Mammalian BarH1 Confers Commissural Neuron Identity on Dorsal Cells in the Spinal Cord

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The Journal of Neuroscience, March 15, 2003, 23(6):1987

BRIEF COMMUNICATION
Mammalian BarH1 Confers Commissural Neuron Identity on Dorsal Cells in the Spinal Cord
Rie Saba¹^,², Norio Nakatsuji², and Tetsuichiro Saito²
¹ Department of Genetics, The Graduate University for Advanced Studies, National Institute of Genetics, Mishima, Shizuoka 411-8540, Japan, and ² Department of Development and Differentiation, Institute for Frontier Medical Sciences, Kyoto University, Kyoto 606-8507, Japan

  ABSTRACT

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
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Commissural neurons in the spinal cord project their axons through the floor plate using a number of molecular interactions,such as netrins and their receptor DCC (deleted in colorectalcancer). However, the molecular cascades that control differentiationof commissural neurons are less characterized. A homeobox gene,MBH1 (mammalian BarH1) was expressed specifically in a subsetof dorsal cells in the developing spinal cord. Transgenic micethat carried lacZ and MBH1-flanking genome sequences demonstratedthat MBH1 was expressed by commissural neurons. To analyze thefunction of MBH1, we established an in vivo electroporation methodfor the transfer of DNA into the mouse spinal cord. Ectopic expressionof MBH1 drove dorsal cells into the fate of commissural neuronswith concomitant expression of TAG-1 (transiently expressed axonalsurface glycoprotein 1) and DCC. Cells ectopically expressingMBH1 migrated to the deep dorsal horn, in which endogenous MBH1-positivecells accumulated. These results suggest that MBH1 functions upstreamof TAG-1 and DCC and is involved in the fate determination ofcommissural neurons in the spinalcord.

Key words: MBH1; homeobox; homeodomain; in vivo electroporation; TAG-1; DCC

  Introduction

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Introduction
Materials and Methods
Results
Discussion
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Commissural neurons in both vertebrates and invertebrates transfer information from one side of their bodies to the otherthrough the midline. Molecular mechanisms regulating axon guidanceof these neurons have been characterized extensively (Tessier-Lavigneand Goodman, 1996; Mueller, 1999; Kaprielian et al., 2001). Netrinsand DCC (deleted in colorectal cancer) play a pivotal role inaxon guidance. Some commissural neurons are generated in the developingdorsal spinal cord, in which domains of progenitor cells are specifiedby helix-loop-helix (HLH) transcription factors (Gowan et al.,2001). The domains are initially established by TGF- $beta$ -like signals(Liem et al., 1997) and produce several cell types, which aredefined by combinatorial expression of homeobox genes (Lee andJessell, 1999; Gross et al., 2002; Muller et al., 2002). The mostdorsal cell type, dI1 (D1), is generated by an HLH factor, MATH1(mouse atonal homolog 1). dI1 cells and a subset of commissuralneurons are lost in MATH1 knock-out mice (Bermingham et al., 2001;Gowan et al., 2001), whereas ectopic expression of MATH1 increasesthe number of dI1 cells (Gowan et al., 2001). However, the molecularcascades that form the link between the generation of the cellsand their migration-axon guidance remain to bedetermined.

Bar-class homeobox (BarH) genes function in the development of various organs. Drosophila BarH genes control the developmentof the retina (Higashijima et al., 1992a) and peripheral nervoussystem (Higashijima et al., 1992b). A mammalian BarH gene, MBH1,is expressed at early stages of neurogenesis and is a potentialregulator of neural HLH genes in the diencephalon (Saito et al.,1998). Outside of the diencephalon, MBH1 is expressed by postmitoticneurons in the midbrain, hindbrain, spinal cord, and retina (Saitoet al., 1998, 2000). Another mammalian BarH gene, MBH2/Barhl1,is also expressed in the spinal cord (Bulfone et al., 2000; Saitoet al., 2000) and suggested to be a downstream gene of MATH1 (Berminghamet al., 2001). Xenopus BarH genes, XBH1 and XBH2, which are orthologsof MBH1 and MBH2, respectively, show distinct expression patterns(Patterson et al., 2000). Expression patterns of MBH1 and MBH2are similar but not identical (Saito et al., 2000), suggestingthat expression of the two genes may be controlled by differentmechanisms.

In this paper, we made transgenic mice carrying lacZ with the MBH1-flanking sequences and examined the cell types of MBH1-expressingcells in the developing mouse spinal cord. The function of MBH1has been revealed using the in vivo electroporationmethod.

