Lhx9: A Novel LIM-Homeodomain Gene Expressed in the Developing Forebrain

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The Journal of Neuroscience, January 15, 1999, 19(2):783-793

Lhx9: A Novel LIM-Homeodomain Gene Expressed in the Developing Forebrain
Sylvie Rétaux¹, Monique Rogard¹, Ingolf Bach², Vieri Failli¹, and Marie-Jo Besson²
¹ Laboratoire de Neurochimie-Anatomie, Institut des Neurosciences, 75005 Paris, France, and ² Howard Hughes Medical Institute, University of California, School of Medicine, La Jolla, California 92093

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

A novel LIM-homeodomain gene, Lhx9, was isolated by degenerate RT-PCR followed by mouse embryonic library screening. Lhx9cDNA encodes a protein that is most closely related to Drosophilaapterous and rodent Lhx2 proteins. The Lhx9 spatiotemporal patternof expression during embryogenesis was similar but distinct fromLhx2. Highest expression levels were found in the diencephalon,telencephalic vesicles, and dorsal mesencephalon. Domains of expressionrespected the proposed neuromeric boundaries (Puelles and Rubenstein,1993). Lhx9 was also expressed in the spinal cord, forelimb andhindlimb mesenchyme, and urogenital system. Although Lhx9 expressionwas sustained in diencephalon and mesencephalon from embryonicday 10.5 (E10.5) to postnatal stages, it was transient in thefuture cerebral cortex, where it was turned off between E14.5and E16.5. Lhx9 expression was highest if not exclusively located(depending on the region of interest) in the intermediate andmantle zones, as opposed to the mitotic ventricular zone. Lhx9protein was tested for interaction with the recently discoveredcofactors of LIM-homeodomain proteins and was found to interactstrongly both with CLIM1 and CLIM2. The expression pattern andstructural characteristics of Lhx9 suggest that it encodes a transcriptionfactor that might be involved in the control of cell differentiationof several neural cell types. Furthermore, Lhx9 protein couldact in a combinatorial manner with other LIM-homeodomain factorsexpressed in overlappingpattern.

Key words: LIM-homeodomain; Lhx9; Lhx2; forebrain; development; neuromeres

  INTRODUCTION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

A major issue in developmental neurobiology is the understanding of forebrain development and patterning. During embryogenesis,the anterior neural tube generates complex and highly organizedstructures, such as the cerebral cortex, the basal ganglia, andthe thalamus. In adults, these structures are interconnected,almost alwaystopographically.

Homeodomain genes play decisive roles in the establishment of cerebral structures and/or the generation of cell types. Amongthem, LIM-homeodomain (LIM-hd) genes encode developmentally expressedtranscription factors that contain a homeodomain and two cysteine-richLIM domains involved in protein-protein interactions (Sanchez-Garciaand Rabbitts, 1994; Dawid et al., 1995). In the current view,the LIM domains inhibit DNA binding by the homeodomain. Afterfixation of cofactors, transcription is activated, and synergismwith other transcription factors is promoted. Indeed, cofactorsfor LIM-hd proteins have been isolated: NLI/Ldb1/CLIM2 and CLIM1interact with LIM domains of LIM homeoproteins to potentiate transactivationof downstream genes (Agulnick et al., 1996; Jurata et al., 1996;Bach et al., 1997). These cofactors probably confer time and spacespecificity to the regulatory action of LIM-hdproteins.

LIM-hd genes were first implicated in cell fate determination in invertebrates; Caenorhabditis elegans mec-3 and lin-11 (Wayand Chalfie, 1988; Freyd et al., 1990) and Drosophila apterous(Lundgren et al., 1995; Thor and Thomas, 1997) determine celltypes and axonal pathfinding. In vertebrates, the spinal cordmotor neurons give an example for similar roles of LIM-hd genes:motor neurons express a set of four LIM-hd genes, in a combinatorialmanner that is correlated to the motor neuron position in thespinal cord and to the type of peripheral innervated target (Tsuchidaet al., 1994). Thus, a LIM-hd combinatorial code might definepathfinding phenotypes. If similar combinations of LIM-hd geneswere expressed in the forebrain, they could participate in theestablishment of its highly organized circuits. Moreover, Drosophilaislet governs aminergic phenotypes (Thor and Thomas, 1997). ForebrainLIM-hd genes could govern neurotransmitter expression in neuronsaswell.

Homeodomain genes expression patterns in the developing CNS have led to the theory of the prosomeric forebrain (Puelles andRubenstein, 1993; Rubenstein et al., 1994; Puelles, 1995). Inthis model, regions and boundaries of expression of developmentalfactors are seen as landmarks for the determination of cerebralareas according to longitudinal and transverse subdivisions thatform segmented structures. LIM-hd genes integrate this model well.Lhx1/lim-1 (Barnes et al., 1994), Lhx2/LH-2 (Xu et al., 1993),Lhx3/pLIM (Seidah et al., 1994; Bach et al., 1995), L3/Lhx8 (Matsumotoet al., 1996), Lhx4/Gsh4 (Li et al., 1994), Lhx5 (Sheng et al.,1997), Lhx6, and Lhx7 (Grigoriou et al., 1998) are all expressedin the developing rodent CNS, and their expression patterns respectneuromeric boundaries (present paper). The role of LIM-hd genesin cellular specification, combined with their apparent functionin the coding of positional information, makes them importantfactors to be studied during brain regionalization andwiring.

