Contribution à l'étude des bases moléculaires des maladies de la croissance et du mécanisme de régulation du gène GH chez l'homme

Pérez, Christelle

12 January 2012

Chez la souris, Six6 et Lhx2 sont exprimés dans l'œil et la glande pituitaire en développement. Par une approche "gènes candidats", les ADN de patients avec un phénotype proche de celui de souris invalidées pour ces gènes ont été séquencés. Aucune mutation a été mise en évidence pour SIX6. Deux variations hétérozygotes faux-sens de LHX2 ont été identifiées mais n'ont pas d'effet (tests in vitro). LHX2 a un rôle régulateur transcriptionnel in vitro sur deux gènes pituitaires (PRL, POU1F1), et en action synergique avec POU1F1. Deux mutations hétérozygotes composites de LHX3 chez un patient non consanguin ont permis d'assigner à ce gène un syndrome décrit uniquement chez des patients consanguins. Une de ces mutations a un effet dominant négatif. POU1F1, impliqué dans la différenciation pituitaire terminale, est associé en pathologie humaine à un déficit en hormone de croissance (GH), PRL et TSHβ. L'expression de GH est régulée par la fixation de POU1F1 sur son promoteur et sur un " Locus Control Region " mais ses cofacteurs ne sont pas connus. Deux mutations faux-sens identifiées dans le domaine de transactivation (TAD) de POU1F1 sont associées à un déficit isolé en GH. La résonnance plasmonique de surface a permis de définir les interactions de POU1F1 (normal et mutés) sur ses séquences cibles ; des extraits nucléaires sont passés avec POU1F1 (normal et mutés) afin d'identifier (par spectrométrie de masse) ses partenaires au locus GH. Une cristallographie du TAD a débuté pour analyser sa structure tridimensionnelle qui est probablement altéré par les mutations identifiées

[SDV:GEN] Life Sciences/Genetics

Croissance

SIX6

LHX2

LHX3

POU1F1

LCR GH

The role of Lhx2 in the hematopoietic stem cell function, liver development and disease

Wandzioch, Ewa

January 2004

During embryonic development, generation of functional organs is dependent on proper interactions between different cell types. Elucidation of the mechanisms operating during organ formation might provide insights into the origin of many pathological disorders in the adult. Gene inactivation studies in mice have provided invaluable tool to study the function of genes critical for morphogenesis of distinct organs. A LIM-homeodomain transcription factor Lhx2 has previously been reported to play a role in fetal liver development and hematopoiesis, as its inactivation leads to lethal anemia due to underdeveloped liver. This thesis focuses on the function of Lhx2 in the development of these two organ systems. Reciprocal signaling between ventral foregut endoderm and mesenchyme of the septum transversum regulates the liver formation, expansion and differentiation. A fully formed liver is composed of endoderm-derived hepatocytes and cholangiocytes and a variety of mesenchyme-derived cell types, such as endothelial cells and hepatic stellate cells. In early stages of liver development Lhx2 is expressed in the liver-associated septum transversum mesenchyme, a part of which becomes integrated into the liver organ and develops into hepatic stellate cells. Functional Lhx2 expression in the hepatic mesenchyme is necessary for normal liver outgrowth and differentiation. Loss of Lhx2 from developing hepatic stellate cells leads to their activation and excessive deposition of collagen fibres, resulting in hepatic fibrosis and severely distorted liver architecture. Transfection of Lhx2 to human stellate cell line downregulates genes associated with stellate cell activation and fibrogenesis. Thus, Lhx2 is the first gene identified to negatively regulate events leading to hepatic fibrosis. Elucidation of the molecular mechanisms involved in this process might therefore be instrumental for the development of novel therapies useful in treatment of this disorder. Fetal liver is also a major site of hematopoiesis in the embryo and provides physiological conditions necessary for the efficient expansion of hematopoietic stem cells (HSCs). The hematopoietic defect observed in Lhx2-deficient embryos is cell-nonautonomous, indicating that Lhx2 might control secreted factors involved in the self-renewal of HSCs. This putative second role of Lhx2 has been investigated by analyzing the mechanism whereby Lhx2 expression generates in vitro self-renewing HSC-like cell lines. Interestingly, in agreement with the cell nonautonomous phenotype of the lethal anemia in Lhx2-/- embryos, the mechanism of self-renewal is dependent on Lhx2 expression and occurs via secreted factor(s). Identification of these factor(s) might potentially allow ex vivo expansion of HSCs for therapeutic purposes. The Lhx2-immortalized HSC-like cell lines share many basic features with HSCs and self-renew in vitro in presence of Steel factor (SF). SF/c-Kit signaling mediates a wide variety of biological activities in cells at many different levels in the hematopoietic hierarchy. We used the HSC-like cell lines as an in vitro model system to compare signal transduction pathways from c-Kit receptor in stem cells versus differentiated hematopoietic cells. HSCs require PI-3K dependent activation of Raf1-Mek-Erk cascade for their survival and self-renewal in response to SF, whereas activation of Erk is PI-3K independent in committed myeloid and mast cells. Thus, the mode of SF/c-Kit signaling is dependent on the differentiation status of the cells.