  Materials and Methods

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Introduction
Materials and Methods
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Generation and analysis of transgenic mice. The MBH1-flanking sequences were obtained by screening a 129/SvJ mouse genomiclibrary (Stratagene, La Jolla, CA) using the entire sequence ofthe MBH1 cDNA (GenBank accession number AB004056) as a probe.We made a construct that carried the lacZ-coding region from BGZA(Yee and Rigby, 1993; Helms et al., 2000) between the 1 kb 5'and 2.5 kb 3' sequences flanking the MBH1-coding region. BGZAwas a gift from Dr. J. Johnson (University of Texas SouthwesternMedical Center, Dallas, TX). Transgenic mice were generated bystandard procedures (Hogan et al., 1986) using fertilized eggsfrom B6C3F1 (C57BL/6 × C3H) crosses. Staged transgenic embryoswere dissected in cold PBS and fixed in 4% paraformaldehyde. Wholemount 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside stainingof the embryos was performed as described previously (Verma-Kurvariet al., 1996). Other constructs that carried longer MBH1-flankingsequences also demonstrated the same lacZ expression pattern asthe above construct, recapitulating endogenous MBH1 expression.After staining, the embryos were postfixed and embedded in paraffin.Microtome sections (7 µm) were stained with Nuclear Fast Red (VectorLaboratories, Burlingame, CA). For immunostaining, fixed embryoswere embedded in OCT compound and sliced at 14 µm using acryostat.

In vivo electroporation. Exo utero surgery and electroporation were performed as described previously (Saito and Nakatsuji,2001). pCAG-EYFP (enhanced yellow fluorescent protein), whichcarried EYFP downstream of a CAG promoter (Saito and Nakatsuji,2001), was used as a control. To express both EYFP and MBH1 inthe same cells, pEYFP-MBH1 was constructed by inserting the MBH1-codingregion downstream of the second CAG promoter of pCAG-EYFP-CAG(Saito and Nakatsuji, 2001). One microliter of DNA solution (140nM) in PBS was injected into the central canal of the spinal cord.Five electric pulses at 22 V were delivered to the spinal cordby holding embryos with forceps-type platinum electrodes. Twokinds of electrodes, half-ring type (see Fig. 2A) and round-platetype with a 3 mm diameter (http://www.frontier.kyoto-u.ac.jp/rc01/in_vivo_electroporation.html),were used for gene transfer into the whole and a part of the spinalcord, respectively. The electric pulses were obtained from anelectroporator, CUY21EDIT (Nepa Gene, Ichikawa, Japan). Survivaland EYFP-positive (EYFP⁺) rates, which were calculated from surviving embryos/operatedand EYFP⁺ spinal cords/surviving embryos, were 56.7 ± 4.6 and 79.9 ± 2.7%,respectively. For functional analysis of genes, each result wasconfirmed by using another independently isolated clone with thesamestructure.

In situ hybridization and immunohistochemistry. In situ hybridization was performed as described previously (Saito et al.,1996). Antisense RNA probes were synthesized from plasmids carryingmouse cDNA clones: pMH4-1 for MBH1 and generous gifts from Dr.T. Jessell (Columbia University, New York, NY) for LH2B (a LIMhomeobox gene), Dr. R. Kageyama (Kyoto University, Kyoto, Japan)for MATH1, and Dr. Q. Ma (Harvard Medical School, Boston, MA)for Ngn2 (neurogenin 2). Frozen sections were incubated with thefollowing primary antibodies: 4D7 [anti-TAG-1 (transiently expressedaxonal surface glycoprotein 1)], AF5 (anti-DCC; Calbiochem, LaJolla, CA), 40.2D6 [anti-Isl1 (Islet-1)], 4F2 [anti-Lim1/2 (ahomeodomain protein)], rabbit polyclonal L1 (anti-LH2A/B, giftfrom Dr. Jessell), goat anti- $beta$ -galactosidase ( $beta$ -gal) (Biogenesis,Kingston, NH), and rabbit anti-GFP (Molecular Probes, Eugene,OR). 4D7, 40.2D6, and 4F2 were obtained from the DevelopmentalStudies Hybridoma Bank (University of Iowa, Iowa City, IA). Signalswere visualized by the following secondary antibodies: donkeyanti-rabbit IgG, anti-mouse IgG, or anti-mouse IgM conjugatedwith Cy3 or FITC (Jackson ImmunoResearch, West Grove, PA); anddonkey anti-goat IgG conjugated with Alexa Fluor 488 (MolecularProbes). Immunofluorescent studies were performed as describedpreviously (Saito and Nakatsuji, 2001).