In a search to isolate more LIM-hd involved in forebrain development, we hypothesized the existence of a subfamily of Lhx2-relatedLIM-hd genes. An RT-PCR cloning strategy allowed the isolationof mouse Lhx9, which is similar to but distinct from Lhx2 in sequenceand expression pattern, the two genes thereby forming a new subfamilyof forebrain LIM-hdgenes.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

RT-PCR cloning. Total RNA from embryonic day 15 (E15) or E18 forebrain were reverse-transcribed to cDNA with avian myeloblastosisvirus reverse transcriptase (Boehringer Mannheim, Mannheim, Germany)and used as templates for PCR reactions (Qiagen, Hilden, Germany)using the following degenerate oligonucleotide primers: 51, ATGCGIACITCITTYAARCAYCAYCARCT;52, ATGAGRACITCITTYAARCAYCARCT; 31, MAYTTIGCIGCIGCRTTYTGRAACCA;and 32, MAYTTIGCYCTIGCRTTYTGRAACCA, where I is an inosine residue.5' (51 and 52) and 3' (31 and 32) primers were designed to isolategenes of the Lhx2 subfamily and were chosen to amplify a stretchof DNA in the homeodomain. Any combination of 3' and 5' primersled to the amplification of a single band of 160 bp as expected.After cloning of this 160 bp fragment into pGEM-T (Promega, Madison,WI), sequencing of 80 independent clones revealed the presenceof three different fragments. One was mouse Lhx2, and the twoothers were unknown. We concentrated on one that we named Lhx9.The 160 bp DNA fragment was used to screen a $lambda$ gt11 E14.5 mousehead cDNA library under high stringency. The Lhx9 cDNA was isolatedusing standard molecular biology techniques and sequenced on bothstrands with Amersham (Les Ulis, France) thermosequenase. The1.016 kb PCR product of Lhx9 cDNA was subcloned into pGEM-T (Promega)for subsequentexperiments.

Tissue preparation. Timed pregnant C57/Black6 mice were anesthetized with 0.1 ml/100 gm body weight pentobarbital. Embryoswere harvested, fixed in 0.1 M 4-morpholinepropanesulfonic acid,pH 7.4, 2 mM EGTA, 1 mM MgSO₄, and 3.7% formaldehyde at room temperature,cryoprotected in 30% sucrose, and frozen by immersion in isopentaneon dry ice. Noon on the day after the night of mating was consideredas E0.5. Postnatal day 1 (P1)-P7 brains were processed identically,except that sucrose was 20%. Whole embryos or dissected brainswere cryostat-sectioned at 20 µm, and sections were stored at $-$ 80°C untiluse.

In situ hybridization and image processing. The pGEM-Lhx9 plasmid was linearized with NdEI or NcoI and used as template forRNA synthesis with T7 or SP6 polymerase in the presence of [³⁵S]UTP (10 mCi/mmol; ICN Biochemicals, Costa Mesa, CA) for antisenseand sense control probes, respectively. The probe thus includedthe 5' noncoding region, the two LIM domains, the linker region,and the beginning of the homeodomain. The Bluescript-Lhx2 plasmidincluding the 1.1 kb Lhx2 insert was linearized with EcoRI, andT3 polymerase was used for antisense probe synthesis as described(Bach et al., 1997). The Bluescript-En2 3' untranslated regionplasmid was linearized with ClaI, and T7 was used to generatean 800 bp En-2 probe. Restriction enzymes were purchased fromAppligene (Heidelberg, Germany) or Promega, and RNA polymeraseswere from Stratagene (La Jolla, CA). Briefly, slides were acetylated,dehydrated progressively, and hybridized 16 hr at 60°C in thepresence of 5 × 10⁵-10⁶ cpm of probe/slide. They were then washed under high stringency,treated 1 hr with RNase A (20 µg/ml), and dehydrated. Sectionswere exposed 2-3 d to Eastman Kodak (Rochester, NY) Biomax MRfilm for autoradiography and then dipped in Kodak NTB-2 emulsion.Emulsions were developed after 10-12 d of exposure, and sectionswere counterstained with methylene blue. Photographs were takenon a Leica (Nussloch, Germany) DMBL microscope, scanned on a Canon(Tokyo, Japan) 2700 scanner, and mounted for figures with Adobe(Mountain View, CA) Photoshop. Images were corrected for colorbalance, contrast, brightness, or cropping, but no other correctionsweremade.