Cell and molecular biology

liver fibrosis

liver development

Lhx2

hematopoietic stem cells

Cell- och molekylärbiologi

Cell and molecular biology

Cell- och molekylärbiologi

Régulation de l’expression du gène Six6 par les facteurs de transcription Lhx2 et Pax6 dans le contexte des cellules souches rétiniennes

Champagne, Marie-Pier

08 1900

La rétinogésèse des vertébrés est la culmination de processus biologiques complexes parfaitement exécutés. Cette délicate orchestration est principalement contrôlée par les facteurs de transcription qui permettent aux progéniteurs rétiniens de proliférer, de s’auto-renouveler et de se différencier de façon appropriée. Les facteurs de transcription à homéodomaine sont les protéines qui sont responsables de la démarcation du site du primordium optique et participeront même à la différenciation tardive des différents types cellulaires de la rétine. Le contrôle génétique concernant l‘activation de l’expression de facteurs de transcription est peu connu. Nous avons étudié les séquences génomique avoisinant le gène Six6 afin d’identifier et mieux comprendre son promoteur. Des expériences d’immunoprécipitation de chromatine et des essais luciférases ont confirmé la liaison et la transactivation synergique du promoteur potentiel de Six6 par Lhx2 et Pax6 in vitro. Cette présente étude confirme et précise également le rôle de Lhx2 au niveau du développement précoce de l’oeil. La compréhension détaillée des réseaux génétiques régulant les progéniteurs rétiniens à former une rétine fonctionnelle est essentielle. En effet, lorsque ces connaissances seront acquises, nous serons en mesure d’appliquer les thérapies cellulaires pour rétablir les fonctions rétiniennes lors de pathologies dégénératives. / Vertebrate eye developement is the result of multiple perfectly executed biological process. This tight orchestration is principaly controled by transcription factors. Homeobox-containing transcription factors are expressed in the presumptive eye field and are required to initiate eye development and for final retinal cell differenciation. The genetic control of these transcription factors are poorly understood. We analysed Six6’s nearby genomic sequence to caracterise potential promoter regions. Chromatin immunoprecipitations and luciferase assays confirmed the binding and the in vitro synergic trans-activation of Six6 potential promoter by Lhx2 and Pax6. This study also demonstrate the contribution of Lhx2 for the establishment of presumptive retina field at the neural plate stage. The detailed knowledge of genetic networks regulating the formation of a fonctional retina by retinal progenitor is crucial. Indeed, when these mecanisms will be eluciated, we will be able to establish regenerative retinal cell therapy.