  Results

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Introduction
Materials and Methods
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MBH1 expression marked a subset of cells in the spinal cord

Expression of MBH1 was detected in the mouse dorsal spinal cord at embryonic day 10.5 (E10.5) (Fig. 1A). At E11.5, the expressionexpanded ventrally to the deep dorsal horn (Fig. 1C). Later thanE12.5, the expression was mainly restricted to the deep dorsalhorn (Fig. 1E). The pattern of the expression during developmentresembled that of ventral migration of some dorsal neurons (Leberand Sanes, 1995), suggesting that MBH1 was expressed by thesemigrating neurons. A stream of cells between the deep dorsal hornand the floor plate also expressed MBH1 at E12.5 (Fig. 1E, arrows).MBH1 expression in the ventral spinal cord became confined toa group of cells dorsolateral to the floor plate at later stages(see Fig. 4B), suggesting that MBH1⁺ cells in the stream are under ventromedial migration at E12.5.

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Figure 1. MBH1 expression in the developing mouse spinal cord. Transverse sections at brachial levels of embryos at E10.5 (A, B), E11.5 (C, D) and E12.5 (E, F) were hybridized with antisense cRNA probes for MBH1 (A, C, E) and immunostained using an anti- $beta$ -gal antibody (B, D, F). Embryos carrying the MBH1/lacZ transgene were used (B, D, F-H). Arrows indicate streams of MBH1⁺ cells between the deep dorsal horn and the floor plate. Control hybridization using a sense-strand probe of MBH1 gave no specific signals (data not shown). Similar expression patterns of MBH1 were observed from cervical to lumbar levels. G, Transverse section of the E10.5 spinal cord was stained with antibodies against the $beta$ -gal (green) and LH2A/B proteins (red). H, Double-label immunostaining with the anti- $beta$ -gal (green) and anti-TAG-1 (red) antibodies of the E11.5 spinal cord. Filled and open arrowheads indicate $beta$ -gal⁺ axons and ventral funiculi, respectively. Scale bars: (in A) A, C, E, 200 µm; B, D, F-H, 100 µm.

Characterization of MBH1-expressing cells

To examine which types of cells expressed MBH1, transgenic mice with lacZ under the control of the MBH1-flanking DNA sequenceswere generated. The transgenic mice expressed the lacZ product $beta$ -gal in a pattern recapitulating endogenous MBH1 expression (Fig.1B,D,F). Coexpression of MBH1 and lacZ was confirmed by immunostainingusing an anti-MBH1 antibody (data not shown). All $beta$ -gal⁺ cells were labeled with antibodies against the LH2A/B proteins(Fig. 1G), a marker of dI1 cells, but not with antibodies againstthe Isl1 and Lim1/2 proteins (data not shown), suggesting thatMBH1 is expressed by dI1cells.

Because the $beta$ -gal protein spreads throughout the cytoplasm, it enabled us to examine the morphologies of MBH1⁺ cells. $beta$ -gal⁺ signals were detected in axons projecting to the floor plateand ventral funiculi (Fig. 1H). The $beta$ -gal⁺ axons were labeled with specific markers of commissural neurons,anti-TAG-1 and anti-DCC antibodies (Fig. 1H; data not shown).These results indicate that MBH1 is expressed by commissuralneurons.

In vivo electroporation into the spinal cord

To examine the function of MBH1, we established a system for the forced expression of a gene in the mouse spinal cord by modifyingour in vivo electroporation method to the brain (Saito and Nakatsuji,2001). The uterine wall was cut to see embryos clearly, and DNAwas injected into the central canal of the spinal cord (Fig. 2).Then electric pulses were applied to the spinal cord using half-ring-typeelectrodes (Fig. 2A). The electrodes helped better survival ofembryos by limiting electric pulses mainly onto the spinal cord.After electroporation, a reporter gene, EYFP, was expressed onlyin one side of the spinal cord (Fig. 2B,C).

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Figure 2. DNA transfer into the mouse spinal cord by in vivo electroporation. A, Schematic representation of DNA injection and electrodes. EYFP was introduced into the E11.5 spinal cord. B, Dorsal view of an embryo at E13.5, 2 d after electroporation. C, Semi-illuminated view of B. EYFP was expressed in only one side of the spinal cord closer to the anode. Scale bars: 2 mm.