In vitro protein-protein interaction assays. PCR products of full-length CLIM1a and CLIM2 were ligated in frame into the XhoI-XbaIsites of the bacterial expression vector pGEX-KG to yield a glutathioneS-transferase (GST) fusion protein. The PCR product of the 1.016kb Lhx9 cDNA was subcloned into the pGEM-T vector (Promega), and[³⁵S]methionine-labeled Lhx9 protein was produced using the Promegain vitro transcription-translation kit, SP6 RNA polymerase, and[³⁵S]methionine. The in vitro protein-protein interaction assayswere performed as described previously (Bach et al., 1995).

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cloning of Lhx9, a novel LIM homeodomain gene

The RT-PCR strategy for cloning new LIM-hd genes expressed in the forebrain was based on the observation that the Lhx2 homeodomainwas slightly different from other LIM-hd genes expressed in moreposterior parts of the brain. An SFKHH amino acid sequence wasfound in the N terminus part of its homeodomain, instead of theoften encountered TITAK motif. We hypothesized the existence ofother genes of the same subfamily that could be specific for theforebrain. Degenerate PCR primers were thus designed to amplifya theoretical 160 bp DNA fragment spanning almost the entire homeodomain(with a 5' primer at the level of the SFKHH motif and a 3' primerat the level of the highly conserved VWFQN motif close to theC terminus of the homeodomain). Sequencing of the 160 bp RT-PCRfragment revealed a new sequence (19 nucleotides of 102 were differentfrom Lhx2 but were conservative at the amino acid level). ThisPCR fragment was used to screen an E14.5 mouse head $lambda$ gt11 cDNAlibrary and allowed the isolation of Lhx9. The ~1 kb cDNA contained5' noncoding sequences and, in the open reading frame, two LIMdomains and a homeodomain (Fig. 1A, shading). The C-terminal partand the stop codon were not included in this cDNA. Additionalscreens could not identify the 3' end missing sequences. However,the 300 amino acids encoded by the cDNA are largely sufficientto allow for Lhx9 classification and riboprobe synthesis. Thereare two in-frame methionine residues (Fig. 1A, boxed) located10 amino acids apart at the level of the translation initiationsite. Based on similarity with Lhx2, we postulate that the secondmethionine will be used for translation start. Lhx9 shares 69%identity with rat Lhx2 at the amino acid level and 68% at thenucleotide level. The amino acid identity rises to 95% in theLIM domains (Fig. 1B) and to 100% in the homeodomain. The maindifferences between the two proteins are located between the secondLIM domain and the homeodomain. The linker fragment between LIM2and the homeobox is shorter in Lhx9 [79 amino acids (aa) in Lhx9and 96 aa in Lhx2] and is more closely related in sequence andin length to chick Lhx2B [also 79 aa long (G. Tremml and T. M.Jessell, unpublished data; GenBank accession number L35566](Nohno et al., 1997). A basic sequence (RPRKRK; Fig. 1A, underlined)that might serve as a nuclear translocation signal is conservedin the middle of the linker region. The sequence similaritiesbetween Lhx9 and Lhx2 strongly support the notion that they aretwo closely related family members (Fig. 1B). Indeed, a comparisonwith other LIM-hd genes in GenBank showed that Lhx9 belongs toa growing subfamily including vertebrate Lhx2, Drosophila apterous,and C. elegans ttx-3 (Hobert et al., 1997). Moreover, the veryhigh (overall 94%) identity between mouse Lhx9 and chick Lhx2suggests that chick Lhx2 could rather be the avian homolog ofrodent Lhx9 (Fig. 1B).

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Figure 1. Sequence of murine Lhx9. A, Nucleotide and deduced amino acid sequence of Lhx9. Amino acids are indicated by single-letter code. The two in-frame ATG start codons are boxed. The sequence between the two possible start codons is in italics solely to indicate that based on homology with Lhx2, the second one is more likely to be used. LIM1, LIM2, and the hd are indicated by shading. The putative nuclearization signal is underlined. B, Comparison of murine Lhx9 with rat and chick Lhx2. The percentage of identity in each domain between gene products is indicated. GenBank/EMBL accession numbers: L06804 (rat Lhx2), L35566 (chick Lh2B), and AB005882 (chick Lh2A).

Expression of Lhx9 during embryogenesis of the nervous system

Whole-mount in situ hybridization showed that the onset of Lhx9 expression in the nervous system was at approximately E10.5(data not shown). Thus, from E11.5 onward, the expression patternwas studied by in situ hybridization on sections (Figs. 2, 3;Table 1). From E11.5 to E14.5, Lhx9 expression was relativelywidespread throughout the CNS alar neuroepithelium, with an increasebetween E11.5 and E12.5 (Fig. 2, compare A,B with C,D). Expressionremained high in the following stages.

