic, 1973; Rakic, 1990; Tan et al., 1998). In contrast,the vast majority of telencephalic interneurons originate subcorticallyin the ganglionic eminences (GEs) (Anderson et al., 1997a; Tamamakiet al., 1997).
Although these studies demonstrated that the majority of corticalinterneurons arise from the ventral telencephalon, they didnot rule out the possibility that the cortex produces some interneurons,perhaps as many as 20–30% (Anderson et al., 1997a). Invitro experiments revealed that cortical progenitor cells arecompetent to produce interneurons (Gotz and Bolz, 1994; He etal., 2001), raising questions about the reasons they fail togenerate large numbers of interneurons normally during embryonicdevelopment. One possibility is that the environment in thedorsal telencephalon does not support the production of interneurons,because of the absence of inductive signals and/or the presenceof inhibitory signals.
Although the intrinsic control of cortical interneuron developmenthas been studied extensively (Anderson et al., 1997b, 1999;Casarosa et al., 1999; Sussel et al., 1999), the function ofextrinsic signals in the specification of interneurons is lesswell established. One of the most investigated secreted morphogens,sonic hedgehog (Shh), is expressed at a high level in cellsof the ventral telencephalon at embryonic day 11.5 (E11.5) andonward (Kohtz et al., 1998; Sussel et al., 1999; Nery et al.,2001; Tekki-Kessaris et al., 2001). Shh has been implicatedin several aspects of CNS development, such as proliferation(Dahmane and Ruiz-i-Altaba, 1999; Wallace, 1999; Wechsler-Reyaand Scott, 1999) and cell fate determination (Marti et al.,1995; Roelink et al., 1995; Chiang et al., 1996; Ericson etal., 1996). The role of Shh in interneuron development has beensuggested by studies of its impact on Dlx (Kohtz et al., 1998,2001), which has been implicated in the specification of interneurons(Stuhmer et al., 2002). A direct demonstration that Shh inducesinterneurons was reported recently in monolayer cultures ofFGF-stimulated cortical cells (Yung et al., 2002). It remainsto be determined, however, whether Shh induces interneuronsunder more physiological conditions. Development in corticalexplants more closely resembles development in vivo (Burrowset al., 1997). In the present study we used explants of E11.5mouse telencephalon to test the hypothesis that regional differencesin both inductive and inhibitory environmental signals controlthe production of GABAergic versus glutamatergic neurons bydorsal telencephalic progenitors.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Explant cultures. Timed-pregnant CD1 mice (Charles River Laboratories,Wilmington, MA) were killed with CO₂. E11.5, E13, or E16 embryoswere placed in sterile HBSS (Invitrogen, Bethesda, MD), andthe brains were dissected. Dorsolateral and dorsomedial wallsof the telencephalon were dissected (Fig. 1 A) and transferredto nucleopore filters (13 mm, 0.2 µm pore; Corning, FisherScientific, Pittsburgh, PA) floating on serum-free culture medium(Bottenstein and Sato, 1979) containing 25 µg/ml insulin(Sigma, St. Louis, MO). For some experiments, GEs (medial andlateral) were also dissected. Approximately 25–30 minlater, 30 µl of culture medium containing retrovirus wasadded to the tops of the filters carrying dorsal telencephalicexplants. This results in a selective infection of progenitorcells in the VZ (Burrows et al., 1997). Viruses included: controlvirus (titer: 1–2 x 10 ⁷cfu/ml), which expresses ${beta}$ -galactosidase( ${beta}$ -gal), and dominant-negative bone morphogenetic protein receptorIb (dnBMPRIb) virus (titer: 1–2 x 10 ⁷cfu/ml), which coexpresses ${beta}$ -gal (Lillien and Raphael, 2000). In experiments in which Shhsignaling was blocked, explants were cultured in the presenceof either a Shh neutralizing monoclonal antibody (5E1) (Ericsonet al., 1996) [diluted in 1:5; Developmental Studies HybridomaBank, (DSHB) Iowa City, IA] or different concentrations of cyclopamine(0.5, 5.0, and 10.0 µM; Toronto Research Chemicals Inc.,North York, Ontario, Canada). Cyclopamine at 5 µM wasfound to be the most effective. 5E1 or cyclopamine was addedto the culture medium daily. For controls, explants were exposedto culture supernatant containing a control antibody (anti-Pax6antibody) (DSHB) or DMSO. In some experiments recombinant FGF2(10 ng/ml; R & D Systems, Minneapolis, MN), recombinantBMP4 (10 ng/ml; R & D Systems) or unmodified recombinantShh-N (0.05, 0.5, or 5.0 µg/ml; R & D Systems) wasadded to cultures. After 4 d in culture, explants were dissociatedenzymatically using 0.1% trypsin (Sigma) in calcium and magnesium-freeHBSS for 15 min at 35°C. After trituration, the dissociatedcell suspensions were plated on poly-D-lysine (PDL) (Sigma)-coatedglass slides (1 x 10 ⁵ cells each in serum-free medium) for1 hr at 37°C before they were fixed and labeled with antibodies(see below). In some experiments, cells were dissociated after4 d in explant culture then grown as a monolayer on polyornithine-coatedcoverslips for 3 d in serum-free medium before they were stainedwith antibodies (Fig. 1 A'). Dissociation facilitates the removalof trophic factors added to the explants (such as FGF2, Shh)and accelerates differentiation.