Rétine

Développement

Lhx2

Pax6

Six6

Progéniteur rétinien

Vésicule optique

Facteur de transcription

Homéodomaine

Retina

Homeobox

Development

Transcription factor

Optic vesicle

Molecular and cellular analysis of Lhx2 function in hematopoietic stem cells

Richter, Karin

January 2007

The formation of blood, hematopoiesis, is a dynamic process originating from a small number of hematopoietic stem cells (HSCs). To sustain hematopoiesis throughout life HSCs have the unique capacity to differentiate into all mature hematopoietic lineages as well as generating more HSCs by a mechanism referred to as self-renewal. However, the regulation of these processes is largely unknown. During embryonic development HSCs expand in the fetal liver, indicating that this environment supports HSC self-renewal. The LIM-homeobox gene Lhx2 is expressed in the fetal liver during this period and Lhx2 null mutant mice die in utero due to severe anemia caused by an environmental defect in the fetal liver. Embryonic stem cells differentiate in vitro, forming embryoid bodies (EBs) containing various tissues including hematopoietic progenitor cells. Introduction of Lhx2 into this system by retroviral transfer led to the generation of cytokine dependent HSC-like cell lines that were multipotent and expressed surface markers similar to embryonic HSCs. However, the specificity and efficiency of this event could not be elucidated. To further evaluate the function of Lhx2 expression during hematopoietic development, Lhx2 was introduced into an ES cell system where expression could be efficiently turned on. This approach revealed that Lhx2 induce self-renewal of distinct multipotent hematopoietic progenitor/stem cells present in the EB, with the ability to form HSC-like cell lines. The Lhx2 induced self-renewal is growth factor specific since stem cell factor and interleukin-6 are necessary and sufficient for this process. However, Lhx2 expression blocked erythroid differentiation and interfered with early ES cell commitment, indicating that the effect of Lhx2 is cell type specific. Since HSCs of early embryonic origin are inefficient in engrafting adult recipients upon transplantation, we wanted to address whether we could generate cell lines retaining this capacity by expression of Lhx2 in hematopoietic cells from adult bone marrow. This led to the generation of clonal and cytokine dependent HSC-like cell lines capable of generating erythroid, myeloid and lymphoid cells upon transplantation into lethally irradiated recipients. When transplanted into stem cell-deficient mice, they contributed to circulating erythrocytes for at least 18 months, revealing a remarkable potential for self-renewal and differentiation in vivo. However, expression of Lhx2 was maintained in vivo and most engrafted mice developed a transplantable myeloproliferative disorder resembling human chronic myeloid leukemia. Thus, elucidation of the mechanism for Lhx2 function in HSC-like cell lines would give insights into both normal and pathological regulation of HSCs. Down-regulation of Lhx2 expression in HSC-like cell lines with inducible Lhx2 expression led to rapid loss of stem cell characteristics and differentiation into various hematopoietic cell types. Thus, global gene expression analysis comparing Lhx2+ HSC-like cell lines to their Lhx2- progeny would give insights into the molecular basis for Lhx2 function in stem cells. A number of differentially expressed genes overlapped with previously reported HSC enriched genes, further emphasizing the resemblance between HSCs and the HSC-like cell lines also at the molecular level. Moreover, a number of genes were identified with functions or expression patterns related to Lhx2 in other organs. Collectively, these data suggest that these HSC-like cell lines represent a relevant model system for normal HSCs on the molecular and the functional level as well as for evaluating Lhx2 function in the development of various tissues in the embryo as well as in disease.

Hematopoietic stem cells

Lhx2

cell lines

self renewal

SCF

IL-6

chronic myeloproliferative disorder

global gene expression analysis

Molecular biology

Molekylärbiologi

Stem cell function and organ development : analysis of Lhx2 function in hematopoietic stem cells and eye development / Stamcellsfunktion och organutveckling : studier av blodstamceller och ögonutveckling