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Figure 2. Lhx9 expression on brain sections from E11.5 (A, B), E12.5 (C-E, J), E13.5 (H, I), and P7 (K) embryos and comparison with En-2 (F, G) on dark-field illumination photomicrographs. In this and subsequent figures, pictures are oriented so that anterior is right and dorsal is at the top. A, C, Parasagittal sections through the entire brain at indicated stages. B, D, Horizontal sections (level and orientation indicated by white bars in A, C, respectively). G, En-2 expression on a section adjacent to that shown in D. E, F, Adjacent coronal hemisections showing the comparison of Lhx9 (E) and En-2 (F) expression in the anterior hindbrain. H, I, Bright-field (I) and dark-field (H) views of the same area showing the correlation between the position of the tpc and the tract of the postoptic commissure (tpoc) and Lhx9 sharp boundaries of expression (arrowheads). J, Coronal section through the spinal cord. K, Coronal section at the level of the hippocampus and thalamus at P7, showing expression in CA3, CA4, and the dentate gyrus (dg) and the delineation of various thalamic nuclei by Lhx9 hybridization signal. cl, Central lateral; hr, habenula; lp, lateral posterior; md, mediodorsal; va, ventral anterior; re, reuniens; rh, rhomboid. See Table 1 for anatomical abbreviations. Scale bars: A-I, K, 100 µm; J, 50 µm.


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Table 1. List of anatomical abbreviations

In the telencephalic vesicles Lhx9 mRNA was expressed in the future cerebral cortex, the hippocampus, the claustrum primordium(where it could correspond to a stream of migratory cells fromthe striatum to the cortex; see De Carlos et al., 1996), and thecaudal ganglionic eminence (amygdaloid complex) (Figs. 2A-C, 3A-C).It was also expressed in the olfactory bulb primordium (Figs.2C, 3A). Interestingly, levels of expression in the telencephalicwalls depended on the region examined: it was relatively weakin the parietal neocortex, high in the frontal neocortex (datanot shown), and strongest in the archicortex (hippocampal field;Fig. 3B,C).

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Figure 3. Lhx9 expression at E13.5. A, Sagittal section through the entire brain. B-F, coronal sections through the telencephalon and diencephalon (plan of section indicated by white bars in A) showing Lhx9 transverse boundaries in the rostrocaudal extension. The dotted line indicates the zli. Scale bars, 100 µm. See Table 1 for anatomical abbreviations.

The diencephalon showed the highest expression levels (Figs. 2C,D, 3). Moreover, in this region, expression was observed inlongitudinal and transverse bands, with sharp boundaries thatrespect the neuromeric regionalization proposed by Puelles andRubenstein (1993) (Fig. 3). Indeed, from caudal to rostral (Fig.3A), Lhx9 was expressed in the pretectum (p1 prosomere) and inthe dorsal thalamus (except for a thin ventral band close to thealar-basal boundary), the epithalamus, and the epiphysis in prosomerep2. Expression stopped abruptly at the zona limitans intrathalamica,showing no expression in the ventral thalamus (p3 prosomere; Fig.3C-F). The supraoptic-paraventricular area and the eminentia thalamiagain formed a band of strong expression in the p4 prosomere thatabuts on a negative region around the optic stalk (prosomeresp5 and p6; Fig. 3A,D,E). A narrow band including the retrochiasmaticarea and the tuberal hypothalamus expressed Lhx9 and representedthe only domains of expression in the basal plate (Fig. 3A,F;also see Fig. 8A). Interestingly, the boundaries of expressionof Lhx9 at the diencephalic-mesencephalic junction delineatedperfectly the borders of the trajectory used by pioneering tractsof the posterior and postoptic commissure (Fig. 2H,I).

Posteriorly, Lhx9 was expressed throughout the tectum in the mesencephalon (Figs. 2A-D, 3A), in the walls of the hindbrain(Fig. 2A,E), and in nuclei in the ventral midbrain and hindbrain(Fig. 4I). The comparison with En-2, a major homeobox gene definingthe mesencephalic-metencephalic region, showed that the expressionof the two genes was quite different, neither totally overlappingnor strictly complementary (Fig. 2, compare D with G, E with F).

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Figure 4. Comparison of Lhx2 (A-E, J), Lhx9 (F-I, L), and En-2 (K) expression on sections. A, F, Parasagittal adjacent sections through the entire brain at E14.5, comparing expression of Lhx2 (A) and Lhx9 (F). B, C, Coronal sections at E13.5 showing Lhx2 expression in the telencephalon and diencephalon. Sections are adjacent to those shown in Figure 3, B and E, respectively, for comparison of transverse boundaries. D, G, Horizontal adjacent sections showing Lhx2 (D) and Lhx9 (G) expression in the eye and optic stalk at E14.5. The asterisk in G points to the nonspecific signal attributable to the presence of the eye pigmented epithelium. E, H, Adjacent parasagittal section showing Lhx2 (E) and Lhx9 (H) in the dorsal diencephalon and pretectum at E13.5. Note the absence of Lhx2 in the pineal gland. I-K, Adjacent parasagittal sections at E13.5 to compare Lhx9 (I), Lhx2 (J), and En-2 (K) expression through the mesencephalon and metencephalon. Arrows in I and J show the thinning of expression at the isthmus. L, Sagittal section through the midbrain of a P1 animal to show the Lhx9 sharp boundary between the superior and the inferior colliculi. Compare with I (earlier stage). Scale bars, 100 µm. ne, Nasal epithelium. See Table 1 for abbreviations.