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Figure 1. Dorsolateral progenitors generate more interneurons than dorsomedial progenitors in E11.5 telencephalic explants. A, Coronal sections from E11.5 mouse telencephalon were stained for GABA to show the extent of tangential migration of GABAergic neurons from the ganglionic eminences. This panel also illustrates how explants were dissected from different telencephalic regions. A', Explant cultures from E11.5 telencephalon were infected with a control retrovirus that expresses ${beta}$ -galactosidase. Four days later, the fate of infected cells was determined immunocytochemically 1 hr after dissociation (C, C', E, E', H, H', K, K'). Some of these dissociated cells were cultured as monolayers for an additional 3d (7 div total; D, D',F,F', I, I', L, L'). Cultures were stained with ${beta}$ -gal and either the general interneuron marker GABA (C', D', E, F), the early neuronal marker TuJ1 (E', F', H', I'), or the projection neuron marker glutamate (K',L'). Some of the dissociated cells were double labeled for TuJ1 and GABA at 4 (E, E') and 7 div (F, F') to confirm that all GABA+ cells were also TuJ1+, therefore neurons. Arrows in C, D, H, I, K, and L point to ${beta}$ -gal+ cells that are also labeled with a cell-type marker. Arrows in C', D', H', I', K', and L' show GABA+, TuJ1+ or glutamate+ cells, which are also ${beta}$ -gal+. Arrows in E show 2 GABA + cells, which are TuJ1 + (E'). Note that many of the TuJ1 + cells (E') are not immunoreactive for GABA (E). In F, arrows point to two of the five GABA+ cells, and F' indicates that these cells are also TuJ1+. *p < 0.0001, comparing dorsolateral progenitors to dorsomedial progenitors.

Aggregate cultures. Dorsomedial telencephalic wall and ganglioniceminence explants were dissected from E11.5 embryonic brains.To distinguish progenitor cells arising from the dorsomedialwall, "responding" explants (dorsomedial wall explants) were infectedwith control retrovirus as described above, whereas the "inducing"tissues (dorsomedial wall or GEs) remained uninfected. One dayafter infection, explants were dissociated enzymatically (seeabove), and an equal number of cells from infected and uninfectedexplants (2–3 x 10 ⁵ total cells) were mixed in 15 mlconical centrifuge tubes. Centrifugation was used to form anaggregate (Watanabe and Raff, 1990), and three aggregates percondition were transferred to nucleopore filters floating onserum-free medium. After 3 d in culture, aggregates were dissociatedand prepared for immunostaining as described for explants.
Immunocytochemistry. Dissociated cells plated on glass slidesor coverslips were fixed in 4% paraformaldehyde (PFA) in 0.1M phosphate buffer (PB), pH 7.4, or in 4% PFA in 3% PIPES bufferfor 10 min at room temperature. Cells were fixed with 4% PFAin 0.1 M PB and 0.1% glutaraldehyde (Sigma) to stain with anti-GABAantibody or 4% PFA in 0.1 M PB and 3% glutaraldehyde to stainwith monoclonal anti-glutamate antibody. After rinsing withPBS, cells were blocked in PBS containing 10% fetal bovine serum(FBS) (Invitrogen) and 0.1% Triton X-100. Cells were then incubatedin primary antibodies for 1 hr. The following primary antibodieswere used: rabbit anti- ${beta}$ -galactosidase (1:1000; Cortex Biochem,Inc., San Leandro, CA), mouse anti- ${beta}$ -galactosidase (1:200; Promega,Madison, WI), mouse anti-TuJ1 (1:400; Covance Research Products,Berkeley, CA), mouse anti-PCNA (1:100; Sigma), rabbit anti-GABA(1:2000; Sigma), mouse anti-GAD6 (1:2; DSHB), rabbit anti-glutamate(1:2000; Sigma), and mouse anti-glutamate (1:2000; Chemicon,Temecula, CA). Staining was visualized with fluorescent secondaryantibodies: donkey anti-mouse or anti-rabbit cy2 or cy3 (cy2:1:200, cy3: 1:800; Jackson ImmunoResearch, West Grove, PA).Secondary antibodies were applied for 30 min at room temperature.Finally, cells were rinsed in PBS and mounted in 95% glycerolin PBS. Fluorescent images were obtained using a Leica (Nussloch,Germany) DMR microscope. Sensys digital camera (PhotometricsLtd., Tuscon, AZ), IPLab, and Adobe Photoshop 6.0 software (AdobeSystems Inc., San Jose, CA).
Data collection and analysis. In each experiment 100 infectedcells ( ${beta}$ -gal+ cells) were counted per condition per antibody,and the proportion of neurons (TuJ1+), proliferating cells (PCNA+),excitatory neurons (glutamate+), or interneurons (GABA+ or GAD6+)was determined. At least three experiments were performed percondition. Data are represented as mean (%) ± SEM. Toverify whether differences between distinct conditions reachthe significance level p < 0.05, t tests were used.
Immunohistochemical staining of cortical sections. Cryostatsections (20 µm) were cut from E11.5 mouse brains. Afterfixation with 4% PFA in 0.1 M PBS, pH 7.4, in the presence of0.1% glutaraldehyde (Sigma) and blocking in PBS containing 10%fetal bovine serum (Invitrogen) and 0.1% Triton X-100, sectionswere incubated in primary antibody (rabbit anti-GABA, 1:2000;Sigma) overnight at 4°C. Sections were rinsed and incubatedin secondary antibody (donkey anti-rabbit cy2, 1:200; JacksonImmunoResearch) for 2 hr. The staining was photographed witha Leica DMR microscope using fluorescence optics.

   Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Regional differences in interneuron development
We wanted to investigate the generation of interneurons fromprogenitors in the dorsal telencephalic wall before the beginningof interneuron migration from the ventral telencephalon. Wealso wanted to determine whether there were regional differenceswithin the dorsal telencephalon in the capacity of progenitorcells to produce interneurons. To address these issues we usedexplants of E11.5 mouse telencephalon comparing medial and lateraldorsal telencephalic walls. Explants were dissected as indicatedin Figure 1A. To label proliferating cells in the dorsal telencephalicventricular zone, progenitors in explants were infected witha retrovirus that expresses the histochemical marker ${beta}$ -gal (Burrowset al., 1997). The phenotypes of the progeny of virus-infectedcells were determined either after acute dissociation of explantsafter 4 d in vitro (div) or after dissociation of 4 div explantsand culture as a monolayer for an additional 3 d (7 div total)(Fig. 1A'). Cells were double-labeled for the lineage marker ${beta}$ -gal to identify the virus infected cells (Fig. 1C,D,H,I,K,L)and either TuJ1, an early neuronal marker (Fig. 1E',F',H',I'),GABA, a general marker for inhibitory interneurons (Fig. 1C',D',E,F),or glutamate to label projection neurons (Fig. 1K',L').
In the dorsal telencephalon, lateral wall-derived progenitorcells generated significantly more GABAergic interneurons thandid progenitor cells in the medial telencephalic region after4dinexplant culture (Fig. 1B). When cells from dorsomedial (DM)or dorsolateral (DL) wall explants were dissociated after 4div and allowed to differentiate for an additional3das monolayers(7 div total) in the absence of exogenous growth factors, theproportion of interneurons was further increased, but medial-lateraldifferences in the generation of interneurons were still apparent(Fig. 1B). All GABA+ cells were also TuJ1+ at 4 and 7 div (Fig.1E,E',F,F'). To confirm the regional difference in interneurondevelopment, we used another well characterized marker of interneurons,GAD65 (Benson et al., 1994; Phelps et al., 1999), a synthesizingenzyme for GABA. At 7 div, 89.3 ± 1.8% of the GABA+ cellswere GAD+ (n = 4). The proportion of GAD+ cells among controlvirus-infected cells was higher laterally than medially (GAD+/ ${beta}$ -gal+: 26 ± 2.2% vs 50.3 ± 3.5%; medial vs lateral;7 div; n = 4; p = 0.002), confirming the results obtained usingGABA immunostaining to identify interneurons. None of the GABAergiccells showed any level of glutamate expression at 4 or 7 div,in either the control virus-infected or the uninfected populations(glutamate+/GABA+: 0 ± 0; n = 4).
There was no difference in the proportion of neurons after 7div (Fig. 1G), although DL telencephalic explants produced significantlymore neurons than did DM telencephalic explants after 4 div.This might reflect more extensive proliferation in DM than inDL telencephalic explants at 4 div (18.5 ± 1.4 vs 8.5± 0.5%; DM vs DL; n = 10; p < 0.0001), which delayedneuronal differentiation medially. Analyzing the productionof glutamatergic neurons revealed a complementary differencein their development compared with GABAergic neurons. By 7 divmore glutamatergic neurons were produced from DM-derived progenitorsthan from DL ones (Fig. 1J). None of the glutamatergic neuronswere GABA+ (GABA+/glutamate+: 0 ± 0; n = 3).
To determine whether the potential of dorsal telencephalic progenitorcells to generate interneurons is restricted to certain developmentalstages, we analyzed DM and DL telencephalic explants from E13and E16 embryonic brains after 4–7 div. We did not observean age-related decline in the competence of dorsal telencephalicprogenitor cells to produce interneurons. Moreover, more GABAergicneurons were produced from late progenitors than from earlyones. For example, when progenitor cells were labeled by controlvirus infection at E13, 38.8 ± 5.7% of DM progenitorsgenerated GABA+ neurons after 7 div, compared with 26.6 ±1.3% of E11.5 progenitors (p = 0.004). E13 DL progenitors alsoproduced a high proportion of interneurons after 7 div (55.7± 11.6%). Even at E16, 26 ± 1.8% of DL telencephalicwall progenitors expressed GABA after 4 d in explant cultures.
Ventral telencephalon enhances production of interneurons by DM telencephalic progenitors
The fact that DL telencephalic progenitors generated more interneuronsthan their medial counterparts raised the possibility that GEs,which are closer to DL cortex, produce a signal that promotesthe development of interneurons in the adjacent dorsal telencephalon.To determine whether ventral telencephalic signals can modulatethe production of interneurons by dorsal telencephalic progenitors,aggregates were formed from cells derived from DM telencephalicexplants and GEs (Fig. 2 A).

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Figure 2. Ventral telencephalic cells can induce the generation of interneurons from dorsomedial progenitors via Shh. A, Schematic diagram illustrates the experimental procedure by which aggregate cultures were prepared from ganglionic eminences and dorsomedial telencephalon. B, The proportion of GABAergic interneurons generated by ${beta}$ -gal+ dorsomedial progenitors was increased in cultures in which dorsomedial progenitors were cocultured with ganglionic eminence-derived cells (M*+GE), compared with the ones in which dorsomedial telencephalic cells were cultured alone (M*+M). Blocking Shh signaling with cyclopamine (5 µM; cyc) diminished interneuron production induced by GE (M*+GE+cyc). A ventrally derived signal or signals increased the proliferation of dorsomedial progenitors (C) and decreased neuronal differentiation (D), suggesting that it delayed neuronal differentiation by stimulating proliferation. These effects of ventral cells were also blocked by cyclopamine. *p = 0.04; **p $<=$ 0.009.