Ectopic expression of MBH1

Using this system, pEYFP-MBH1, which carried both the EYFP and MBH1 genes downstream of ubiquitous CAG promoters, was introducedinto the E11.5 mouse spinal cord. At this stage, DNA will be takenup by cells that are not fated to express MBH1 for the followingtwo reasons: (1) endogenous MBH1⁺ cells are away from the ventricle (Fig. 1C), and (2) DNA is transferredto cells adjacent to the ventricle by this method (Saito and Nakatsuji,2001). DNA will be also introduced mainly into dorsal cells, becausethe central canal is wider in the dorsal side. Transfection withEYFP alone as a control mostly labeled only dorsal cells, as expected(Fig. 3A). In contrast, more ventral EYFP⁺ cells were generated by coexpression with MBH1 (Fig. 3B, arrows).The ventral EYFP⁺ cells had morphologies similar to some commissural neurons (Silos-Santiagoand Snider, 1992). Transfection of MBH1 also produced more EYFP⁺ commissural axons (Fig. 3B, arrowhead). The cells transfectedwith EYFP alone projected ascending EYFP⁺ axons ipsilaterally (Fig. 3C, arrow) but not commissural axons(Fig. 3E). In contrast, cells ectopically expressing MBH1 projectedascending commissural axons (Fig. 3F, arrowhead). Coexpressionof MBH1 and EYFP in the same cells was confirmed by immunostainingusing the anti-MBH1 antibody (data not shown). There were moreTAG-1⁺ axons observed in the MBH1-transfected side (Fig. 3G). EYFP⁺ axons were labeled with the anti-TAG-1 antibody (Fig. 3H). Similarly,more DCC⁺ axons were generated by ectopic expression of MBH1, and the EYFP⁺ axons were also DCC⁺ (data not shown). These results indicate that the axons of thecells ectopically expressing MBH1 had acquired molecular identitiesas commissural axons and that ipsilaterally projecting dorsalneurons were transfated into commissural neurons by misexpressionof MBH1.

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Figure 3. Generation of commissural neurons by ectopic expression of MBH1. E11.5 mouse spinal cords were transfected with EYFP alone (A, C, E, I) and both EYFP and MBH1 (B, D, F-H, J). Right sides of sections were closer to the anode and transfected with these genes (A, B, G, H). A, B, Transverse sections of the spinal cord at brachial levels, 2 d after electroporation. Arrows and arrowhead indicate EYFP⁺ cells with morphologies similar to migratory commissural neurons and commissural axons, respectively. Similar patterns of EYFP⁺ cells and axons were observed through all axial levels of the spinal cord in all electroporated EYFP⁺ embryos (n = 15 for EYFP alone; n = 25 for coexpression of EYFP and MBH1). Lateral (C, D, I, J) and ventral (E, F) views of the spinal cord electroporated at lumbar levels, 3 (C-F) and 4 (I, J) d after electroporation. Rostral is to the left. Arrow and arrowhead indicate EYFP⁺ ipsilaterally projecting and commissural axons, respectively. G, H, Transverse section of the E12.5 spinal cord, 1 d after transfection with EYFP and MBH1. The section was stained with antibodies against TAG-1 (red) and GFP (green). Misexpression of either LH2B, a LIM homeobox gene, or PHD1, a paired-like homeobox gene expressed in the dorsal spinal cord (Saito et al., 1996), did not generate more commissural axons. Scale bars: (in A) A, B, 100 µm; (in C) C, E, 200 µm; (in D) D, F, 200 µm; G, 100 µm; (in I) I, J, 200 µm.

Migration patterns of MBH1-misexpressing cells

Four days after electroporation, cells expressing EYFP alone remained in the dorsal spinal cord (Fig. 3I). In contrast, mostof MBH1-misexpressing cells were observed in the middle of thespinal cord (Fig. 3J), suggesting that MBH1-misexpressing cellsmay have migrated from the dorsal spinal cord. To compare MBH1-misexpressingcells with endogenous MBH1⁺ cells, in situ hybridization was performed (Fig. 4). At E12.5,1 d after electroporation, more cells expressing MBH1 were detectedin the dorsal area of the MBH1-transfected side (Fig. 4A). Expressionlevels of MBH1 were higher in the MBH1-misexpressing cells thanthose of endogenous MBH1, reflecting a strong activity of theCAG promoter. Those cells appeared to migrate toward the deepdorsal horn, whereas the endogenous MBH1⁺ cells had already settled in the deep dorsal horn at this stage(Fig. 4A, arrowhead). Two days after electroporation, many MBH1-misexpressingcells settled down in the deep dorsal horn, in which the endogenousMBH1⁺ cells accumulated (Fig. 4B). A minor population of the MBH1-misexpressingcells was detected in the ventral spinal cord as well as the endogenousMBH1⁺ cells. These results suggest that the cells ectopically expressingMBH1 migrate to endogenous MBH1⁺ domains.