Dahl, Lina

January 2010

When a multicellular organism suffers damages to tissues/organs it heals itself by either substituting the lost cellular matrix by scar formation or by regenerating the lost tissue. Regeneration likely occurs by a recapitulation of the developmental process that formed the organ. Many processes regulating organ development are based on epithelial-mesenchymal interactions and a strict control of organ specific stem/progenitor cells. Elucidation of the molecular basis of these processes is therefore vital in order to develop novel therapies in regenerative medicine. The LIM homebox gene Lhx2 is interesting in this context since Lhx2 has been shown to be important for the formation of several organs by regulating epithelial-mesenchymal interactions and progenitor cell function. Targeted inactivation of Lhx2 leads to a lethal anemia due to malformed liver and severe neural abnormalities such as hypoplasia of the forebrain and anophtalmia. Thus, elucidation of the mechanisms of the function of Lhx2 in different organ systems would give important insights into the molecular mechanisms regulating epithelial-mesenchymal interactions and stem/progenitor cell function. To elucidate the function of Lhx2 in the hematopoietic system Lhx2 was initially expressed in hematopoietic progenitor cells derived from ES cells differentiated in vitro using retroviral vectors. This approach led to the generation of hematopoietic stem cell (HSC)-like cell lines suggesting that Lhx2 could impact HSC function. However neither the specificity nor the efficiency of the Lhx2-induced phenotype could be determined using this approach. To be able to elucidate the function of Lhx2 in the hematopoietic system, an ES cell line with inducible Lhx2 expression was generated. Lhx2 expression induces self-renewal of a distinct hematopoietic progenitor cell from which HSC-like cell lines were established. Down-regulation of Lhx2 in these HSC-like cell lines leads to a rapid loss of stem cell character, providing a good model to study the molecular function of Lhx2 in hematopoietic stem/progenitor cells. A global gene expression analysis was performed comparing the Lhx2+ stem cell population to the Lhx2- differentiated progeny. This approach identified genes putatively linked to self-renewal/differentiation of HSCs. A considerable proportion of the genes showed an overlapping gene expression pattern with Lhx2 expression in tissue of non-hematopoietic origin suggesting that Lhx2 function in stem/progenitor cells partly overlap with Lhx2 function during organ development. In order to define other Lhx2-dependent progenitor cell populations and to generate a tool to analyze the function of Lhx2 in organ development a new transgenic mouse model was generated. By using a specific part of the Lhx2 promoter to drive expression of Cre recombinase in vivo (Lhx2-Cre mice) we have been able to define the first eye committed progenitor cells in the forebrain. By using the Lhx2-Cre mice it will be possible to distinguish the function of genes during eye development from their function in the patterning of the forebrain e.g. the eye field transcription factors. Conditional inactivation of Lhx2 in these eye specific progenitor cells causes an immediate developmental arrest. The transgene is also active in Lhx2-/- embryonic forebrain, but re-expression of Lhx2 in Lhx2-/- progenitor cells only promote formation of retinal pigment epithelium cells. Analysis of genes expressed by the Lhx2+ stem cell population allowed us to define novel genes putatively linked to Lhx2 function in eye development. Thus, we have defined the progenitor cells in the forebrain committed to eye development and the expansion and patterning of these progenitors are dependent on Lhx2. Although commitment to eye development is Lhx2-independent, Lhx2 might be important for the acquisition of the oligopotent fate of these progenitor cells.

Lhx2

hematopoietic system

hematopoietic stem cell

progenitor

embryonic stem cell

embryoid body

eye development

forebrain

eye field transcription factor

Régulation de l’expression du gène Six6 par les facteurs de transcription Lhx2 et Pax6 dans le contexte des cellules souches rétiniennes