Progenitor cells from the medial wall of the dorsal telencephalonwere labeled with control retrovirus, whereas GE cells werenot infected. When E11.5 DM wall cells were mixed with cellsfrom GEs, we found that there was a 1.5-fold increase in theproportion of GABAergic neurons generated by DM progenitorscompared with progenitors in aggregates of DM wall alone (Fig.2B). This provided further support for the idea that local environmentalcues, rather than limited potential of progenitors, are responsiblefor the low production of interneurons in the DM telencephalonunder normal circumstances.
Blocking Shh signaling inhibits the interneuron-inducing effect of the ventral telencephalon
After observing that ventral telencephalon could promote interneurondevelopment by DM telencephalic progenitors, we wanted to identifythe factor or factors that could be responsible for this effect.Shh is a good candidate for mediating interneuron developmentfor several reasons. First, it is highly and specifically expressedin ventral telencephalon early in development (E11 and onward)(Kohtz et al., 1998; Sussel et al., 1999; Nery et al., 2001;Tekki-Kessaris et al., 2001). Second, cortical explants culturedin the presence of Shh start to express Dlx genes (Kohtz etal., 1998), which are believed to be essential for interneurondevelopment (Stuhmer et al., 2002). Third, Shh has been shownto increase the number of clones that contain GABAergic neuronsin cultures of FGF-expanded cortical progenitors (Yung et al.,2002).
To determine whether the interneuron-inducing effect of theventral telencephalon in aggregate cultures was mediated byShh, we blocked Shh signaling in these cultures. One day afteraggregates were formed from E11.5 DM telencephalic and GE cells,5 µM cyclopamine was added to cultures to block Shh signaling.Cyclopamine blocked the induction of interneurons by ventraltelencephalic cells (Fig. 2B). This provides further supportfor the idea that Shh produced by the ventral telencephalonpromotes the development of interneurons in the dorsal telencephalon.Cyclopamine also inhibited proliferation of DM wall progenitorsinduced by GE in aggregates (Fig. 2C), and increased the proportionof neurons to the level seen in cultures of DM alone (Fig. 2D).
Blocking endogenous Shh signaling in the dorsal telencephalon inhibits interneuron development
The experiments above demonstrated that ventral telencephaloncan promote the development of interneurons from DM telencephalicprogenitor cells, and that the induction depended on Shh. Shhis expressed in the dorsal telencephalon by E14 (Dahmane etal., 2001). At earlier stages of development, it has been reportedthat Shh may be expressed ectopically in explants of dorsaltelencephalon (Tekki-Kessaris et al., 2001). It is also possiblethat Shh produced by ventral telencephalon diffuses into moredorsal regions of the telencephalon even at early stages ofdevelopment (Incardona et al., 2000; Zeng et al., 2001). Todetermine whether "endogenous" Shh signaling contributes to interneurondevelopment in DL cortex, E11.5 DL explants were cultured inthe absence or presence of cyclopamine (Cooper et al., 1998;Incardona et al., 1998) or an Shh-neutralizing antibody (Ericsonet al., 1996). When Shh signaling was blocked with cyclopamine(5 µM), the proportion of GABAergic neurons in the DLtelencephalon was reduced at 4 and 7 div (Fig. 3A). A similareffect was observed with Shh neutralizing antibody (17.3 ±2.6 vs 11.0 ± 1.7%; control antibody vs anti-Shh antibody;after 4 div; n = 4; p = 0.02). Cyclopamine also reduced thegeneration of interneurons in DM telencephalic explants (9.3± 0.9 vs 6.0 ± 0.6%; DMSO vs cyclopamine; 4 div;n = 4; p = 0.007). When Shh was blocked, we noted a complementaryincrease in glutamatergic neurons compared with interneuronsat 4 and 7 div in DL explants (Fig. 3B). Blocking Shh signalingalso caused a decrease in proliferation (Fig. 3C), as reportedby Dahmane et al. (2001), but it did not lead to a significantdifference in the proportion of neurons at 4 and 7 div (Fig.3D). These results imply that Shh signaling is involved in thedevelopment of interneurons in the dorsal telencephalon andmay regulate the relative proportion of inhibitory and excitatoryneurons.

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Figure 3. Shh regulates the generation of interneurons from dorsal telencephalic progenitors. E11.5 dorsolateral and dorsomedial telencephalic explants were infected with control retrovirus expressing ${beta}$ -gal. A, The proportion of infected cells in the dorsolateral wall that expressed GABA decreased in the presence of cyclopamine (5µM), an inhibitor of Shh signaling. Cyclopamine was added to explants for 3 d (4 div total). Explants were dissociated and cultured for 3 more days as monolayers without cyclopamine (7 div total). B, A complementary increase in glutamatergic neurons was observed when cyclopamine was added to explants. C, Blocking Shh also decreased proliferation, but did not cause a significant change in the proportion of neurons (D). Adding recombinant Shh to dorsomedial telencephalic explants for 3 d (4 div total) increased the generation of interneurons (E). Exogenous Shh reduced neuronal differentiation at 4 div (H), which might be caused by increased proliferation (G). Cells from dissociated explants were also cultured as monolayers for 3 d without Shh (7 div total). The proportion of interneurons was still greater in cultures that had been exposed to Shh (E). The proportion of neurons was not different after 7 div, but the production of glutamatergic neurons showed a complementary decrease compared to GABAergic neurons in Shh-treated cultures (F). *p = 0.04; **p $<=$ 0.008; ***p = 0.0003.