In the spinal cord, Lhx9 was expressed as a gradient in the dorsal part of the neuroepithelium (Fig. 2J, corresponding tothe region where commissural and association neurons differentiate)but not in motorneurons.

Between E14.5 and E16.5, a major change in Lhx9 expression occurred in the neocortical neuroepithelium, because it was turnedoff (Fig. 5; see below). However, expression persisted in thearchicortex (in the dentate gyrus, CA3 and CA4) later on, as wellas in the diencephalon, midbrain, and hindbrain. Indeed, at earlypostnatal stages, (P1-P7), expression was particularly abundantin the dorsal thalamus where it allowed the delineation of variousnuclei (Fig. 2K). Lhx9 marked a sharp boundary between the very-high-expressinginferior colliculus and the high-expressing superior colliculus(Fig. 4L). A number of mesencephalic and pons nuclei, includingdeep cerebellar nuclei, still expressed Lhx9 at these postnatalstages (data not shown).

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Figure 5. Comparison of Lhx9 (left) and Lhx2 (right) expression in the neocortical epithelium at indicated stages. The pial surface (p) is at the top, and the ventricular surface (v) is at the bottom. Left and right photographs were taken on adjacent sections. cp, Cortical plate; iz, intermediate zone; mz, marginal zone; pp, preplate; sp, subplate; svz, subventricular zone; vz, ventricular zone. Scale bars, 100 µm.

In summary, Lhx9 expression was relatively widespread, mostly in the alar region of the neuroepithelium. In this respect,it is noteworthy that expression was absent from the large regionof the ganglionic eminences in the ventral telencephalon (correspondingto the striatal-pallidalprimordium).

Lhx9 and Lhx2 are expressed in overlapping but distinct patterns

Because Lhx9 and Lhx2 are closely related family members, we next compared directly the expression of the twogenes.

Concerning regional expression, the two genes were expressed mainly in overlapping patterns, with few noticeable exceptions:Lhx2 was expressed in the ganglionic eminences, the eyes, theoptic stalk, and the neuromeres surrounding the optic stalk, whereasLhx9 was not (compare Figs. 4A,F, 3B, 4B). In the prosencephalicregion, the two mRNAs were expressed in complementary patterns,showing bands of expression with sharp boundaries, separated byexpression-negative zones. More precisely, Lhx2 was not expressedin the eminentia thalami-supraoptic paraventricular areas, whereasLhx9 was, but the Lhx9-negative zone at the optic stalk, preopticarea, and anterior hypothalamus was Lhx2 positive (compare Figs.4A,F, 4D-G, 3E, 4C). Expression of the two genes was perfectlyoverlapping in the dorsal thalamus and was absent for both genesin the ventral thalamus (Fig. 4, compare A-F). Thus, the additionof the two expression domains covered almost the entire diencephalicarea with the exception of the ventral thalamus (for summary,see Fig. 8A).

In the tectal epithelium, the expression patterns of the Lhx genes were overlapping in the marginal layers (Fig. 4I-J). Incontrast to engrailed, Lhx9 and Lhx2 were not expressed as a gradient.Their expression domains spanned the mesencephalic-metencephalicjunction, slightly thinning out at the isthmus (Fig. 4I-J, arrows).Furthermore, when compared with En-2, they were not as largelyexpressed in the ventral mesencephalon (Fig. 4, compare I-K).

Interesting differences between the two family members were observed at the cellular level. In the telencephalic vesicles,Lhx9 mRNA was exclusively located in the differentiating layersof the neuroepithelium, as opposed to the mitotic ventricularzone, whereas Lhx2 was expressed throughout the depth of the neocorticalepithelium, including the ventricular and the differentiatingmantle zones (Fig. 5). Concerning the timing of Lhx9 and Lhx2expression, a major difference was again found in the neocortex.Whereas Lhx9 expression stopped between E14.5 and E16.5, Lhx2was still expressed in the neocortex until P1 (Fig. 5) and later(data not shown). Moreover, although Lhx9 stopped in hippocampalfields CA1 and CA2 around birth (Fig. 3K), Lhx2 was still expressedin the whole hippocampus (data notshown).

Thus, Lhx9 and Lhx2 are expressed in patterns that are compatible both for redundant and complementary roles during brainregionalization andneurogenesis.

Lhx9 expression outside the CNS

Lhx9 was also expressed in a few developing regions outside the CNS. This included the developing forelimb and hindlimb buds,where a gradient of expression was observed at early stages inthe distal mesenchyme (Fig. 6B,C). Later on, expression was progressivelyrestricted to the interdigit spaces corresponding to the regionwhere programmed cell death happens for finger formation and tothe region surrounding the cartilages (Fig. 6D,E). Moreover, Lhx9mRNA was also highly expressed in the caelomic cavity at the levelof the urogenital ridge, including the gonads and parts of thepancreas and liver epithelium (Fig. 6A). As opposed to Lhx2, Lhx9was expressed neither in the nasal epithelium nor in the pituitary(Fig. 4A).