Champagne, Marie-Pier

08 1900

La rétinogésèse des vertébrés est la culmination de processus biologiques complexes parfaitement exécutés. Cette délicate orchestration est principalement contrôlée par les facteurs de transcription qui permettent aux progéniteurs rétiniens de proliférer, de s’auto-renouveler et de se différencier de façon appropriée. Les facteurs de transcription à homéodomaine sont les protéines qui sont responsables de la démarcation du site du primordium optique et participeront même à la différenciation tardive des différents types cellulaires de la rétine. Le contrôle génétique concernant l‘activation de l’expression de facteurs de transcription est peu connu. Nous avons étudié les séquences génomique avoisinant le gène Six6 afin d’identifier et mieux comprendre son promoteur. Des expériences d’immunoprécipitation de chromatine et des essais luciférases ont confirmé la liaison et la transactivation synergique du promoteur potentiel de Six6 par Lhx2 et Pax6 in vitro. Cette présente étude confirme et précise également le rôle de Lhx2 au niveau du développement précoce de l’oeil. La compréhension détaillée des réseaux génétiques régulant les progéniteurs rétiniens à former une rétine fonctionnelle est essentielle. En effet, lorsque ces connaissances seront acquises, nous serons en mesure d’appliquer les thérapies cellulaires pour rétablir les fonctions rétiniennes lors de pathologies dégénératives. / Vertebrate eye developement is the result of multiple perfectly executed biological process. This tight orchestration is principaly controled by transcription factors. Homeobox-containing transcription factors are expressed in the presumptive eye field and are required to initiate eye development and for final retinal cell differenciation. The genetic control of these transcription factors are poorly understood. We analysed Six6’s nearby genomic sequence to caracterise potential promoter regions. Chromatin immunoprecipitations and luciferase assays confirmed the binding and the in vitro synergic trans-activation of Six6 potential promoter by Lhx2 and Pax6. This study also demonstrate the contribution of Lhx2 for the establishment of presumptive retina field at the neural plate stage. The detailed knowledge of genetic networks regulating the formation of a fonctional retina by retinal progenitor is crucial. Indeed, when these mecanisms will be eluciated, we will be able to establish regenerative retinal cell therapy.

Rétine

Développement

Lhx2

Pax6

Six6

Progéniteur rétinien

Vésicule optique

Facteur de transcription

Homéodomaine

Retina

Homeobox

Development

Transcription factor

Optic vesicle

Caractérisation moléculaire du rôle de Lhx2 dans le développement de l'oeil et du cerveau