Exogenous Shh can enhance interneuron generation by dorsomedial progenitors
The regional difference in interneuron development that we observedin the dorsal telencephalon is consistent with the idea thatventral telencephalic cells produce an inductive signal, mostlikely Shh, and the proximity of DL cortex to the source ofthis positive signal causes DL progenitors to produce more interneuronsthan their medial counterparts. Our results above suggestedthat DL cortex contained endogenous Shh, because adding cyclopamineto DL explant cultures could diminish the production of interneurons.This is also consistent with a previous study showing the presenceof Shh in E13.5 cortical explants (Tekki-Kessaris et al., 2001).If an insufficient level of Shh signaling is what prevents DMprogenitors from becoming interneurons with a higher frequency,then adding exogenous Shh to DM wall explants should increasethe probability that DM progenitors generate interneurons.
To address whether exogenous Shh can mimic the interneuron-inducingeffect of ventral telencephalon, DM telencephalic explants weredissected, and recombinant Shh was added to the cultures atdifferent concentrations: 0.05, 0.5, and 5 µg/ml. Shhat a concentration of 0.5 or 5.0 µg/ml increased the percentageof GABAergic interneurons after 4 d in explant culture (Fig.3E). It also stimulated proliferation (Fig. 3G), as reportedby Rowitch et al. (1999), raising questions about the ultimatefate of the dividing cells. Shh-treated progenitors still generatedmore interneurons than untreated cultures after 7 div (Fig.3E). A significant increase in GABA+ cells was also apparentin cultures treated with 0.05 µg/ml Shh as explants (after7 div: 24.8 ± 0.8% vs 39.5 ± 3.5%; untreated vsShh-treated; n = 4; p = 0.01). The percentage of neurons wasnot altered after 7 div (Fig. 3H); however, there was a complementaryreduction in glutamatergic neurons in the Shh-treated cultures(Fig. 3F). These data support the idea that Shh promotes thedevelopment of interneurons and that Shh levels in the DM telencephalonare suboptimal for interneuron generation.
BMP inhibits interneuron generation from dorsolateral telencephalic progenitor cells
Although a limiting concentration of Shh in the dorsal telencephalon,particularly the DM region, could account for regional differencesin interneuron development, inhibitors in the DM wall couldalso be involved in regulation of interneuron differentiation.BMPs are normally expressed at higher levels in the DM wall(Furuta et al., 1997; Grove et al., 1998) and antagonize Shhsignaling in many tissues (Ericson et al., 1995; Liem et al.,1995; Watanabe et al., 1998; Zhu et al., 1999). To test theeffect of BMP on interneuron development, DL telencephalic explantswere dissected from E11.5 mouse brains, and BMP4 was added tothe cultures. Application of BMP4 decreased the proportion ofinterneurons at 4 and 7 div (Fig. 4A). There was also a decreasein proliferation after treatment with BMP4 (Fig. 4B), as reportedby others (Kalyani et al., 1998; Mabie et al., 1999; Zhu etal., 1999), although neuronal differentiation was not altered(Fig. 4C). These results suggest that increasing the level ofBMP in the DL telencephalon causes DL progenitors to behavemore like DM progenitors with respect to interneuron generation.This supports the idea that a dorsomedially derived inhibitorsuppresses interneuron development in the dorsal telencephalon.When Shh was added to DM telencephalic explants, it could overcomethis inhibition; however, when BMP4 was added together withShh (Shh+BMP), BMP inhibited the inductive effect of Shh (Fig.4 D). This implies that the balance between Shh and BMP4 concentrationsdetermines the proportion of interneurons generated.

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Figure 4. BMP4 inhibits the generation of interneurons. A–C, Dorsolateral telencephalic explants were infected with control virus expressing ${beta}$ -gal at E11.5 and cultured in the absence or presence of BMP4 (10 ng/ml) for 3 d (4 div total). After 4 div the proportion of GABA+ (A), PCNA+ (B), or TuJ1+ (C) cells was determined among the virus-infected, ${beta}$ -gal+ cells. Cells from dissociated explants were also cultured as monolayers for 3 d without BMP4 (7 div total). Dorsolateral telencephalic progenitors generated fewer interneurons (A), approximately equal proportions of neurons (C), and divided less extensively (B) after explants were treated with BMP4 compared with untreated explants. D, E11.5 dorsomedial telencephalic explants were infected with control virus and cultured in Shh alone (0.5 µM) or Shh+BMP4 (0.5 µM Shh; 10 ng/ml BMP4) for 3 d (4 div total). Explants were dissociated, cultured as monolayers without exogenous factors, and the proportion of GABAergic neurons was determined 3 d later (7 div total). Shh alone induced the production of interneurons, but BMP4 inhibited the interneuron-inducing effect of Shh. *p $<=$ 0.03; **p $<=$ 0.0006.

Blocking BMP signaling increases the generation of GABAergic interneurons from dorsomedial telencephalic progenitor cells
To confirm that the DM signal that limits interneuron developmentnormally is BMP, DM telencephalic explants were dissected fromE11.5 embryos and infected with a retrovirus transducing dominant-negativeBMPRIb (dnBMPRIb) and ${beta}$ -gal (Lillien and Raphael, 2000) or controlvirus. DnBMPRIb and control retrovirus-infected explants werecultured for 4 d before they were dissociated and either processedfor immunocytochemistry or allowed to differentiate for 3 moredays (7 div total). In acutely dissociated explant culturesthere was no significant difference in the proportion of interneuronsbetween control and dnBMPRIb-infected cells, however when thesecells were allowed to differentiate further, dnBMPRIb-infectedcells produced considerably more GABAergic interneurons thancontrol virus-infected cells (Fig. 5A). A comparable differencebetween control and dnBMPRIb virus-infected DM cells was observedusing GAD antibody to distinguish interneurons (GAD+/ ${beta}$ -gal+:26± 2.2% vs 51 ± 4.6%; control vs dnBMPRIb virus;7 div; n = 4; p = 0.002). In contrast to DM progenitors, whenDL progenitors were infected with dnBMPRIb or control virus,we could not see a significant increase in the proportion ofinterneurons generated from dnBMPRIb-infected progenitors (39.3± 3.2 vs 46.0 ± 3.8%; control virus vs dnBMPRIbvirus; 7 div; p = 0.25). This observation further supports theidea that an interneuron-inhibiting signal is most abundantor active in the DM telencephalon. As noted previously, dnBMPRIbvirus increased proliferation (Fig. 5B) (Lillien and Raphael,2000) and reduced differentiation into neurons in explant cultureat 4 div (Fig. 5C). However, after the dissociated cells differentiatedfor 3 more days (7 div total) in the absence of exogenous mitogens,the proportion of neurons generated from dnBMPRIb-infected cellsapproached that seen in control-infected cultures (Fig. 5C).The percentage of glutamatergic neurons was reduced among cellsinfected with dnBMPRIb virus (Fig. 5D), suggesting a complementarychange in interneurons and projection neurons. These observationsfurther support the idea that endogenous BMPs normally inhibitthe production of interneurons in the dorsal telencephalon,particularly in the DM wall.