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Figure 4. Comparison of MBH1-misexpressing cells with endogenous MBH1⁺ cells using in situ hybridization. After electroporation at E11.5, transverse sections of the mouse spinal cord were annealed with antisense cRNA probes of MBH1 (A, B), MATH1 (C), and LH2B (D). Right sides were transfected. Embryos were recovered at E12.5 (A, C, D) and at E13.5 (B). Arrowheads and arrows indicate endogenous MBH1⁺ domains and MBH1-misexpressing cells, respectively. Expression of MATH1 and LH2B was not upregulated at E13.5 either (data not shown). Transfection with EYFP alone did not affect the expression of the genes (data not shown). Scale bar (in A): A-D, 100 µm.

Next we examined whether the misexpression of MBH1 affects other genes. Expression of MATH1 and LH2B, which are related tothe differentiation of commissural neurons, was not upregulated(Fig. 4C,D; data not shown). Furthermore, no increase of LH2A/B⁺ cells was detected using the anti-LH2A/B antibody (data not shown).These findings suggest that MATH1 and LH2A/B are not downstreamof MBH1.

  Discussion

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Introduction
Materials and Methods
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Discussion
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Commissural neuron differentiation by MBH1

The results obtained by the ectopic expression of MBH1 suggest that MBH1 regulates at least three aspects of the differentiationof commissural neurons. Expression of TAG-1 and DCC, which aremarkers of commissural neurons, were induced by MBH1. BecauseDCC is a receptor of netrins, the ectopic expression of DCC maybe responsible for axon projection of the MBH1-misexpressing cellsto the floor plate. Their axons elongated along the floor plateafter crossing it, as do endogenous commissural neurons. The MBH1-misexpressingcells appeared to migrate to the endogenous MBH1⁺ domains. These findings suggest that several genes involved inthe differentiation of commissural neurons are regulated downstreamof MBH1.

There are several types of commissural neurons at various dorsoventral domains in the spinal cord. Only two domains were MBH1⁺, showing that MBH1 is expressed by a subset of commissural neurons.The expression of MBH1 at E10.5, which was restricted to the dorsaledge of the spinal cord, was similar to that of MATH1, but theexpression of MATH1 was limited to the ventricular zone and detectedat E9.5 (Helms and Johnson, 1998; data not shown), earlier thanthat of MBH1. All $beta$ -gal⁺ cells of the MBH1/lacZ transgenic embryos expressed LH2A/B, whichis a marker of dI1 cells and expressed downstream of MATH1. Theseresults indicate that MBH1 is expressed in a lineage of cellsthat have expressed MATH1. All LH2A/B⁺ cells, however, appeared not to be $beta$ -gal⁺, suggesting that MBH1 is expressed in a subset of LH2A/B⁺ cells. The expression patterns of MBH1 were similar to thoseof LH2B in the spinal cord (Fig. 4; data not shown), suggestingthat MBH1 may be expressed in the same lineage of cells that expressLH2B.

Misexpression of MBH1 generated more commissural neurons without induction of LH2A/B, suggesting that LH2A/B may not exertthe same function as MBH1 in the differentiation of commissuralneurons. This was confirmed by ectopic expression of LH2B in thespinal cord, which did not produce more commissural neurons (datanot shown). On the other hand, misexpression of MATH1 generatedmore commissural neurons (data not shown), suggesting that MATH1is upstream of MBH1. At E11.5, the domain of MBH1 expression closelyresembled the $beta$ -gal⁺ domain of transgenic mice that carried lacZ under the controlof MATH1-flanking sequences (Helms and Johnson, 1998). Moreover,the 3' MBH1-flanking sequence used for the transgenic mice inthis study contained an E-box (CAGCTG), which could bind the MATH1protein (Akazawa et al., 1995; Helms et al., 2000). These findingssuggest that MBH1 may be a downstream target of the MATH1protein.