Tétreault, Nicolas

12 1900

Le développement du système nerveux central (SNC) chez les vertébrés est un processus d'une extrême complexité qui nécessite une orchestration moléculaire très précise. Certains gènes exprimés très tôt lors du développement embryonnaire sont d'une importance capitale pour la formation du SNC. Parmi ces gènes, on retrouve le facteur de transcription à Lim homéodomaine Lhx2. Les embryons de souris mutants pour Lhx2 (Lhx2-/-) souffre d'une hypoplasie du cortex cérébral, sont anophtalmiques et ont un foie de volume réduit. Ces embryons mutants meurent in utero au jour embryonnaire 16 (e16) dû à une déficience en érythrocytes matures. L'objectif principal de cette thèse est de caractériser le rôle moléculaire de Lhx2 dans le développement des yeux et du cortex cérébral. Lhx2 fait partie des facteurs de transcription à homéodomaine exprimé dans la portion antérieure de la plaque neurale avec Rx, Pax6, Six3. Le développement de l'oeil débute par une évagination bilatérale de cette région. Nous démontrons que l'expression de Lhx2 est cruciale pour les premières étapes de la formation de l'oeil. En effet, en absence de Lhx2, l'expression de Rx, Six3 et Pax6 est retardée dans la plaque neurale antérieure. Au stade de la formation de la vésicule optique, l'absence de Lhx2 empêche l'activation de Six6 (un facteur de transcription également essentiel au développement de l'œil). Nous démontrons que Lhx2 et Pax6 coopèrent en s'associant au promoteur de Six6 afin de promouvoir sa trans-activation. Donc, Lhx2 est un gène essentiel pour la détermination de l'identité rétinienne au niveau de la plaque neurale. Plus tard, il collabore avec Pax6 pour établir l'identité rétinienne définitive et promouvoir la prolifération cellulaire. De plus, Lhx2 est fortement exprimé dans le télencéphale, région qui donnera naissance au cortex cérébral. L'absence de Lhx2 entraîne une diminution de la prolifération des cellules progénitrices neurales dans cette région à e12.5. Nous démontrons qu'en absence de Lhx2, les cellules progénitrices neurales (cellules de glie radiale) se différencient prématurément en cellules progénitrices intermédiaires et en neurones post-mitotiques. Ces phénotypes sont corrélés à une baisse d'activité de la voie Notch. En absence de Lhx2, DNER (un ligand atypique de la voie Notch) est fortement surexprimé dans le télencéphale. De plus, Lhx2 et des co-répresseurs s'associent à la chromatine de la région promotrice de DNER. Nous concluons que Lhx2 permet l'activation de la voie Notch dans le cortex cérébral en développement en inhibant la transcription de DNER, qui est un inhibiteur de la voie Notch dans ce contexte particulier. Lhx2 permet ainsi la maintenance et la prolifération des cellules progénitrices neurales. / Central nervous system (CNS) development in vertebrates is an extremely complex process that requires tight molecular control. Some very early expressed genes during embryonic development are of tremendous importance for CNS development. Among those, we find the LIM homeodomain protein Lhx2. Embryos that lack Lhx2 (Lhx2-/-) suffer from cerebral cortex hypoplasia, are anophtalmic and have smaller liver. The mutant embryos die in utero at embryonic day 16 (e16) due to a deficit in mature erythrocytes. The principal objective of this thesis was to characterize the molecular function of Lhx2 in eye and cerebral cortex development. Lhx2 is a part of the homeodomain transcription factors expressed in the anterior neural plate along with Rx, Pax6 and Six3. Eye development starts by a bilateral evagination of this region. We show here that Lhx2 expression is crucial for the first steps of eye formation. Indeed, in absence of Lhx2, Rx, Six3 and Pax6 expression is delayed in the anterior neural plate. At the optic vesicle stage, Lhx2 mutation precludes the initiation of Six6 expression (an homeodomain transcription factor essential for eye development). We demonstrate that Lhx2 and Pax6 bind to Six6 promoter and cooperate for its trans‐activation. So, Lhx2 is essential for retinal identity determination in the neural plate. Later on, it cooperates with Pax6 to establish definitive retinal identity and promote cell proliferation. Lhx2 is strongly express in the telencephalon, the embryonic region that will give rise to cerebral cortex. Lhx2 ablation causes a decrease in neural progenitor cells proliferation in this region. We show that the lack of Lhx2 causes a premature differentiation of the radial glia cells into intermediate progenitors and post‐mitotic neurons. These phenotypes correlate with a decrease activity of the Notch pathway. In Lhx2-/- telencephalon, the atypical Notch‐ligand DNER is strongly overexpressed. Furthermore, Lhx2 and co‐repressors associate at the DNER promoter region. We conclude that Lhx2 allows Notch pathway activation in the developing cerebral cortex. It does so by inhibiting DNER transcription, which is a Notch pathway repressor in this particular context. Thus, Lhx2 allows the maintenance and the proliferation of neural progenitor cells.

Rétinogénèse

Vésicule optique

Télencephale

Neurogénèse

Voie Notch

Retinogenesis

Cellules souches/progenitrices neurales

Neurogenesis

Voie Notch

Optic Vesicle

DNER

Neural stem cells/progenitors

Pax6

Telencephalon

Lhx2

Notch Pathway

The Role of Lhx2 During Organogenesis : - Analysis of the Hepatic, Hematopoietic and Olfactory Systems