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Figure 5. Blocking BMP signaling promotes the production of interneurons. Dorsomedial telencephalic progenitors were infected with control ( ${beta}$ -gal) or dnBMPRIb (coexpressing ${beta}$ -gal) retrovirus at E11.5, and their progeny were analyzed after 4 and 7 div. Blocking BMP in dorsomedial progenitors caused a remarkable increase in interneuron differentiation after 7 div (A), together with a complementary decrease in the percentage of glutamatergic neurons (D). B, Blocking BMP increased proliferation after 4 div in explants. C, Neuronal differentiation was initially reduced if BMP was blocked, consistent with increased proliferation. At 7 div, however, the percentage of neurons among dnBMPRIb and control virus-infected cells was not different. *p < 0.05; **p $<=$ 0.005; ***p $<=$ 0.0009.

Proliferation does not regulate interneuron production
Experiments modifying BMP or SHH signaling suggested a correlationbetween changes in the proportion of proliferating cells andin the proportion of interneurons generated: BMPs decreasedproliferation and also reduced interneurons, whereas Shh anddnBMPRIb had mitogenic effects on telencephalic progenitor cellsand increased interneuron development. These observations raisedthe possibility that increased proliferation is responsiblefor the increase in interneurons. The proliferation stimulatingeffect of fibroblast growth factor 2 (FGF2) is well documented(Gensburger et al., 1987; Tao et al., 1996; Cavanagh et al.,1997; Raballo et al., 2000), therefore we wanted to test whetheradding exogenous FGF2 to dorsal telencephalic cultures wouldalso induce interneurons. FGF2 (10 ng/ml) was added to DM orDL telencephalic explants, and the proportion of total neurons,interneurons, and glutamatergic neurons was determined eitherafter 4 d in explant culture or 3 d after dissociation and cultureof cells as a monolayer in the absence of exogenous FGF2 (7div total). In DM and DL wall explants, FGF2, like Shh, increasedproliferation (Fig. 6A,B). Unlike Shh, however, FGF2 did notincrease the production of interneurons from DM progenitorsafter 4 or 7 div (Fig. 6C). In explants of DL wall, FGF2 actuallyreduced the production of interneurons (Fig. 6D) and increasedthe generation of glutamatergic neurons after 7 div (Fig. 6F).We did not observe a change in the proportion of glutamatergicneurons generated from DM progenitors (Fig. 6E). Neuronal differentiationwas reduced in both DM and DL explants after 4 div, presumablybecause of the increase in proliferation that delayed differentiation.After 7 div a small reduction in neurons was still observedin DL but not DM explants (Fig. 6G,H). These results indicatethat proliferation per se does not control the generation ofinterneurons.

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Figure 6. FGF2 does not induce interneurons in explant cultures. Progenitor cells from E11.5 dorsomedial (DM) and dorsolateral (DL) telencephalic walls were infected with a control retrovirus, cultured as explants in the absence or presence of FGF2 (10 ng/ml) for 3 d (4 div total), and the proportions of proliferating cells, interneurons, projection neurons, and total neurons were determined (4 div). Explants were also dissociated and cultured for an additional 3 d in monolayer cultures in the absence of FGF2 (7 div total). FGF2 did not induce interneurons in DM telencephalic explants (C) and decreased interneuron development in DL telencephalic explants after 7 div (D). Neuronal differentiation was reduced in both DM and DL explant cultures at 4 div after treatment with FGF2 (G, H), probably because of increased proliferation in these cultures (A, B). A small decrease in the percentage of neurons was maintained in FGF2-treated DL cells after 7 div, but not in DM cells (H, G). FGF2 promoted development of glutamatergic neurons in DL, but not in DM cultures (E, F). *p < 0.05; **p $<=$ 0.005.

DnBMPRIb does not act via Shh to regulate interneuron production
In a previous study, we showed that blocking BMP signaling byinfection with a dnBMPR1b virus promoted the maturation of VZprogenitors to a subventricular zone (SVZ) state by a cell nonautonomousmechanism (Lillien and Raphael, 2000). We recently showed thatthis effect of dnBMPRIb virus was mediated by Shh (Viti et al.,2003). To determine whether Shh mediates the effect of dnBMPRIbvirus on interneuron development, we added cyclopamine to blockShh in explants of DM telencephalon infected with dnBMPRIb virus.In contrast to regulation of SVZ development, Shh does not appearto mediate the effect of dnBMPRIb virus on interneuron development.For example, the proportion of GABA+ cells induced by blockingBMP was not reduced when Shh was blocked simultaneously in DMtelencephalic explants (Fig. 7A). Blocking Shh did eliminatethe transient reduction in neurons seen at 4 div among dnBMPR1b-infectedcells (Fig. 7B) and reduction in glutamatergic neurons (Fig.7C). The absence of a reduction in interneurons when BMP andShh signaling were blocked simultaneously suggests that BMPmight inhibit the development of interneurons nonautonomouslyby blocking an as yet unidentified signal that, like Shh, canpromote interneuron development. Alternatively, BMP might actcell-autonomously to block the production of interneurons.