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Figure 6. Lhx9 expression in limbs and urogenital ridge. A, Coronal section through the caelomic cavity and the spinal cord (double arrow) at E11.5. Arrowheads point to the developing gonads (g), pancreas (p), and liver (l). Because sex discrimination is not easy at this stage, it should be noted that the same expression pattern was found in all embryos examined. B, Expression in E10 forelimb after in toto in situ hybridization. p, Proximal; d, distal. C-E, Transverse sections through developing hindlimbs and forelimbs at indicated stages. Arrowheads in C indicate absence of expression in the apical ectodermal ridge. See Results for details. Scale bars: A, C-E, 50 µm; B, 200 µm.

Lhx9 protein interacts with CLIM1 and CLIM2 cofactors

Because the Lhx9 expression pattern is partially overlapping with the expression of the recently isolated cofactors of LIM-hdproteins, we tested whether Lhx9 protein could physically interactwith CLIM1 and CLIM2. GST pull-down assays were performed using[³⁵S]Lhx9 and CLIM1 and CLIM2 GST fusion proteins. The results showthat Lhx9 strongly interacts with both cofactors in vitro (Fig.7), suggesting possible functional interactions in vivo.

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Figure 7. Lhx9 interacts with CLIM1 and CLIM2. Autoradiogram of a representative GST pull-down assay in which ³⁵S-labeled, in vitro-translated Lhx9 was tested for its ability to bind bacterially expressed GST fusions of CLIM1 and CLIM2. Ten percent (10%i) of the total ³⁵S-labeled protein input and binding to beads alone are shown.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Lhx9 and Lhx2 form a subfamily of LIM-hd genes

We have isolated a new LIM-hd gene named Lhx9, thereby increasing the number of LIM-hd genes expressed in the developing CNS.Lhx9 is most closely related to rodent Lhx2 (Xu et al., 1993)and chick Lh2B-Lh2A (Nohno et al., 1997), Drosophila apterous(Lundgren et al., 1995), and C. elegans ttx-3 (Hobert et al.,1997). In particular, these proteins share a short but notabledifference in their homeodomain when compared with other LIM-hdfactors. Surprisingly, although the homology between mouse Lhx9and chick Lh2B is very high (94%), the Lhx9 expression patternis more related to chick Lh2A, at least in limbs, in which chickLh2A expression was thoroughly described (Nohno et al., 1997).The high degree of conservation between Lhx9 and Lhx2 suggeststhat they belong to the same subfamily. Interestingly, in vertebrates,LIM-hd genes are often encountered in pairs of closely relatedhomologs, such as Lhx1/Lhx5, Lhx3/Lhx4, Lhx6/Lhx7/Lhx8, and nowLhx2/Lhx9. Generally, the two genes of the pair show similar expressionpatterns (Fig. 8B). This redundancy among the gene family suggestscritical and complementary (or synergistic) roles played by thesetranscription factors during brain formation.

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Figure 8. Summary of Lhx9 and Lhx2 expression patterns in the context of the neuromeric model (A) and schematic representation of Lhx combinatorial expression in the developing brain (B). Adapted from Puelles and Rubenstein (1993). A, Schematic E13.5 brain shows similarities, differences, and boundaries of expression of Lhx9 (yellow) and Lhx2 (dotted). Expression in the ventral mesencephalon and metencephalon is not indicated because of its rather "nuclear-like" pattern. B, Compilation of expression data for Lhx1/5 (red; Sheng et al., 1997), Lhx2/9 (blue; this paper), Lhx3/4 (pink; Li et al., 1994; Bach et al., 1995), and Lhx6/7/8 (green; Matsumoto et al., 1996; Grigoriou et al., 1998) on a "flattened brain" adapted from Bulfone et al. (1993). Gene expression is indicated by color-coded numbers, and a possible Lhx combinatorial code clearly emerges. The anteroposterior extension of expression is recapitulated by arrows at the bottom. Basal plate expression is not indicated. The zli is indicated by a dotted line. p1-p6, Prosomeres 1-6. See Table 1 for anatomical abbreviations.

In this respect, it is interesting to rediscuss the phenotype of Lhx2^/ embryos with the knowledge of the existence of Lhx9. Lhx2^/ embryos are anophtalmic, with an aplasic archicortex and hypoplasicneocortex and basal ganglia, but their diencephalon and mesencephalonlook normal (Porter et al., 1997). Porter et al. (1997) hypothesizedthat, depending on the region examined, the more or less defectivephenotype could result from functional compensation by an unknownrelative gene. Lhx9 is not expressed in eyes and basal gangliabut is present in the neocortex, archicortex, diencephalon, andmesencephalon. Thus, functional compensation by Lhx9 might actuallyhappen for the neocortex, diencephalon, and mesencephalon cases.It should be noted that the expression patterns of Lhx1 and Lhx5are also compatible for a partial functional redundancy at theselevels, including basal ganglia (Sheng et al., 1997). In contrast,the eyeless phenotype of Lhx2^/ embryos suggests that Lhx2 is a major factor of this family inthe eye. Finally, in the case of the hippocampus, it appears thatalthough Lhx9 is relatively strongly expressed in this area, itis not able to compensate for the lack of Lhx2 expression. Thiscould mean that Lhx9 functions in the archicortex and neocortexare different. However, more detailed data on Lhx1 and Lhx5 expressionwould help in understanding the possible Lhx combinations forregional specification. Overall, the very high expression levelsof Lhx9 in the diencephalon and mesencephalon, combined with thelack of phenotype in these areas in Lhx2^/ embryos, suggests that Lhx9 plays an important role in the specificationof the thalamus andtectum.