Kolterud, Åsa

January 2004

During embryonic development a variety of tissues and organs such as the lung, eye, and kidney are being formed. The generation of functional organs is regulated by reciprocal cell-cell interactions. Via the secretion of soluble molecules one type of cells affect the fate of their neighboring cells. A central issue in organogenesis is how a cell interprets such extrinsic signals and adopts a specific fate, and how the cell in response to this signal establishes reciprocal signaling. Transcription factors play a critical role in this process and my thesis focuses on the role of the LIM-homeodomain transcription factor, Lhx2, in the development of three different organ systems, the liver, the hematopoietic system and the olfactory system. The liver is formed from endoderm of the ventral foregut and mesenchyme of the septum transversum (st) and its development depends upon signaling interactions between these two tissues. As the liver becomes a distinct organ it is colonized by hematopoietic cells and serves as hematopoietic organ until birth. The fetal liver provides a microenvironment that supports the expansion of the entire hematopoietic system (HS) including the hematopoietic stem cells (HSCs). Liver development in Lhx2-/- embryos is disrupted leading to a lethal anemia due to insufficient support of hematopoiesis. To further investigate the role of Lhx2 in liver development I analyzed gene expression from the Lhx2 locus during liver development in wild-type and Lhx2-/- mice. Lhx2 is expressed in the liver associated st mesenchymal cells that become integrated in the liver and contribute to a subpopulation of hepatic stellate cells in adult liver. Lhx2 is not required for the formation of these mesenchymal cells, suggesting that the phenotype in Lhx2-/- livers is due to the presence of defective mesenchymal cells. The putative role of Lhx2 in the expansion of the HS was examined by introducing Lhx2 cDNA into embryonic stem cells differentiated in vitro. This approach allowed for the generation of immortalized multipotent hematopoietic progenitor cell (HPC) lines that share many characteristics with normal HSCs. The Lhx2-dependent generation of HSC-like cell lines suggests that Lhx2 plays a role in the maintenance and/or expansion of the HS. To isolate genes putatively linked to Lhx2 function, genes differentially expressed in the HPC lines were isolated using a cDNA subtraction approach. This allowed for the identification of a few genes putatively linked to Lhx2 function, as well as several stem cell-specific genes. The antagonist of Wnt signalling, Dickkopf-1 (Dkk-1), was identified in the former group of genes as it showed a similar expression pattern in the fetal liver, as that of Lhx2 and expression of Dkk-1 in fetal liver and in HPC lines appeared to be regulated by Lhx2. This suggests that Dkk-1 plays a role in liver development and/or HSC physiology during embryonic development. During development of the olfactory epithelium (OE) neuronal progenitors differentiate into mature olfactory sensory neurons (OSNs) that are individually specified into over a thousand different subpopulations, each expressing a unique odorant receptor (OR) gene. The expression of Lhx2 in olfactory neurons suggested a potential role for Lhx2 in the development of OSNs. To address this OE from Lhx2-/- and wild-type mice was compared. In the absence of functional Lhx2 neuronal differentiation was arrested prior to onset of OR expression. Lhx2 is thus required for the development of OSN progenitors into functional, individually specified OSNs. Thus, Lhx2 trigger a variety of cellular responses in different organ systems that play important roles in organ development in vivo and stem cell expansion in vitro.

Developmental biology

LIM-homeobox gene

Lhx2

fetal liver

hepatic stellate cells

hematopoietic stem cells

septum transversum

self-renewal

odorant receptor genes

olfactory epithelium

olfactory sensory neuron

Utvecklingsbiologi

Developmental biology

Utvecklingsbiologi

Caractérisation moléculaire du rôle de Lhx2 dans le développement de l'oeil et du cerveau