A recent report has shown that excess commissural neurons were generated in Lbx1 (a Ladybird-like homeobox gene 1) mutantmice because of mis-specification of dorsal interneurons (Grosset al., 2002). This is similar to our results from the misexpressionof MBH1. However, expression of Isl1 and Lim1/2, which are affectedin the mutant mice, were not perturbed by the misexpression ofMBH1 (data not shown). This result suggests that MBH1 generatesectopic commissural neurons independently of a transcriptionalcascade exerted in the Lbx1 mutantmice.

Regulation of cell migration by MBH1

The transgenic mice carrying lacZ with the MBH1-flanking sequences visualized MBH1⁺ cells. At E10.5 and E11.5, the stages when the MBH1⁺ cells were located between the dorsal edge and the deep dorsalhorn in the spinal cord, they showed morphologies typical of somemigratory neurons (unipolar with leading processes) (Leber andSanes, 1995). Together with expression patterns of MBH1, thissuggests that MBH1 is expressed during the migration of commissuralneurons. The endogenous MBH1⁺ cells migrated to the deep dorsal horn along the marginal zoneof the spinal cord. In contrast, MBH1-misexpressing cells appearednot to follow the same route as the endogenous MBH1⁺ cells but rather to take a direct shortcut route from their birthplacesin the ventricular zone to the deep dorsal horn. These observationssuggest that MBH1 may instruct the cells where to migrate, respondingto an extracellular factor in the spinal cord. The factor maybe released from the deep dorsal horn to attract the cells ormay exclude the cells from the dorsolateral region of the spinalcord.

MBH1 was also expressed by granule cells during their migration in the developing cerebellum (Saito et al., 2000). MATH1,TAG-1, and DCC are all expressed in the developing cerebellumas well (Yamamoto et al., 1990; Akazawa et al., 1995; Liveseyand Hunt, 1997), suggesting that there is a common cascade ofgenes between commissural neurons and thecerebellum.

Various functions of BarH genes

Some commissural neurons are generated downstream of Ngn2 (Simmons et al., 2001). We showed that forced expression of MBH1upregulates Ngn2 in P19 cells, reflecting expression patternsof the two genes in the developing diencephalon (Saito et al.,1998). Ngn2 was not activated by ectopic expression of MBH1 inthe developing spinal cord (data not shown). MBH1 requires anotherunknown factor that is transiently expressed in P19 cells to upregulateNgn2 (Saito et al., 1998). The factor may have been absent inthe spinal cord at the stage when MBH1 was ectopically expressed.MBH1 was expressed in mitotically active cells in the ventricularzone of the diencephalon, whereas postmitotic cells expressedMBH1 in the spinal cord. MBH1 may have different functions atdifferent stages of neurogenesis. Similarly, Drosophila BarH genesshow various functions (Higashijima et al., 1992a,b).

In vivo electroporation in mouse

Both gain- and loss-of-function analyses are essential to establish gene function. Gene knock-out techniques have enabledthe loss-of-function analysis of many genes in mouse. On the otherhand, gain-of-function approaches have been used extensively inchick. The genes and gene combinations that regulate some stagesof development are not exactly the same between chick and mouse.This report demonstrates that the in vivo electroporation techniqueis a powerful tool to reveal gene function in the mouse. Thistechnique will greatly facilitate functional analyses of genes,because it may also be applied to knock-out and transgenicmice.

  FOOTNOTES

Received Sept. 25, 2002; revised Dec. 3, 2002; accepted Dec. 18, 2002.

This work was supported in part by a grant from the Japan Society for the Promotion of Science and Grants-in-Aids for ScientificResearch on Priority Areas-Neural Net Project and -Advanced BrainScience Project from Ministry of Education, Culture, Sports, Science,and Technology of Japan (T.S.). We thank Masuko Tanaka and JunkoKutsuna for their technical assistance and Dr. Takayuki Sakuraifor his kind advice for generating transgenic mice. We are gratefulto Drs. Thomas Jessell, Jane Johnson, Ryoichiro Kageyama, andQiufu Ma for antibodies and plasmids. We also acknowledge theDevelopmental Studies Hybridoma Bank maintained by the Universityof Iowa (Iowa City, IA) for supply of monoclonalantibodies.

Correspondence should be addressed to Tetsuichiro Saito, Department of Development and Differentiation, Institute for FrontierMedical Sciences, Kyoto University, Shogoin, Sakyo-ku, Kyoto 606-8507.E-mail: tesaito{at}frontier.kyoto-u.ac.jp.

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Materials and Methods
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Discussion
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