Lhx9 respects neuromeric boundaries

Transverse and longitudinal subdivisions of the developing brain, corresponding to domains and boundaries of expression ofa number of developmental factors, and coincident with morphologicalstructures such as ventricular ridges and external furrows, haveallowed the proposal of a neuromeric organization of the forebrain,as described in the model of Puelles and Rubenstein (e.g., Bulfoneet al., 1993, 1995; Porteus et al., 1994). The detailed studyof Lhx9 and Lhx2 expression patterns shows that they respect theproposed neuromeric boundaries. This is summarized in Figure 8A,and we would like to discuss the following points. (1) The expressionpatterns clearly corroborate the proposed demarcations for p4prosomere and distinguish nicely both p3-p4 and p4-p5 boundaries,which is important because most gene markers do not distinguishthe p3-p4 limit well. (2) In a more recent variation of theirearly model, Bulfone et al. (1995) suggest that the entire cerebralcortex (ncx and acx) could be either in p5 (implying that thelge-cortex boundary is longitudinal, and that the cge is the telencephalicportion of p4) or in p4, implying that the lge-cortex boundaryis transverse (i.e., neuromeric). The expression patterns observedhere are consistent with both views. From the Lhx9 pattern, thecge clearly belongs to p4. In the telencephalon, however, theLhx9 spatiotemporal pattern respects the putative transverse boundarybetween the archicortex (with strong and persistent expression)and the neocortex (with lower and transient expression), a patternthat is compatible with the early model with acx in p4 and ncxin p5. On the other end, as in many other genes, Lhx9 also distinguishesthe cortex-lge boundary, a feature that is more in favor of therecent model in which this boundary is viewed as neuromeric. (3)In the diencephalon, Lhx2 and Lhx9 also give a sharp delineationof the ventral thalamus (in p3) that is free of signal betweenthe adjacent prosomeres p4 and p2 (including the dorsal thalamuswith massive expression and the epithalamus), thereby respectingthe zona limitans intrathalamica. The other diencephalic subdivisionsare well respected, with longitudinal and transverse divisionsaround the optic stalk region. At this level it is interestingto note that the Lhx9-negative optic stalk zone is complementarywith Lhx2-positive areas. Also, Lhx9 and Lhx2 patterns respecta narrow negative band in the ventral part of the dorsal thalamus,close to the alar-basal boundary, that is similar to the Gbx-2expression pattern at this level (Bulfone et al., 1993). Interestingly,in the tectum, a sharp boundary appeared between the inferiorand superior colliculi around birth and could be relevant to theestablishment of optic versus auditory systems. Taken together,these results show that the Lhx9 pattern integrates well in theneuromeric model and could participate in the establishment ofthe identity ofneuromeres.

The observation that Lhx9 (and Lhx2) expression borders the pathway of pioneering tracts at the dimesencephalic junction isalso interesting. Indeed, it has been hypothesized that domainsand boundaries of expression of a position-encoding homeodomaingene give landmarks for the establishment of the main axonal tractsin the brain (Figdor and Stern, 1993; Wilson et al., 1993; Macdonaldet al., 1994; Rétaux et al., 1996). The two LIM-hd genes studiedhere might participate as local cues for the guidance of commissuralaxons at the dimesencephalicjunction.

Lhx9 is transiently expressed in the marginal layers of the neocortical epithelium

Before E11, the cerebral walls are constituted of a pseudostratified ventricular epithelium in which progenitor proliferationoccurs (for review, see Caviness et al., 1995). The onset of mousecortical neurogenesis has been reported between E10 and E11 (Angevineand Sidman, 1961; Caviness, 1982), a time that corresponds almostexactly to the onset of Lhx9 expression. Moreover, as opposedto Lhx2 and Lhx1 (Sheng et al., 1997), whose expression spansthe depth of the cortical neuroepithelium, Lhx9 expression isrestricted to the outer layers. From its expression pattern inthe cortical preplate where the first postmitotic cells are located,and from its absence in the mitotic ventricular zone, Lhx9 isa good candidate as a factor implicated in differentiation andphenotype acquisition. Moreover, neocortical Lhx9 expression isswitched off between E14.5 and E16.5. The exact time of Lhx9 decreasein expression will have to be determined precisely, and the correlationwith events related to neurogenesis will have to be studied. However,from birth-dating studies, this stage in mice (~E16.5) correspondsapproximately to the completion of generation of layer VI-V neurons,to the beginning of layer IV generation, and to the arrival ofthalamic afferents (Caviness, 1982; Polleux et al., 1997). Thus,Lhx9 is expressed during the time deep layer (VI-V) cortical neuronsaregenerated.