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Figure 7. Blocking BMP does not stimulate interneuron generation via Shh. E11.5 dorsomedial telencephalic explants were infected with dnBMPRIb or a control retrovirus and cultured in the absence or presence of cyclopamine (5 µM) for 3 d (4 div total). Explants were dissociated and cultured for 3 d as monolayers (7 div total). The phenotype of infected cells was analyzed after 4 and 7 div. A, Blocking BMP promoted the generation of interneurons, but blocking Shh simultaneously could not diminish this increase. Inhibiting BMP reduced the proportion of neurons after 4 div (B) and the proportion of glutamatergic neurons (C). The effects of the BMP block on total neurons and glutamatergic neurons were inhibited by cyclopamine, unlike the effect of BMP block on interneuron generation. *p < 0.05; **p = 0.0001.

   Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

In vivo studies indicated that most interneurons in rodentsare generated in the ventral telencephalon, although they leftopen the possibility that some interneurons originate from dorsaltelencephalic progenitors (Anderson et al., 1997a). Studiesin vitro have demonstrated that dorsal progenitors are competentto generate interneurons. In the present study we addressedthe possible mechanisms underlying the disparity between invitro competence and in vivo behavior. We demonstrate that Shhcan induce interneuron development in explants of dorsal telencephalon.Moreover, endogenous BMPs inhibit the generation of interneuronsdorsally. Shh is predominantly expressed in the ventral telencephalon,whereas the highest expression of BMPs is observed dorsally.These findings suggest that an insufficient level of Shh and/orthe inhibitory effect of BMPs normally reduce the probabilitythat dorsal telencephalic progenitors become interneurons.
Shh promotes interneuron development from dorsal telencephalic progenitors
Several lines of evidence support the idea that Shh promotesthe production of interneurons in the telencephalon. First,early in development Shh is expressed specifically by ventraltelencephalic cells (Kohtz et al., 1998; Nery et al., 2001).In vivo at this developmental stage GABAergic interneurons arelocalized to the ventral telencephalon (Fig. 1A), thereforeShh expression and the site of interneuron development colocalize.Second, in aggregate cultures of E11.5 DM and ventral telencephalon,ventral cells induce interneuron development from dorsal progenitors,and this can be blocked by cyclopamine (Fig. 2B). Third, ifrecombinant Shh is added to E11.5 cortical explants, it canmimic the interneuron-inducing effect of the ventral telencephalon(Fig. 3E). This is consistent with the findings of a recentpublication in which Shh was shown to promote interneuron developmentin monolayer cultures of FGF2-treated cortical progenitors (Yunget al., 2002).
Shh expression is not restricted to ventral regions of the CNS,becoming apparent in the dorsal telencephalon around E14 (Dahmaneet al., 2001). In explant cultures dissected from E11.5–E16dorsal telencephalon, progenitors gave rise to a significantproportion of GABAergic interneurons. This could be caused bythe ectopic expression of Shh in E11.5 explant cultures (Albertaet al., 2001; Tekki-Kessaris et al., 2001), although Shh couldbe present at later ages (Dahmane et al., 2001). If Shh is presentin the dorsal telencephalon later in development and it canpromote interneuron development, one would expect that at leastlate cortical progenitors might give rise to interneurons. Severalobservations support this possibility. For example, Letinicet al. (2002) showed that in organotypic slice cultures of humanembryonic forebrain, cortical VZ/SVZ cells could differentiateinto interneurons, and it has been suggested that a subpopulationof interneurons that expresses calretinin might arise from thecortical SVZ at later stages of embryonic mouse development(Xu et al., 2003).
If early cortical progenitors do not generate interneurons normally,but later gestation and early postnatal progenitors may giverise to interneurons (Xu et al., 2003), it raises the possibilitythat progenitor maturation is involved in interneuron development.A recent study from our laboratory demonstrated that Shh couldpromote the maturation of VZ progenitors to an SVZ state, characterizedby expression of a higher level of EGFRs among a subset of progenitors(Viti et al., 2003). One possibility is that Shh induces interneuronsin the dorsal telencephalon by promoting the VZ–SVZ transitionvia EGFR induction and biases SVZ progenitors toward generatingGABAergic interneurons. FGF2 also promotes the development ofan EGFR+ subset of progenitors (Lillien and Raphael, 2000).FGF2, however, does not increase the development of interneuronsfrom dorsal telencephalic progenitors in our hands (Fig. 6C,D).It is not known whether FGF2- and Shh-induced SVZ progenitorsdiffer in their potential to give rise to neurons versus glialcells or to subtypes of neurons. It is possible that FGF2-inducedSVZ progenitors are biased to become projection neurons or astrocytes(Levison and Goldman, 1993; Tarabykin et al., 2001; Tramontinet al., 2003), whereas Shh-induced SVZ progenitors are biasedto generate interneurons or oligodendrocytes (Orentas et al.,1999). It is also possible that EGFR+ cells are not obligatoryprecursors of interneurons, because interneuron induction couldbe elicited at lower concentrations of Shh than upregulationof EGFR expression (A. Gulacsi, unpublished observations). Therelationship between EGFR expression and interneuron generationremains to be clarified, but it should be noted that progenitorsin the rostral migratory stream that give rise to olfactorybulb interneurons express a high level of EGFRs (Eagleson etal., 1996; Doetsch et al., 2002).