Tétreault, Nicolas

12 1900

Le développement du système nerveux central (SNC) chez les vertébrés est un processus d'une extrême complexité qui nécessite une orchestration moléculaire très précise. Certains gènes exprimés très tôt lors du développement embryonnaire sont d'une importance capitale pour la formation du SNC. Parmi ces gènes, on retrouve le facteur de transcription à Lim homéodomaine Lhx2. Les embryons de souris mutants pour Lhx2 (Lhx2-/-) souffre d'une hypoplasie du cortex cérébral, sont anophtalmiques et ont un foie de volume réduit. Ces embryons mutants meurent in utero au jour embryonnaire 16 (e16) dû à une déficience en érythrocytes matures. L'objectif principal de cette thèse est de caractériser le rôle moléculaire de Lhx2 dans le développement des yeux et du cortex cérébral. Lhx2 fait partie des facteurs de transcription à homéodomaine exprimé dans la portion antérieure de la plaque neurale avec Rx, Pax6, Six3. Le développement de l'oeil débute par une évagination bilatérale de cette région. Nous démontrons que l'expression de Lhx2 est cruciale pour les premières étapes de la formation de l'oeil. En effet, en absence de Lhx2, l'expression de Rx, Six3 et Pax6 est retardée dans la plaque neurale antérieure. Au stade de la formation de la vésicule optique, l'absence de Lhx2 empêche l'activation de Six6 (un facteur de transcription également essentiel au développement de l'œil). Nous démontrons que Lhx2 et Pax6 coopèrent en s'associant au promoteur de Six6 afin de promouvoir sa trans-activation. Donc, Lhx2 est un gène essentiel pour la détermination de l'identité rétinienne au niveau de la plaque neurale. Plus tard, il collabore avec Pax6 pour établir l'identité rétinienne définitive et promouvoir la prolifération cellulaire. De plus, Lhx2 est fortement exprimé dans le télencéphale, région qui donnera naissance au cortex cérébral. L'absence de Lhx2 entraîne une diminution de la prolifération des cellules progénitrices neurales dans cette région à e12.5. Nous démontrons qu'en absence de Lhx2, les cellules progénitrices neurales (cellules de glie radiale) se différencient prématurément en cellules progénitrices intermédiaires et en neurones post-mitotiques. Ces phénotypes sont corrélés à une baisse d'activité de la voie Notch. En absence de Lhx2, DNER (un ligand atypique de la voie Notch) est fortement surexprimé dans le télencéphale. De plus, Lhx2 et des co-répresseurs s'associent à la chromatine de la région promotrice de DNER. Nous concluons que Lhx2 permet l'activation de la voie Notch dans le cortex cérébral en développement en inhibant la transcription de DNER, qui est un inhibiteur de la voie Notch dans ce contexte particulier. Lhx2 permet ainsi la maintenance et la prolifération des cellules progénitrices neurales. / Central nervous system (CNS) development in vertebrates is an extremely complex process that requires tight molecular control. Some very early expressed genes during embryonic development are of tremendous importance for CNS development. Among those, we find the LIM homeodomain protein Lhx2. Embryos that lack Lhx2 (Lhx2-/-) suffer from cerebral cortex hypoplasia, are anophtalmic and have smaller liver. The mutant embryos die in utero at embryonic day 16 (e16) due to a deficit in mature erythrocytes. The principal objective of this thesis was to characterize the molecular function of Lhx2 in eye and cerebral cortex development. Lhx2 is a part of the homeodomain transcription factors expressed in the anterior neural plate along with Rx, Pax6 and Six3. Eye development starts by a bilateral evagination of this region. We show here that Lhx2 expression is crucial for the first steps of eye formation. Indeed, in absence of Lhx2, Rx, Six3 and Pax6 expression is delayed in the anterior neural plate. At the optic vesicle stage, Lhx2 mutation precludes the initiation of Six6 expression (an homeodomain transcription factor essential for eye development). We demonstrate that Lhx2 and Pax6 bind to Six6 promoter and cooperate for its trans‐activation. So, Lhx2 is essential for retinal identity determination in the neural plate. Later on, it cooperates with Pax6 to establish definitive retinal identity and promote cell proliferation. Lhx2 is strongly express in the telencephalon, the embryonic region that will give rise to cerebral cortex. Lhx2 ablation causes a decrease in neural progenitor cells proliferation in this region. We show that the lack of Lhx2 causes a premature differentiation of the radial glia cells into intermediate progenitors and post‐mitotic neurons. These phenotypes correlate with a decrease activity of the Notch pathway. In Lhx2-/- telencephalon, the atypical Notch‐ligand DNER is strongly overexpressed. Furthermore, Lhx2 and co‐repressors associate at the DNER promoter region. We conclude that Lhx2 allows Notch pathway activation in the developing cerebral cortex. It does so by inhibiting DNER transcription, which is a Notch pathway repressor in this particular context. Thus, Lhx2 allows the maintenance and the proliferation of neural progenitor cells.

Rétinogénèse

Vésicule optique

Télencephale

Neurogénèse

Voie Notch

Retinogenesis

Cellules souches/progenitrices neurales

Neurogenesis

Voie Notch

Optic Vesicle

DNER

Neural stem cells/progenitors

Pax6

Telencephalon

Lhx2

Notch Pathway