Although Lhx2 was first hypothesized to play a role in cortical neuron differentiation (Xu et al., 1993), it is probably alsoinvolved in precursor proliferation (Porter et al., 1997). Asdiscussed above, Lhx9 is rather involved in differentiation. Otherhomeobox genes from the Emx and Otx families are expressed ininteresting patterns in the cortical neuroepithelium: Emx2 islocated exclusively in proliferating cells, whereas Emx1 is foundin both proliferating and differentiated neurons (Gulisano etal., 1996). Otx1 is specifically expressed in dividing and differentiatedlayer V-VI neurons (Frantz et al., 1994). Genes from other families,such as T-Brain1, are expressed exclusively in postmitotic corticalcells (Bulfone et al., 1995). Thus, it seems possible that combinationsof all these transcription factors interact to regulate corticalneurogenesis and layer formation (also see nextsection).

Lhx9 protein interacts with CLIM cofactors

In the pituitary, interaction between CLIM cofactors and LIM domains of the LIM-hd protein P-lim promotes synergistic interactionsbetween P-lim and the homeobox-only protein P-otx on the glycoproteinhormone $alpha$ subunit promoter (Bach et al., 1997). The CLIMs couldphysically and functionally interact as well with a number ofLIM-hd proteins to confer time and space specificity to the transcriptionalcontrol they exert. CLIM1 and CLIM2 are widely expressed in thedeveloping brain (Bach et al., 1997), including regions whereLhx9 is expressed. Moreover, we show that Lhx9 strongly interactswith both of them. In the cortical neuroepithelium, for example,CLIM1 is selectively expressed in the cortical plate, as wellas Lhx9 until approximately E16.5. Otx1 is expressed in dividingand differentiating layer V-VI neurons (see above; Frantz et al.,1994). Making a parallel with the interactions described in thepituitary between P-lim, P-otx, and CLIMs, it is interesting tohypothesize that a trio of the same protein families, i.e., Lhx9,Otx1, and CLIM1, are candidates for functional interaction involvedin the generation of deep layer corticalneurons.

LIM-hd genes acting in a combinatorial manner?

In the spinal cord, the combinatorial expression of the four LIM-hd genes, Islet-1, Islet-2, Lim-1, and Lim-3, distinguishessubclasses of motor neurons that select distinct axonal pathwaysand that occupy different columns in the spinal cord (Tsuchidaet al., 1994). Although the complexity of the formation of structuresand connections is probably degrees higher in the brain than inthe spinal cord, the growing list of LIM-hd genes expressed inthe forebrain suggests a possible similar role in the forebrain.In Figure 8B we present a tentative summary of the expressiondomains of Lhx1-9. A combinatorial pattern clearly emerges inthe developing brain, with pairs of closely related homologs sharingcomparable domains of expression and taking part in the determinationof distinct parts of the brain (always respecting the prosomericlimits and particularly the zona limitans). For example, the richestcombination is found in the mge, with a unique expression of Lhx6-7-8that is restricted to p5. Of interest, Lhx1, Lhx2, Lhx5, and Lhx9are all expressed in the diencephalon and in the cortex (Shenget al., 1997; present work). If they act in a combinatorial mode,they could participate in the establishment of the highly topographicthalamocortical and/or corticothalamic projections (for review,see Molnar and Blakemore, 1995). Lhx9, highly expressed in medianline and associative thalamic nuclei, could participate in theconnections with the Lhx9-expressing frontal cortex. Noteworthyis the expression of Lhx9 in a number of limbic-related structuressuch as the archicortex, the olfactory bulb, the amygdala, thediagonal band, and the septum, pointing out a possible implicationof Lhx9 in the development of the limbicsystem.

In summary, in the family of LIM-hd genes that are often expressed in pairs in the developing CNS, Lhx9 is one of the missingpartners for Lhx2. Its expression pattern strongly suggests arole in forebrain development, both in the specification of brainsubdivisions and in cellulardetermination.

  FOOTNOTES

Received May 11, 1998; revised Oct. 13, 1998; accepted Nov. 4, 1998.

This work was supported by the Association Franco-Israelienne pour la Recherche Scientifique et Technique, Fondation pourla Recherche Médicale, and Centre National de la Recherche Scientifique.We are grateful to Dr. A. Joyner for the En-2 in situ probe andJ. L. Duband and Y. Bassaglia for discussions about Lhx9 in thecaelomiccavity.
Correspondence should be addressed to Dr. Sylvie Rétaux, Laboratoire de Neurochimie-Anatomie, Institut des Neurosciences,9 quai St. Bernard, 75005 Paris,France.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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