It has been shown that most if not all cortical interneuronsexpress Dlx (Anderson et al., 1997b; Letinic et al., 2002) andthat expression of Dlx genes in the dorsal telencephalon caninduce GAD65 expression, characteristic of interneurons (Stuhmeret al., 2002). Shh was shown to induce Dlx expression in thedorsal telencephalon, however there was a temporal restrictionin the competence of dorsal progenitors to exhibit this responseto Shh (Kohtz et al., 1998). It is unlikely, however, that dorsalprogenitors lose their capacity to generate interneurons duringembryonic development. For example, we found that progenitorsfrom E13 and E16 cortical explants can still differentiate intointerneurons. The competence of later progenitors to produceinterneurons is also consistent with their derivation from SVZprogenitors (Xu et al., 2003).
Several studies of Shh misexpression in the dorsal domain ofthe CNS have shown that Shh induces oligodendrocytes (Poncetet al., 1996; Pringle et al., 1996; Orentas et al., 1999). Forexample, when mouse embryos were infected with a Shh-expressingretrovirus at E9.5, the majority of infected cells became oligodendrocytesby postnatal day 21 (P21) (Nery et al., 2001). A general decreasein neurons was also observed, however the subtypes of neuronswere not reported. The results of that study could be interpretedto suggest that Shh does not induce interneurons in vivo inthe dorsal telencephalon. An alternative interpretation, however,is that during the 4 week interval between injection and analysis,oligodendrocyte progenitors may have divided more extensivelythan those of interneurons, masking an effect of Shh on interneurons.
BMPs normally suppress interneuron development
BMP4 is expressed in the dorsomedial telencephalon (Furuta etal., 1997; Mehler et al., 1997), although BMP4 immunoreactivityhas also been detected in the lateral telencephalic wall (Liet al., 1998). In many tissues BMPs antagonize responses toShh (Ericson et al., 1995; Mekki-Dauriac et al., 2002), thereforethey represent a reasonable candidate for inhibiting interneurongeneration dorsally. Our study shows that exogenous BMP4 decreasesinterneuron development from dorsal progenitors and antagonizestheir induction by Shh (Fig. 4A,D), while blocking endogenousBMP signaling with a virus expressing dnBMPRIb increases thegeneration of interneurons (Fig. 5A). The inhibitory effectof BMP contradicts a recent study in which it was found thatBMP and Shh interact cooperatively to promote interneuron specification(Yung et al., 2002). In that study Shh and BMP2 were added tomonolayer cultures of FGF2-primed E12.5 cortical progenitors.In contrast, we used explant cultures, in which cell–cellinteractions are maintained, as in the in vivo environment.Moreover, our cultures were not primed with FGF2, which canalter properties of progenitors (Lillien and Raphael, 2000).These differences in culture preparations might account forthe difference in the effect of BMP on interneurons we observed.
How might extrinsic factors act to regulate interneuron development?
Several mechanisms could underlie the regulation of interneurondevelopment by Shh and BMP. For example, Shh could promote interneurongeneration by suppressing the inhibitory effect of BMPs (Fig.4D). Shh has been shown to antagonize BMP signaling at severallevels (Zhu et al., 1999; Mekki-Dauriac et al., 2002). FGF2has also been shown to antagonize BMP signaling in other systemsas well as in embryonic cortex (Lillien and Raphael, 2000; Andersonet al., 2002). If just inhibiting BMP signaling was sufficientto induce interneurons, then FGF should mimic the effect ofShh on interneuron development. Our findings showed that thisis not the case.
An alternative mechanism to explain the antagonistic effectof BMP and Shh on interneuron development is that generationof interneurons is regulated by proliferation. BMPs inhibitproliferation, whereas blocking BMP signaling or adding Shhstimulates proliferation, and these changes in proliferationare correlated with changes in the percentage of interneurons.FGF2 also stimulates proliferation but it does not promote thegeneration of interneurons, therefore a proliferation-basedmechanism is not likely.
Shh was recently shown to maintain the survival of neuroepithelialcells by preventing Ptc-1-induced apoptotic cell death (Thibertet al., 2003). It is not likely that changes in interneurongeneration were attributable to the selective survival or deathof interneurons, because changes in interneurons were usuallycoupled to complementary changes in glutamatergic neurons, andthe overall number of neurons was not altered.
We showed previously that blocking BMP signaling with a dnBMPRIbvirus promoted the development of EGFR+ SVZ progenitors viaShh (Lillien and Raphael, 2000; Viti et al., 2003). In contrast,in the present study we found that Shh does not mediate interneurondevelopment induced by blocking BMP with dnBMPRIb (Fig. 7A).This suggests that BMP does not inhibit interneuron generationsimply by inhibiting Shh and that Shh may not be required forgeneration of interneurons. An Shh-independent mechanism thatis also antagonized by BMPs may promote the generation of interneurons,as noted for the generation oligodendrocytes (Nery et al., 2001).Alternatively, BMPs may act directly to inhibit the generationof interneurons by a mechanism that cannot be blocked by FGF2.

   Footnotes

Received July 9, 2003; revised September 18, 2003; accepted September 22, 2003.
This work was supported by National Institutes of Health GrantNS38306. We thank Jennifer Phillips and Kristi Weigle for technicalassistance and Amy Sinor and Dr. Stewart Anderson for theircomments on this manuscript.
Correspondence should be addressed to Dr. Laura Lillien, Departmentof Neurobiology and Pittsburgh Cancer Institute, Universityof Pittsburgh School of Medicine, W1454 Biomedical Science Tower,Pittsburgh, PA 15261. E-mail: lillien+{at}pitt.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/239862-11$15.00/0

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